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Last Updated :2024/09/26

研究者情報

マスター

アカウント(マスター)

  • 氏名

    森川 正章(モリカワ マサアキ), モリカワ マサアキ

所属(マスター)

  • 地球環境科学研究院 環境生物科学部門 環境分子生物学分野

所属(マスター)

  • 地球環境科学研究院 環境生物科学部門 環境分子生物学分野

独自項目

syllabus

  • 2021, 環境分子生物学特論Ⅰ, Advanced Course in Environmental Molecular Biology I, 修士課程, 環境科学院, 微生物学、極限環境、分子生物学、生態学、分子昆虫学、哺乳類、発生生理化学、生化学 Microbiology,extremophiles,molecular biology,ecology,molecular Entomology, development and biochemistry in mammals
  • 2021, 大学院共通授業科目(教育プログラム):JICA開発大学院連携プログラム環境科学, Inter-Graduate School Classes(Educational Program):JICA Development Studies Program for Environmental Science, 修士課程, 大学院共通科目, 再生可能エネルギー、賦存量、太陽エネルギー、風力、地熱・温泉熱、バイオマス、水力、水・エネルギー・食料ネクサス、トレードオフ、生態系、温室効果ガス、化石燃料、環境、光合成 Renewable energy, Potential, Solar energy, Wind power, Geothermal and hot spring water heat, Biomass, Hydropower, Water-energy-food nexus, Trade-off, Ecosystem, Greenhouse gas, Fossil fuels, Environment, Photosynthesis
  • 2021, 再生可能エネルギー総論, Introduction to Renewable Energy, 修士課程, 環境科学院, 再生可能エネルギー、賦存量、太陽エネルギー、風力、地熱・温泉熱、バイオマス、水力、水・エネルギー・食料ネクサス、トレードオフ、生態系、温室効果ガス、化石燃料、環境、光合成 Renewable energy, Potential, Solar energy, Wind power, Geothermal and hot spring water heat, Biomass, Hydropower, Water-energy-food nexus, Trade-off, Ecosystem, Greenhouse gas, Fossil fuels, Environment, Photosynthesis
  • 2021, 分子生物学基礎論, Fundamental Course in Molecular Biology, 修士課程, 環境科学院, 分子生物学,転写,翻訳,微生物の群集構造解析,微生物の呼吸活性,電子顕微鏡観察,遺伝子操作,バイオフィルム形成,植物ストレス耐性,バイオセンサー,昆虫免疫系,昆虫体表脂質, 動物細胞 molecular biology, transcription, translation, bacterial culture, bacterial community structure analysis, bacterial respiration activity, electron microscopic observation, genetic manipulation, biofilm formation, stress tolerance of plants, biosensor, insect immune system, insect body surface lipids, animal cells
  • 2021, 科学・技術の世界(1単位), The World of Science and Technology, 学士課程, 全学教育, 現代生物科学,21世紀に生物科学が解決しなければならない課題,生体高分子,細胞の構造と機能,エネルギー代謝,細胞の成長と分裂,遺伝現象と遺伝子発現制御
  • 2021, 機能生物学Ⅰ, Functional Biology I, 学士課程, 理学部, 遺伝子、メンデルの法則、組換え、変異、ゲノム、集団、遺伝的浮動、自然選択、進化、系統樹、代謝、同化と異化、呼吸と発酵、光合成
  • 2021, 環境生物学Ⅰ, Environmental Biology I, 学士課程, 理学部, 環境で生かされる生物そして環境を創造する生物?環境と生物の不可避な相互関係
  • 2021, 生物学Ⅰ, Biology I, 学士課程, 全学教育, 生体高分子,細胞の構造と機能,エネルギー代謝,細胞の成長と分裂,遺伝現象と遺伝子発現制御
  • 2021, 一般教育演習(フレッシュマンセミナー), Freshman Seminar, 学士課程, 全学教育, 極限環境、好熱菌、低温菌、好塩菌、好酸性菌、好アルカリ性菌、メタン生成菌、地下微生物、微生物学基礎
  • 2021, 環境生物学Ⅰ, Environmental Biology I, 学士課程, 理学部
  • 2021, ISP生物科学実習Ⅱ・a, ISP Biological Laboratory Course II・a, 学士課程, 理学部, 生物の環境応答と適応
  • 2021, ISP生物科学実習Ⅱ・b, ISP Biological Laboratory Course II・b, 学士課程, 理学部, 生物の環境応答と適応
  • 2021, 環境生物学実習, Laboratory Course in Environmental Biology, 学士課程, 理学部, 生物の環境応答と適応

researchmap

プロフィール情報

学位

  • 工学博士(1994年10月 大阪大学)
  • 名誉博士(生物科学)(2022年10月 タイ国カセサート大学)

プロフィール情報

  • 公開用メールアドレス

    morikawaees.hokudai.ac.jp

  • 森川, モリカワ

  • 正章, マサアキ

  • ID各種

    200901006119139020

対象リソース

業績リスト

研究キーワード

  • 環境バイオテクノロジー   極限生命工学   環境分子微生物学   Extremity Life Science   Envionmental Molecular Microbiology   

研究分野

  • 環境・農学 / 自然共生システム / 植物成長促進細菌
  • ライフサイエンス / 応用微生物学

経歴

  • 2023年04月 - 現在 大阪大学生物工学国際交流センター 招聘教授
  • 2004年05月 - 現在 北海道大学教授 大学院地球環境科学研究院 環境生物科学部門
  • 2004年05月 - 現在 Professor,Faculty of Environmental Earth Science, Hokkaido University
  • 2020年08月 - 2026年09月 JST/JICA-SATREPS Project Leader
  • 2020年08月 - 2026年09月 地球規模課題対応国際科学技術協力プログラム SATREPS (JST/JICA) 研究代表者
  • 2011年10月 - 2020年03月 JST-ALCA Project Leader
  • 2011年10月 - 2020年03月 先端的低炭素化技術開発 JST-ALCA 研究代表者
  • 2004年05月 - 2006年03月 北海道大学教授 大学院地球環境科学研究科 生態環境科学専攻
  • 1995年07月 - 2004年04月 大阪大学助教授 大学院工学研究科 物質・生命工学専攻
  • 1995年07月 - 2004年04月 Associate Professor,Graduate School of Engineering, Osaka University
  • 2001年05月 - 2002年03月 Visiting Researcher, Harvard Medical School
  • 2001年 - 2002年 文部科学省長期在外研究員(ハーバード大学医学部 微生物学・分子遺伝学教室)-2002. 3.
  • 1996年 - 2001年 生物系特定産業技術研究推進機構プログラム 総括研究代表者
  • 1996年 - 2001年 Project Leader,BRAIN
  • 1990年04月 - 1995年06月 大阪大学助手 工学部発酵工学科
  • 1990年04月 - 1995年06月 Research Associate, Osaka University
  • 1985年04月 - 1989年03月 日清製油株式会社研究所 研究員
  • 1985年04月 - 1989年03月 Researcher,The Nisshin Oil Mills Co. Ltd.
  • 1986年04月 - 1988年03月 工業技術院化学技術研究所(出向)
  • 1986年04月 - 1988年03月 Visiting Researcher,MITI

学歴

  • 1983年04月 - 1985年03月   大阪大学   大学院工学研究科   発酵工学専攻 博士前期課程
  • 1983年04月 - 1985年03月   大阪大学
  • 1979年04月 - 1983年03月   大阪大学   工学部   発酵工学科
  • 1979年04月 - 1983年03月   大阪大学
  • 1976年04月 - 1979年03月   府立生野高等学校

委員歴

  • 2023年06月 - 現在   環境バイオテクノロジー学会   会長
  • 2007年06月 - 現在   環境バイオテクノロジー学会   理事
  • 2005年09月 - 現在   パキスタン高等教育委員会   外国人専門委員
  • 1998年04月 - 現在   バイオインダストリー協会 新資源生物変換研究会   幹事
  • 2015年06月 - 2023年05月   環境バイオテクノロジー学会   副会長

受賞

  • 2022年11月 日本水処理生物学会 第25回論文賞
     Isolation and Characterization of Novel Plant Growth-Promoting Bacteria from the Fronds of Duckweed 
    受賞者: 岩下智貴;田中靖浩;玉木秀幸;米田;牧野彩花;遠山忠;鎌形洋一;森川正章;森一博
  • 2022年10月 タイ国カセサート大学 名誉博士号
  • 2019年11月 日本水処理生物学会 第22回論文賞
     Biomass production and nutrient removal through cultivation of Euglena gracilis in domestic wastewater 
    受賞者: 黒田真史;堀野太郎;井上大介;森川正章;池 道彦
  • 2017年 ISCDRA First Place “2017 Knowing to Growing Duckweed Application Award”
     Evaluation of environmental bacterial communities as a factor affecting the growth of duckweed Lemna minor 
    受賞者: H. Ishizawa;M. Kuroda;M. Morikawa;M. Ike
  • 2011年 日本農芸化学会 第8回農芸化学研究企画賞
  • 2007年 天野エンザイム 第8回 酵素応用シンポジウム研究奨励賞
  • 2003年 バイオインダストリー協会 奨励賞
     発酵と代謝
  • 1999年 日本生物工学会 第7回生物工学論文賞
     
    受賞者: 森川 正章;岩佐 毅;柳田 祥三;今中 忠行;阪大院;工;京大院
  • 1994年 日本生物工学会 第2回生物工学論文賞
     
    受賞者: 森川 正章;今中 忠行
  • 1993年 日本生物工学会 第1回生物工学論文賞
     
    受賞者: 森川 正章;伊東 幹人;今中 忠行

論文

  • Kengo Kubota, Takashi Otani, Teruki Hariu, Takumi Jin, Tadashi Tagawa, Masaaki Morikawa, Yu-You Li
    Journal of Water Process Engineering 2024年08月 [査読有り]
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  • Tadashi Toyama, Maki Kobayashi, Rubiy Atno, Masaaki Morikawa, Kazuhiro Mori
    Chemosphere 361 142592 - 142592 2024年08月 [査読有り][通常論文]
     
    The phyto-Fenton process, which generates hydroxyl radicals through Fenton and Fenton-like reactions using plant-derived hydrogen peroxide (H2O2) and ferrous iron (Fe (II)) can degrade organic pollutants. Duckweed, an aquatic plant, is promising for a co-beneficial phytoremediation process that combines wastewater treatment and biomass production for biofuel feedstock. However, the phyto-Fenton process using duckweed has not been extensively studied. Because sulfamethoxazole (SMX), a major antibiotic, is distributed widely and is an emerging contaminant, its effective removal from contaminated water is necessary. The present study investigated the possibility of the simultaneous efficient removal of SMX from polluted water and biomass production for fuel feedstock by the phyto-Fenton process using duckweed. This is the first attempt to demonstrate the co-benefits of SMX removal and biomass production using duckweed. Intracellular H2O2 was produced using four duckweeds, Lemna aequinoctialis, L. minor, Landolina punctata, and Spirodela polyrhiza, in the range of 16.7-24.6 μ mol g-1 fresh weight, and extracellular H2O2 was released into the water phase. Consequently, duckweed could be used as an H2O2 supply source for the phyto-Fenton process. Specifically, 0.5 g fresh duckweed almost completely eliminated 1 mg L-1 SMX after 5 d in 50 mL sterile modified Hoagland solution containing 10 mM Fe (II). Fe (II)-dependent elimination of SMX indicated the occurrence of phyto-Fenton reaction. The phyto-Fenton process using duckweed effectively removed SMX. S. polyrhiza duckweed similarly removed 1 mg L-1 SMX even in sewage effluent containing other organic contaminants. During this treatment, duckweed biomass was generated at 7.95 g dry weight m-2 d-1, which was converted into methane at 353 normal liters CH4 kg-1 volatile solids by anaerobic digestion. For the first time, this study clearly demonstrates the potential for simultaneous SMX removal and biomass production from SMX-contaminated wastewater using duckweed.
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  • Tanasap Nithimethachoke, Chanita Boonmak, Masaaki Morikawa
    Extremophiles : life under extreme conditions 28 1 18 - 18 2024年02月14日 [査読有り]
     
    We have accidentally found that a thermophilic Geobacillus kaustophilus HTA426 is capable of degrading alkanes although it has no alkane oxygenating enzyme genes. Our experimental results revealed that a putative ribonucleotide reductase small subunit GkR2loxI (GK2771) gene encodes a novel heterodinuclear Mn-Fe alkane monooxygenase/hydroxylase. GkR2loxI protein can perform two-electron oxidations similar to homonuclear diiron bacterial multicomponent soluble methane monooxygenases. This finding not only answers a long-standing question about the substrate of the R2lox protein clade, but also expands our understanding of the vast diversity and new evolutionary lineage of the bacterial alkane monooxygenase/hydroxylase family.
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  • Yasuhiro Tanaka, Erina Tozawa, Tomoki Iwashita, Yosuke Morishita, Hideyuki Tamaki, Tadashi Toyama, Masaaki Morikawa, Yoichi Kamagata, Kazuhiro Mori
    Microbes and environments 39 3 2024年 
    The "duckweed-microbes co-cultivation method" is a microbial isolation technique that effectively recovers diverse microbes, including rarely cultivated bacterial phyla, from environmental samples. In this method, aseptic duckweed and microbes collected from an environmental sample are co-cultivated for several days, and duckweed-associated microbes are then isolated from its roots using a conventional agar plate-based cultivation method. We herein propose several improvements to the method in order to specifically obtain members of the rarely cultivated bacterial phylum, Verrucomicrobiota. In systems using river water as the inoculum, the marked enrichment of Verrucomicrobiota was observed after 10 days of co-cultivation, particularly in the roots and co-cultivated media. We also successfully isolated 44 strains belonging to subdivisions 1, 3, and 4 of the phylum Verrucomicrobiota from these systems. This was achieved by changing the concentration of nitrogen in the co-cultivation medium, which is known to affect duckweed growth and/or metabolism, and by subjecting the fronds and co-cultivated media as well as the roots after co-cultivation to microbial isolation.
  • Chanita Boonmak, Sirapat Kettongruang, Buranaporn Buranathong, Masaaki Morikawa, Kannika Duangmal
    Archives of microbiology 206 1 43 - 43 2023年12月26日 [査読有り]
     
    Duckweed has been highlighted as an invaluable resource because of its abilities to remove nitrogen and phosphorus from wastewater coupling with the production of high starch/protein-containing plant biomass. Duckweed recruits microbes and particularly forms a stable "core" bacterial microbiota, which greatly reduces the colonization efficiency of plant growth-promoting bacteria (PGPB). In this study, natural duckweeds were enriched in a sterilized-partially treated wastewater effluent from a poultry farm. After 24 days of cultivation, the duckweed-associated bacteria (DAB) were isolated and evaluated for their plant growth-promoting (PGP) potentials by co-cultivation with axenic Spirodela polyrhiza. Ten species were found in more than one location and could be considered candidates for the stable "core" DAB. Among them, all isolates of Acinetobacter soli, Acidovorax kalamii, Brevundimonas vesicularis, Pseudomonas toyotomiensis, and Shinella curvata increased duckweed growth in Hoagland medium. The highest PGP ability was observed in Sh. curvata W12-8 (with EPG value of 208.72%), followed by Paracoccus marcusii W7-16 (171.31%), Novosphingobium subterraneum W5-13 (156.96%), and Ac. kalamii W7-18 (156.96%). However, the highest growth promotion in the wastewater was observed when co-cultured with W7-16, which was able to increase biomass dry weight and root length of duckweed by 3.17 and 2.26 folds, respectively.
  • Kensuke Kaneko, Daiki Kobayashi, Shiro Masaki, Kenji Washio, Masaaki Morikawa, Tatsufumi Okino
    JOURNAL OF APPLIED PHYCOLOGY 2023年04月 [査読有り]
     
    The gene encoding vanadium-dependent bromoperoxidase (V-BPO) was cloned for the first time from the red alga Laurencia saitoi, which produces pharmaceutically promising brominated diterpenoids and triterpenoids. The molecular weight of V-BPO from L. saitoi (LsVBPO1) was the highest (77.0 kDa) among previously reported V-BPOs from Laurencia with a peptide insertion Asn194-Ser221 containing short Gln repeats. It shares approximately 60% amino acid sequence identity with V-BPOs from L. nipponica (LnVBPO1 and LnVBPO2) and L. okamurae (LoVBPO1a and LoVBPO2a). Heterologously expressed LsVBPO1 in Escherichia coli was partially purified and exhibited low but significant bromination activity of 38 U mg(-1) protein using monochlorodimedone. The pH optimum was 8.0, which was more alkaline than that for LnVBPOs and LoVBPO2a (pH 7.0). The K-m for H2O2 was 0.04 mM, comparable to LnVBPO1 (0.026 mM), LnVBPO2 (0.025 mM), and LoVBPO2a (0.014 mM). LsVPBO1 retained its bromination activity until 45 degrees C for 20 min. When incubated at 55 degrees C for 20 min, catalytic activity decreased rapidly, as shown for LnVBPO1 and LoVBPO2a (retained at 45 degrees C, decreased at 55 degrees C) and LnVBPO2 (retained at 55 degrees C, decreased at 65 degrees C). Unlike other V-BPOs from Laurencia (LnVBPO1, LnVBPO2, and LoVBPO2a), dialysis and concentration during purification process were rapidly inactivated LsVBPO1, suggesting its structural instability.
  • Hidehiro Ishizawa, Yukiko Kaji, Yuki Shimizu, Masashi Kuroda, Daisuke Inoue, Ayaka Makino, Ryosuke Nakai, Hideyuki Tamaki, Masaaki Morikawa, Michihiko Ike
    Journal of Water and Environment Technology 21 1 49 - 58 2023年01月 [査読有り]
  • Takafumi Ishikawa, Kenji Washio, Kensuke Kaneko, Xiao Rong Tang, Masaaki Morikawa, Tatsufumi Okino
    Applied Phycology 3 1 120 - 131 2022年12月31日 [査読有り]
  • Sajjad Kamal Shuvro, Rahul Jog, Masaaki Morikawa
    Plant Growth Regulation 2022年09月21日 [査読有り]
  • Chin-Soon Phan, Jakia Jerin Mehjabin, Andrea Roxanne J. Anas, Masahiro Hayasaka, Reiko Onoki, Juting Wang, Taiki Umezawa, Kenji Washio, Masaaki Morikawa, Tatsufumi Okino
    Journal of Natural Products 2022年08月10日 [査読有り]
  • Ayaka Makino, Ryosuke Nakai, Yasuko Yoneda, Tadashi Toyama, Yasuhiro Tanaka, Xian-Ying Meng, Kazuhiro Mori, Michihiko Ike, Masaaki Morikawa, Yoichi Kamagata, Hideyuki Tamaki
    Microorganisms 10 8 1564 - 1564 2022年08月03日 [査読有り]
     
    Plant growth-promoting bacteria (PGPB) can exert beneficial growth effects on their host plants. Little is known about the phylogeny and growth-promoting mechanisms of PGPB associated with aquatic plants, although those of terrestrial PGPB have been well-studied. Here, we report four novel aquatic PGPB strains, MRB1–4 (NITE P-01645–P-01648), for duckweed Lemna minor from our rhizobacterial collection isolated from Lythrum anceps. The number of L. minor fronds during 14 days co-culture with the strains MRB1–4 increased by 2.1–3.8-fold, compared with an uninoculated control; the plant biomass and chlorophyll content in co-cultures also increased. Moreover, all strains possessed an indole-3-acetic acid production trait in common with a plant growth-promoting trait of terrestrial PGPB. Phylogenetic analysis showed that three strains, MRB-1, -3, and -4, were affiliated with known proteobacterial genera (Bradyrhizobium and Pelomonas); this report is the first to describe a plant-growth promoting activity of Pelomonas members. The gammaproteobacterial strain MRB2 was suggested to be phylogenetically novel at the genus level. Under microscopic observation, the Pelomonas strain MRB3 was epiphytic and adhered to both the root surfaces and fronds of duckweed. The duckweed PGPB obtained here could serve as a new model for understanding unforeseen mechanisms behind aquatic plant-microbe interactions.
  • Kyosuke Yamamoto, Yasuko Yoneda, Ayaka Makino, Yasuhiro Tanaka, Xian-Ying Meng, Junko Hashimoto, Kazuo Shin-Ya, Noriyuki Satoh, Manabu Fujie, Tadashi Toyama, Kazuhiro Mori, Michihiko Ike, Masaaki Morikawa, Yoichi Kamagata, Hideyuki Tamaki
    Microbiology resource announcements 11 2 e0045521  2022年02月17日 
    We report a complete genome sequence of a novel bacterial isolate, strain TBR-22, belonging to the class Vicinamibacteria of the phylum Acidobacteria, which was isolated from duckweed fronds. The genome expands our knowledge of the lifestyle of this abundant but rarely characterized phylum.
  • Kyosuke Yamamoto, Yasuko Yoneda, Ayaka Makino, Yasuhiro Tanaka, Xian-Ying Meng, Junko Hashimoto, Kazuo Shin-Ya, Noriyuki Satoh, Manabu Fujie, Tadashi Toyama, Kazuhiro Mori, Michihiko Ike, Masaaki Morikawa, Yoichi Kamagata, Hideyuki Tamaki
    Microbiology resource announcements 11 1 e0045321  2022年01月20日 
    Here, we report a draft genome sequence of a bacterial strain, F-183, isolated from a duckweed frond. Strain F-183 belongs to the family Bryobacteraceae of the phylum Acidobacteria, and its genomic information would contribute to understanding the ecophysiology of this abundant but rarely characterized phylum.
  • Tadashi Toyama, Kazuhiro Mori, Yasuhiro Tanaka, Michihiko Ike, Masaaki Morikawa
    MOLECULAR PLANT-MICROBE INTERACTIONS 35 1 28 - 38 2022年01月 [査読有り]
     
    Duckweeds (Lemnaceae) are representative producers in fresh aquatic ecosystems and also yield sustainable biomass for animal feeds, human foods, and biofuels, and contribute toward effective wastewater treatment; thus, enhancing duckweed productivity is a critical challenge. Plant-growth -promoting bacteria (PGPB) can improve the productivity of terrestrial plants; however, duckweed-PGPB interactions remain unclear and no previous study has investigated the molecular mechanisms underlying duckweed-PGPB interaction. Herein, a PGPB, Ensifer sp. strain SP4, was newly isolated from giant duckweed (Spirodela polyrhiza), and the interactions between S. polyrhiza and SP4 were investigated through physiological, biochemical, and metabolomic analyses. In S. polyrhiza and SP4 coculture, SP4 increased the nitrogen (N), chlorophyll, and ribulose-1,5-bisphosphate carboxylase/oxygenase (RuBisCO) contents and the photosynthesis rate of S. polyrhiza by 2.5-, 2.5-, 2.7-, and 2.4-fold, respectively. Elevated photosynthesis increased the relative growth rate and biomass productivity of S. polyrhiza by 1.5 and 2.7-fold, respectively. Strain SP4 significantly altered the metabolomic profile of S. polyrhiza, especially its amino acid profile. N stable isotope analysis revealed that organic N compounds were transferred from SP4 to S. polyrhiza. These N compounds, particularly glutamic acid, possibly triggered the increase in photosynthetic and growth activities. Accordingly, we propose a new model for the molecular mechanism underlying S. polyrhiza growth promotion by its associated bacteria Ensifer sp. SP4, which occurs through enhanced N compound metabolism and photosynthesis. Our findings show that Ensifer sp. SP4 is a promising PGPB for increasing biomass yield, wastewater purification activity, and CO2 capture of S. polyrhiza.
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  • Construction of a black-dirt formation model using microorganisms obtained from the toilet bowl
    Michitaka Muramatsu, Chie Ito, Kazuma Niizeki, Mitsuhiro Gomi, Masaaki Morikawa
    Journal of Environmental Biotechnology 21 1 63 - 66 2021年07月 [査読有り][通常論文]
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  • Yasuko Yoneda, Kyosuke Yamamoto, Ayaka Makino, Yasuhiro Tanaka, Xian-Ying Meng, Junko Hashimoto, Kazuo Shin-ya, Noriyuki Satoh, Manabu Fujie, Tadashi Toyama, Kazuhiro Mori, Michihiko Ike, Masaaki Morikawa, Yoichi Kamagata, Hideyuki Tamaki
    MICROORGANISMS 9 6 2021年06月 [査読有り][通常論文]
     
    Duckweeds are small, fast growing, and starch- and protein-rich aquatic plants expected to be a next generation energy crop and an excellent biomaterial for phytoremediation. Despite such an importance, very little is known about duckweed-microbe interactions that would be a key biological factor for efficient industrial utilization of duckweeds. Here we first report the duckweed growth promoting ability of bacterial strains belonging to the phylum Acidobacteria, the members of which are known to inhabit soils and terrestrial plants, but their ecological roles and plant-microbe interactions remain largely unclear. Two novel Acidobacteria strains, F-183 and TBR-22, were successfully isolated from wild duckweeds and phylogenetically affiliated with subdivision 3 and 6 of the phylum, respectively, based on 16S rRNA gene sequence analysis. In the co-culture experiments with aseptic host plants, the F-183 and TBR-22 strains visibly enhanced growth (frond number) of six duckweed species (subfamily Lemnoideae) up to 1.8-5.1 times and 1.6-3.9 times, respectively, compared with uninoculated controls. Intriguingly, both strains also increased the chlorophyll content of the duckweed (Lemna aequinoctialis) up to 2.4-2.5 times. Under SEM observation, the F-183 and TBR-22 strains were epiphytic and attached to the surface of duckweed. Taken together, our findings suggest that indigenous plant associated Acidobacteria contribute to a healthy growth of their host aquatic plants.
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  • Yeni Khairina, Rahul Jog, Chanita Boonmak, Tadashi Toyama, Tokitaka Oyama, Masaaki Morikawa
    Chemosphere 268 129247 - 129247 2021年04月 [査読有り][通常論文]
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  • Hitoshi Nakamoto, Yuhei Yokoyama, Takahiro Suzuki, Yuri Miyamoto, Takashi Fujishiro, Masaaki Morikawa, Yoshihiko Miyata
    The Journal of Biochemistry 170 2 255 - 264 2021年03月26日 [査読有り][通常論文]
     
    Abstract Heat shock protein 90 (Hsp90) is essential for eukaryotic cells, whereas bacterial homologs play a role under stresses and in pathogenesis. Identifying species-specific Hsp90 inhibitors is challenging because Hsp90 is evolutionarily conserved. We found that a cyclic lipopeptide surfactin inhibits the ATPase activity of Hsp90 from the cyanobacterium Synechococcus elongatus (S.elongatus) PCC 7942 but does not inhibit Escherichia coli (E.coli), yeast and human Hsp90s. Molecular docking simulations indicated that surfactin could bind to the N-terminal dimerization interface of the cyanobacterial Hsp90 in the ATP- and ADP-bound states, which provided molecular insights into the species-selective inhibition. The data suggest that surfactin inhibits a rate-limiting conformational change of S.elongatus Hsp90 in the ATP hydrolysis. Surfactin also inhibited the interaction of the cyanobacterial Hsp90 with a model substrate, and suppressed S.elongatus growth under heat stress, but not that of E.coli. Surfactin did not show significant cellular toxicity towards mammalian cells. These results indicate that surfactin inhibits the cellular function of Hsp90 specifically in the cyanobacterium. The present study shows that a cyclic peptide has a great specificity to interact with a specific homolog of a highly conserved protein family.
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  • Natwara Amatyakul, Suthep Thaniyavarn, Masaaki Morikawa, Jiraporn Thaniyavarn
    The Journal of general and applied microbiology 66 6 330 - 338 2021年02月26日 [査読有り][通常論文]
     
    Aureobasidium pullulans YTP6-14 was demonstrated to be an excellent multiple biosurfactant producer utilizing cheap carbon sources available in Thailand, including glycerol and cassava flour hydrolysate. A. pullulans YTP6-14 maximally produced 1.81 g/l biosurfactant in an aqueous layer (BS-AQ) in a medium containing glycerol, and 7.37 or 6.37 g/l biosurfactant in a heavy oil layer (BS-HO) in cassava flour hydrolysate or a glucose containing medium, respectively. Each BS-AQ and BS-HO had critical micelle concentration values of 41.32 mg/l and 13.51 mg/l, and both biosurfactants formed a stable food oil emulsion and reduced the amount of biofilms formed by Streptococcus sobrinus and Streptococcus mutans. BS-AQ and BS-HO were mainly composed of liamocins or exophilins and massoia lactone, respectively.
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  • TOMOKI IWASHITA, YASUHIRO TANAKA, HIDEYUKI TAMAKI, RYOSUKE NAKAI, YASUKO YONEDA, AYAKA MAKINO, TADASHI TOYAMA, YOICHI KAMAGATA, MASAAKI MORIKAWA, KAZUHIRO MORI
    Japanese Journal of Water Treatment Biology 57 1 1 - 9 2021年 [査読有り][通常論文]
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  • Hidehiro Ishizawa, Masashi Kuroda, Daisuke Inoue, Masaaki Morikawa, Michihiko Ike
    FEMS Microbiology Ecology 96 7 2020年07月01日 [査読有り][通常論文]
     
    ABSTRACT Plant growth-promoting bacteria (PGPB) have recently been demonstrated as a promising agent to improve wastewater treatment and biomass production efficiency of duckweed hydrocultures. With a view to their reliable use in aqueous environments, this study analysed the plant colonization dynamics of PGPB and the ecological consequences for the entire duckweed-associated bacterial community. A PGPB strain, Aquitalea magnusonii H3, was inoculated to duckweed at different cell densities or timings in the presence of three environmental bacterial communities. The results showed that strain H3 improved duckweed growth by 11.7–32.1% in five out of nine experiments. Quantitative-PCR and amplicon sequencing analyses showed that strain H3 successfully colonized duckweed after 1 and 3 d of inoculation in all cultivation tests. However, it significantly decreased in number after 7 d, and similar bacterial communities were observed on duckweed regardless of H3 inoculation. Predicted metagenome analysis suggested that genes related to bacterial chemotactic motility and surface attachment systems are consistently enriched through community assembly on duckweed. Taken together, strain H3 dominantly colonized duckweed for a short period and improved duckweed growth. However, the inoculation of the PGPB did not have a lasting impact due to the strong resilience of the natural duckweed microbiome.
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  • Jakia Jerin Mehjabin, Liang Wei, Julie G. Petitbois, Taiki Umezawa, Fuyuhiko Matsuda, Charles S. Vairappan, Masaaki Morikawa, Tatsufumi Okino
    Journal of Natural Products 83 6 1925 - 1930 2020年06月26日 [査読有り][通常論文]
     
    Chemical investigation of the organic extract from Moorea bouillonii, collected in Sabah, Malaysia, led to the isolation of three new chlorinated fatty acid amides, columbamides F (1), G (2), and H (3). The planar structures of 1-3 were established by a combination of mass spectrometric and NMR spectroscopic analyses. The absolute configuration of 1 was determined by Marfey's analysis of its hydrolysate and chiral-phase HPLC analysis after conversion and esterification with Ohrui's acid, (1S,2S)-2-(anthracene-2,3-dicarboximido)cyclohexanecarboxylic acid. Compound 1 showed biosurfactant activity by an oil displacement assay. Related known fatty acid amides columbamide D and serinolamide C exhibited biosurfactant activity with critical micelle concentrations of about 0.34 and 0.78 mM, respectively.
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  • Le Thai Hang, Kazuhiro Mori, Yasuhiro Tanaka, Masaaki Morikawa, Tadashi Toyama
    Bioprocess and Biosystems Engineering 43 6 971 - 980 2020年06月 [査読有り][通常論文]
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  • Antimicrobial electrospun fiber mat from gelatin and crude extract lipopeptides
    Tipnipa Yoochang, Jirarat Anuntagool, Suthep Thaniyavarn, Masaaki Morikawa, Jiraporn Thaniyavarn
    Songklanakarin Journal of Science and Technology 42 1 101 - 108 2020年01月 [査読有り][通常論文]
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  • Hidehiro Ishizawa, Yuka Ogata, Yoshiyuki Hachiya, Ko-ichiro Tokura, Masashi Kuroda, Daisuke Inoue, Tadashi Toyama, Yasuhiro Tanaka, Kazuhiro Mori, Masaaki Morikawa, Michihiko Ike
    Chemosphere 238 124682 - 124682 2020年01月 [査読有り][通常論文]
     
    © 2019 Elsevier Ltd Plant growth-promoting bacteria (PGPB) are considered a promising tool to improve biomass production and water remediation by the aquatic plant, duckweed; however, no effective methodology is available to utilize PGPB in large hydroponic systems. In this study, we proposed a two-step cultivation process, which comprised of a “colonization step” and a “mass cultivation step,” and examined its efficacy in both bucket-scale and flask-scale cultivation experiments. We showed that in the outdoor bucket-scale experiments using three kinds of environmental water, plants cultured through the two-step cultivation method with the PGPB strain, Acinetobacter calcoaceticus P23, yielded 1.9 to 2.3 times more biomass than the control (without PGPB inoculation). The greater nitrogen and phosphorus removals compared to control were also attained, indicating that this strategy is useful for accelerating nutrient removal by duckweed. Flask-scale experiments using non-sterile pond water revealed that inoculation of strain P23 altered duckweed surface microbial community structures, and the beneficial effects of the inoculated strain P23 could last for 5–10 d. The loss of the duckweed growth-promoting effect was noticeable when the colonization of strain P23 decreased in the plant. These observations suggest that the stable colonization of the plant with PGPB is the key for maintaining the accelerated duckweed growth and nutrient removal in this cultivation method. Overall, our results suggest the possibility of an improved duckweed production using a two-step cultivation process with PGPB.
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  • Tadashi Toyama, Tsubasa Hanaoka, Koji Yamada, Kengo Suzuki, Yasuhiro Tanaka, Masaaki Morikawa, Kazuhiro Mori
    Biotechnology for Biofuels 12 1 205 - 205 2019年12月 [査読有り][通常論文]
     
    AbstractBackgroundEuglena gracilis, a unicellular flagellated microalga, is regarded as one of the most promising species as microalgal feedstock for biofuels. Its lipids (mainly wax esters) are suitable for biodiesel and jet fuel. Culture ofE. gracilisusing wastewater effluent will improve the economics ofE. gracilisbiofuel production. Enhancement of the productivity ofE. gracilisbiomass is critical to creating a highly efficient biofuels production system. Certain bacteria have been found to promote microalgal growth by creating a favorable microenvironment. These bacteria have been characterized as microalgae growth-promoting bacteria (MGPB). Co-culture of microalgae with MGPB might offer an effective strategy to enhance microalgal biomass production in wastewater effluent culture systems. However, no MGPB has been identified to enhance the growth ofE. gracilis. The objectives of this study were, therefore, to isolate and characterize the MGPB effective forE. gracilisand to demonstrate that the isolated MGPB indeed enhances the production of biomass and lipids byE. gracilisin wastewater effluent culture system. ResultsA bacterium,Emticiciasp. EG3, which is capable of promoting the growth of microalgaE. gracilis, was isolated from anE. gracilis-municipal wastewater effluent culture. Biomass production rate ofE. graciliswas enhanced 3.5-fold and 3.1-fold by EG3 in the co-culture system using a medium of heat-sterilized and non-sterilized wastewater effluent, respectively, compared to growth in the same effluent culture but without EG3. Two-step culture system was examined as follows:E. graciliswas cultured with or without EG3 in wastewater effluent in the first step and was further grown in wastewater effluent in the second step. Production yields of biomass and lipids byE. graciliswere enhanced 3.2-fold and 2.9-fold, respectively, in the second step of the system in whichE. graciliswas co-cultured with EG3 in the first step. ConclusionEmticiciasp. EG3 is the first MGPB forE. gracilis. Growth-promoting bacteria such as EG3 will be promising agents for enhancingE. gracilisbiomass/biofuel productivities.
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  • Hidehiro Ishizawa, Masashi Kuroda, Kanako Inoue, Daisuke Inoue, Masaaki Morikawa, Michihiko Ike
    Microbial Ecology 77 2 440 - 450 2019年02月15日 [査読有り][通常論文]
     
    © 2019, Springer Science+Business Media, LLC, part of Springer Nature. Despite the considerable role of aquatic plant-associated bacteria in host plant growth and nutrient cycling in aquatic environments, the mode of their plant colonization has hardly been understood. This study examined the colonization and competition dynamics of a plant growth-promoting bacterium (PGPB) and two plant growth-inhibiting bacteria (PGIB) in the aquatic plant Lemna minor (common duckweed). When inoculated separately to L. minor, each bacterial strain quickly colonized at approximately 10 6 cells per milligram (plant fresh weight) and kept similar populations throughout the 7-day cultivation time. The results of two-membered co-inoculation assays revealed that the PGPB strain Aquitalea magnusonii H3 consistently competitively excluded the PGIB strain Acinetobacter ursingii M3, and strain H3 co-existed at almost 1:1 proportion with another PGIB strain, Asticcacaulis excentricus M6, regardless of the inoculation ratios (99:1–1:99) and inoculation order. We also found that A. magnusonii H3 exerted its growth-promoting effect over the negative effects of the two PGIB strains even when only a small amount was inoculated, probably due to its excellent competitive colonization ability. These experimental results demonstrate that there is a constant ecological equilibrium state involved in the bacterial colonization of aquatic plants.
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  • Masashi Kuroda, Taro Horino, Daisuke Inoue, Masaaki Morikawa, Michihiko Ike
    Japanese Journal of Water Treatment Biology 54 4 105 - 113 2018年12月 [査読有り][通常論文]
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  • Yusuke Yamakawa, Rahul Jog, Masaaki Morikawa
    Plant Growth Regulation 86 2 287 - 296 2018年11月06日 [査読有り][通常論文]
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  • Utami, Desi, Kawahata, Ami, Sugawara, Masayuki, Jog, Rahul N., Miwa, Kyoko, Morikawa, Masaaki
    Frontiers in Chemistry 6 251  2018年07月 [査読有り][通常論文]
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  • Toyama, Tadashi, Kasuya, Mari, Hanaoka, Tsubasa, Kobayashi, Naoto, Tanaka, Yasuhiro, Inoue, Daisuke, Sei, Kazunari, Morikawa, Masaaki, Mori, Kazuhiro
    Biotechnology For Biofuels 11 176  2018年06月 [査読有り][通常論文]
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  • Tadashi Toyama, Tsubasa Hanaoka, Yasuhiro Tanaka, Masaaki Morikawa, Kazuhiro Mori
    Bioresource Technology 250 464 - 473 2018年02月01日 [査読有り][通常論文]
     
    To assess the potential of duckweeds as agents for nitrogen removal and biofuel feedstocks, Spirodela polyrhiza, Lemna minor, Lemna gibba, and Landoltia punctata were cultured in effluents of municipal wastewater, swine wastewater, or anaerobic digestion for 4 days. Total dissolved inorganic nitrogen (T-DIN) of 20–50 mg/L in effluents was effectively removed by inoculating with 0.3–1.0 g/L duckweeds. S. polyrhiza showed the highest nitrogen removal (2.0–10.8 mg T-DIN/L/day) and biomass production (52.6–70.3 mg d.w./L/day) rates in all the three effluents. Ethanol and methane were produced from duckweed biomass grown in each effluent. S. polyrhiza and L. punctata biomass showed higher ethanol (0.168–0.191, 0.166–0.172 and 0.174–0.191 g-ethanol/g-biomass, respectively) and methane (340–413 and 343–408 NL CH4/kg VS, respectively) production potentials than the others, which is related to their higher carbon and starch contents and calorific values.
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  • S. Luepongpattana, J. Thaniyavarn, M. Morikawa
    JOURNAL OF APPLIED MICROBIOLOGY 123 6 1488 - 1497 2017年12月 [査読有り][通常論文]
     
    Aims: In order to add to the existing knowledge about structural diversity of biosurfactants, marine environment was chosen to discover a new type of biosurfactant-producing fungus. Methods and Results: A number of fungi were collected from the Gulf of Thailand and examined for biosurfactant productivities. A dimorphic fungus, Aureobasidium pullulans YTP6-14, produced several different biosurfactants in both heavy oil and aqueous layers of the culture. Surface tension of the aqueous layer was decreased to 31.4 mN m(-1) and oil displacement area reached 53 cm(2)/10 mu l after 7 days of cultivation. Critical micelle concentration and minimum surface tension values of the crude biosurfactants prepared from the aqueous layer were 39 mg l(-1) and 31.6 mN m(-1) respectively. Surface tension values remained unchanged over a wide range of pII and NaCl concentrations, suggesting their nonionic feature. LC/MS and NMR analyses revealed that one of the main active compounds in the aqueous layer was 5-hydroxy-2-decenoic acid delta-lactone, known as massoia lactone. Massoia lactone indeed showed significant surface tension reduction capacity of 43.3 mN m(-1) at 1 mg ml(-1). Significance and Impact of the Study: This is the first report for the production of a fragrant biosurfactant, massoia lactone by a fungus A. pullulans. Massoia lactone has been industrially prepared from aromatic bark of an endangered tree species, Cryptocarya massoy, growing in rainforests. This report expands the diversity of biosurfactants produced by A. pullulans and also points to its possibility in contributing to the green sustainable chemistry, and ultimately rainforest conservation.
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  • Hidehiro Ishizawa, Masashi Kuroda, Masaaki Morikawa, Michihiko Ike
    PLANT PHYSIOLOGY AND BIOCHEMISTRY 118 667 - 673 2017年09月 [査読有り][通常論文]
     
    Bacteria colonizing the plant rhizosphere are believed to positively or negatively affect the host plant productivity. This feature has inspired researchers to engineer such interactions to enhance crop production. However, it remains to be elucidated whether rhizobacteria influences plant oxidative stress visa-vis other environmental stressors, and whether such influence is associated with their growth promoting/inhibiting ability. In this study, two plant growth-promoting bacteria (PGPB) and two plant growth-inhibiting bacteria (PGIB) were separately inoculated into axenic duckweed (Lemna minor) culture under laboratory conditions for 4 and 8 days in order to investigate their effects on plant oxidative stress and antioxidant activities. As previously characterized, the inoculation of PGPB and PGIB strains accelerated and reduced the growth of L. minor, respectively. After 4 and 8 days of cultivation, compared to the PGPB strains, the PGIB strains induced larger amounts of O-2(center dot-), H2O2, and malondialdehyde (MDA) in duckweed, although all bacterial strains consistently increased O-2(center dot-) content by two times more than that in the aseptic control plants. Activities of five antioxidant enzymes were also elevated by the inoculation of PGIB, confirming the severe oxidative stress condition in plants. These results suggest that the surface attached bacteria affect differently on host oxidative stress and its response, which degree correlates negatively to their effects on plant growth. (C) 2017 Elsevier Masson SAS. All rights reserved.
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  • T. Toyama, M. Kuroda, Y. Ogata, Y. Hachiya, A. Quach, K. Tokura, Y. Tanaka, K. Mori, M. Morikawa, M. Ike
    WATER SCIENCE AND TECHNOLOGY 76 6 1418 - 1428 2017年09月 [査読有り][通常論文]
     
    Duckweed offers the promise of a co-benefit culture combining water purification with biomass production. Acinetobacter calcoaceticus P23 is a plant growth-promoting bacterium isolated from a duckweed, Lemna aequinoctialis. This study quantified its growth-promoting effect on three duckweeds (L. aoukikusa, L. minor, and Spirodela polyrhiza) in sterile Hoagland solution and evaluated its usefulness in duckweed culture under non-sterile conditions. P23 promoted growth of three duckweeds in sterile Hoagland solution at low to high nutrient concentrations (1.25-10 mg NO3-N/L and 0.25-2.0 mg PO4-P/L). It increased the biomass production of L. aequinoctialis 3.8-4.3-fold, of L. minor 2.3-3.3-fold, and of S. polyrhiza 1.4-1.5-fold after 7 days compared with noninoculated controls. P23 also increased the biomass production of L. minor 2.4-fold in pond water and 1.7-fold in secondary effluent of a sewage treatment plant under non-sterile conditions at laboratory-scale experiments. P23 rescued L. minor from growth inhibition caused by microorganisms indigenous to the pond water. The results demonstrate that the use of P23 in duckweed culture can improve the efficiency of duckweed biomass production, and a positive effect of P23 on duckweed-based wastewater treatment can be assumed.
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  • Hidehiro Ishizawa, Masashi Kuroda, Masaaki Morikawa, Michihiko Ike
    BIOTECHNOLOGY FOR BIOFUELS 10 62  2017年03月 [査読有り][通常論文]
     
    Background: Duckweed (family Lemnaceae) has recently been recognized as an ideal biomass feedstock for biofuel production due to its rapid growth and high starch content, which inspired interest in improving their productivity. Since microbes that co-exist with plants are known to have significant effects on their growth according to the previous studies for terrestrial plants, this study has attempted to understand the plant-microbial interactions of a duckweed, Lemna minor, focusing on the growth promotion/inhibition effects so as to assess the possibility of accelerated duckweed production by modifying co-existing bacterial community. Results: Co-cultivation of aseptic L. minor and bacterial communities collected from various aquatic environments resulted in changes in duckweed growth ranging from -24 to + 14% compared to aseptic control. A number of bacterial strains were isolated from both growth-promoting and growth-inhibitory communities, and examined for their co-existing effects on duckweed growth. Irrespective of the source, each strain showed promotive, inhibitory, or neutral effects when individually co-cultured with L. minor. To further analyze the interactions among these bacterial strains in a community, binary combinations of promotive and inhibitory strains were co-cultured with aseptic L. minor, resulting in that combinations of promotive-promotive or inhibitory-inhibitory strains generally showed effects similar to those of individual strains. However, combinations of promotive-inhibitory strains tended to show inhibitory effects while only Aquitalea magnusonii H3 exerted its plant growth-promoting effect in all combinations tested. Conclusion: Significant change in biomass production was observed when duckweed was co-cultivated with environmental bacterial communities. Promotive, neutral, and inhibitory bacteria in the community would synergistically determine the effects. The results indicate the possibility of improving duckweed biomass production via regulation of co-existing bacterial communities.
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  • Chanapa Dejwatthanakomol, Jirarat Anuntagool, Masaaki Morikawa, Jiraporn Thaniyavarn
    SCIENCEASIA 42 4 252 - 258 2016年08月 [査読有り][通常論文]
     
    In this study, the production and characterization of a biosurfactant from yeast Wickerhamomyces anomalus strain PY189 was carried out. The highest efficiency for biosurfactant production was found when the organism was grown in a medium containing 4% (v/v) soya bean oil and 0.4% (w/v) NaNO3 at 30 degrees C and pH 5.5 for 7 days. After 7 days of cultivation, W. anomalus PY189 was able to produce up to 0.57 g/l of biosurfactant as ethyl acetate extracts. The culture supernatant was able to reduce the surface tension of the culture broth from 42.5 mN/mto 36.5 mN/m with a critical micelle concentration of 204 mg/l. The crude extract of biosurfactants was then applied to the encapsulation of lemongrass oil. Emulsions of lemongrass oil in 20 mg/dl maltodextrin solution (oil: maltodextrin solution ratios of 0.2:1, 0.15:1, and 0.1:1) containing 0.8% and 1% (w/v) crude biosurfactant extract were stable for at least 24 h and had an average oil droplet size of less than 10 mu m. Lemongrass oil microcapsules were later produced using a spray drying technique. This microcapsule exhibited microbial growth inhibition activity against E. coli, S. aureus, and Salmonella at 5% (w/v) concentration.
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  • Julius Adam V. Lopez, Sultan S. Al-Lihaibi, Walied M. Alarif, Ahmed Abdel-Lateff, Yasuyuki Nogata, Kenji Washio, Masaaki Morikawa, Tatsufumi Okino
    JOURNAL OF NATURAL PRODUCTS 79 4 1213 - 1218 2016年04月 [査読有り][通常論文]
     
    A mass spectrometry (MS)-guided isolation has led to the purification of a new cyanobactin, wewakazole B (1), along with the known compound curacin D from a Red Sea Moorea producens. The planar structure of 1 was elucidated using a combination of NMR and MS techniques. After ozonolysis and acid hydrolysis, the absolute configurations of the amino acid components of 1 were determined by chiral-phase LC-MS and HPLC analyses. Notably, compound 1 exhibited cytotoxic activity toward human MCF7 breast cancer cells (IC50 = 0.58 mu M) and human H460 lung cancer cells (IC50 = 1.0 mu M) and was also found to be inactive in a siderophore assay.
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  • Toru Fukano, Mitsuhiro Gomi, Yukihiko Osaki, Masaaki Morikawa
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 79 7 1207 - 1215 2015年07月 [査読有り][通常論文]
     
    The bacterial community structure was compared between the third days', one week', and three weeks' biofilm samples from the surface of a household toilet bowl. It was found that the PCR-DGGE band pattern of 16S rRNA gene was dramatically changed after the third day and was not further changed until three weeks. This result suggests that there are early and late colonizing bacterial groups. One of the early colonizers isolated from the third days' sample was Rhizobium sp. R8, a closest relative to Rhizobium giardinii, which exhibited the highest biofilm formation activity in an artificial urine condition. R8 produced extracellular polysaccharides containing galactose, glucose, and mannose at the molar ratio of 8:1:1, which were probably responsible for the biofilm formation. Its excelled biofilm formation and urease activities together with the lack of nodulation and nitrogen fixing genes in R8 suggest that this strain has been specifically adapted to urine condition in a toilet bowl.
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  • Julius Adam Velasco Lopez, Sultan S. Al-Lihaibi, Walied M. Alarif, Ahmed Abdel-Lateff, 鷲尾 健司, 森川 正章, 沖野 龍文
    天然有機化合物討論会講演要旨集 57 PosterP23  天然有機化合物討論会実行委員会 2015年 
    シアノバクテリアは、新規生物活性物質の有望な探索源である。1 特に、Moorea producens(旧名Lyngbya majuscula)からは新規化合物が報告され続けている。例えば、チューブ重合阻害物質であるcuracin A、アクチン重合促進物質であるhectochlorin、神経活性物質であるjamaicamide B、antillatoxin B、kalkitoxin2-6などが挙げられる。本研究では、紅海で採集したシアノバクテリアの化合物のプロファイルをLC/MSにより分析し、データベース(MarinLit)で解析した。その結果、新規化合物の存在が示唆されたM. producens から環状ドデカペプチドwewakazole B (1)を単離し、構造を決定した。 単離・精製 赤褐色で糸状のシアノバクテリアをサウジアラビアのジェッダでスキューバにより採集した。サンプルの一部をRNAlater 溶液中で保存し、標準的な16S rRNA配列決定に使用した。シアノバクテリア特異的プライマーの106Fと1509Rおよび内部プライマーの359Fと781R7,8 を用いたところ、M. producensと同定された。また、メタノール抽出物を酢酸エチルと水、ついでブタノールと水で溶媒分画した。各画分をMCF-7乳ガン細胞に対する細胞毒性、トリプシン阻害活性、タテジマフジツボAmphibalanus amphitriteキプリス幼生に対する付着阻害活性などの生物活性試験に供すると共に、LC/MS分析を実施し、データベース (MarinLit9)で検索した。その結果、どの画分も活性を示さなかったが、酢酸エチル画分にみられたピーク([M+H]+ m/z 1127) が新規物質と予想され、単離を目指すこととした。シリカゲルカラムクロマトグラフィー (hexane-EtOAc、EtOAc-MeOH) により8画分に分離され、LC/MSにより目的のピークはEtOAc-MeOH (3:1)で溶出された画分7に含まれることが示された。さらに、逆相のHPLC (0-20 min 30 – 80% MeCN, 20-40 min 80% MeCN, Cosmosil 5C18-AR, 10 × 250 mm, 3 mL/min, UV 210 nm) で得られた画分をさらに精製したところ(0-20 min 50 – 70% MeCN, Cosmosil 5C18-MS, 4.6 × 250 mm, 1 mL/min, UV 210 nm) 、0.4 mg の 1が得られた。 構造決定 分子式C58H70N12O12がHRESIMS ([M+H]+ m/z 1127.5310, ∆ = 0.39 ppm)によって得られ、不飽和度30であった。1H NMRスペクトルには複数のアミドプロトンおよび芳香族プロトン(δH ≥ 7.0)とアミノ酸残基の α-プロトン(δH 4-6)、さらに3つの鋭いシングレット(δH 2.41, 2.53, 8.02)が観測された。これらMSとNMRのデータを用いてあらためてMarinLitによって検索したところ、wewakazole10 に類似していると考えられ、上記の鋭いシングレットピークは2個のメチルオキサゾール(MeOxz)のメチルプロトンとオキサゾール(Oxz)のメチンプロトン1個と帰属された。HSQC データにより8個のα-メチン、2組の一置換フェニル基、6個のメチル、13個のメチレンとさらにもう1個のメチンプロトンが認められた。Wewakazole のHSQC と比較すると1ではδC 140.6と δH 8.02の間にHSQC相関がなかった。しかし、HMBCでは1JCH 相関 (210 Hz) が観測され、オキサゾールであることが示された。COSY、 TOCSYおよびHMBCスペクトルにより9個のアミノ酸残基と3個 (View PDFfor the rest of the abstract.)
  • Masayuki Sugawara, Akira Hosoyama, Atsushi Yamazoe, Masaaki Morikawa
    Genome Announcements 3 1 e00026-15  2015年 [査読有り][通常論文]
     
    Acinetobacter calcoaceticus strain P23 is a plant growth-promoting bacterium, which was isolated from the surface of duckweed. We report here the draft genome sequence of strain P23. The genome data will serve as a valuable reference for understanding the molecular mechanism of plant growth promotion in aquatic plants.
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  • Kensuke Kaneko, Kenji Washio, Taiki Umezawa, Fuyuhiko Matsuda, Masaaki Morikawa, Tatsufumi Okino
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 78 8 1310 - 1319 2014年08月 [査読有り][通常論文]
     
    The marine red alga genus Laurencia is one of the richest producers of unique brominated compounds in the marine environment. The cDNAs for two Laurencia nipponica vanadium-dependent bromoperoxidases (LnVBPO1 and LnVBPO2) were cloned and expressed in Escherichia coli. Enzyme assays of recombinant LnVBPO1 and LnVBPO2 using monochlorodimedone revealed that they were thermolabile but their K-m values for Br- were significantly lower than other red algal VBPOs. The bromination reaction was also assessed using laurediol, the predicted natural precursor of the brominated ether laurencin. Laurediol, protected by trimethylsilyl at the enyne, was converted to deacetyllaurencin by the LnVBPOs, which was confirmed by tandem mass spectrometry. Native LnVBPO partially purified from algal bodies was active, suggesting that LnVBPO is functional in vivo. These results contributed to our knowledge of the biosynthesis of Laurencia brominated metabolites.
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  • Wakako Suzuki, Masayuki Sugawara, Kyoko Miwa, Masaaki Morikawa
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 118 1 41 - 44 2014年07月 [査読有り][通常論文]
     
    Acinetobacter cakoaceticus P23 is a plant growth-promoting bacterium that was isolated from the surface of duckweed (Lemna aoubilmsa). The bacterium was observed to colonize on the plant surfaces and increase the chlorophyll content of not only the monocotyledon Lemna minor but also the dicotyledon Lactuca sativa in a hydroponic culture. This effect on the Lactuca sativa was significant in nutrient-poor ( x 1/100 dilution of H2 medium) and not nutrient-rich ( x 1 or x1/l0 dilutions of H2 medium) conditions. Strain P23 has the potential to play a part in the future development of fertilizers and energy-saving hydroponic agricultural technologies. (C) 2013, The Society for Biotechnology, Japan. All rights reserved.
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  • Le Thi Nhi Cong, Cung Thi Ngoc Mai, Masaaki Morikawa, Nghiem Ngoc Minh
    JOURNAL OF ENVIRONMENTAL SCIENCE AND HEALTH PART A-TOXIC/HAZARDOUS SUBSTANCES & ENVIRONMENTAL ENGINEERING 49 7 777 - 786 2014年06月 [査読有り][通常論文]
     
    This work is aimed to assess the aerobic biotransformation of a branched side chain alkylbenzene, iso-pentylbenzene, by Candida viswanathii TH1. The yeast Candida viswanathii TH1 isolated from oil-polluted sediments collected in coastal zones in Vietnam exhibited as a strain that could better transform branched aromatic hydrocarbons in biofilm (pellicle) than in planktonic form. During incubation of TH1 as biofilm with iso-pentylbenzene, the seven intermediates produced were benzoic acid, phenylacetic acid, 2-methyl-4-phenyl-butan-1-ol, 2-hydroxy-phenylacetic acid, 2-methyl-4-phenylbutyric acid, succinic acid and iso-valerophenone as revealed by gas chromatography/mass spectra and high-performance liquid chromatography analyses. The occurrence of these intermediates showed that iso-pentylbenzene could be oxidized not only via mono- but also by a sub-terminal oxidation pathway. This is the first study on iso-pentylbenzene transformation by a biofilm-forming Candida viswanathii strain. The catabolic versatility of the biofilm-forming strain TH1 and its use for mono and sub-terminal oxidation during the transformation of iso-pentylbenzene enhance our understanding of the degradation of branched side chain phenylalkanes and give new insight into the potential role of such species in the transformation of other recalcitrant aromatic compounds.
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  • Chanita Boonmak, Yasunori Takahashi, Masaaki Morikawa
    EXTREMOPHILES 18 3 515 - 523 2014年05月 [査読有り][通常論文]
     
    An extremely thermophilic bacterium, Geobacillus thermoleovorans B23, is capable of degrading a broad range of alkanes (with carbon chain lengths ranging between C11 and C32) at 70 A degrees C. Whole-genome sequence analysis revealed that unlike most alkane-degrading bacteria, strain B23 does not possess an alkB-type alkane monooxygenase gene. Instead, it possesses a cluster of three ladA-type genes, ladA alpha(B23), ladA beta(B23), and ladB (B23), on its chromosome, whose protein products share significant amino acid sequence identities, 49.8, 34.4, and 22.7 %, respectively, with that of ladA alkane monooxygenase gene found on a plasmid of Geobacillus thermodetrificans NG 80-2. Each of the three genes, ladA alpha(B23), ladA beta(B23), and ladB (B23), was heterologously expressed individually in an alkB1 deletion mutant strain, Pseudomonas fluorescens KOB2 Delta 1. It was found that all three genes were functional in P. fluorescens KOB2 Delta 1, and partially restored alkane degradation activity. In this study, we suggest that G. thermoleovorans B23 utilizes multiple LadA-type alkane monooxygenases for the degradation of a broad range of alkanes.
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  • 金子 賢介, 鷲尾 健司, 梅澤 大樹, 小林 大毅, 湯 暁蓉, 松田 冬彦, 森川 正章, 沖野 龍文
    天然有機化合物討論会講演要旨集 56 Poster53  天然有機化合物討論会実行委員会 2014年 
    紅藻ウラソゾ (Laurencia nipponica) から含臭素環状エーテル laurencin (1) が単離されて以来 1, 2)、ソゾ属からは、現在までに 600 を超える多様なハロゲン化合物 (主に臭素付加化合物) が単離・報告されている 3)。これらソゾ由来含臭素化合物の生合成における鍵反応は、環形成を伴った臭素付加反応と考えられている。 村井らは、同過程の触媒酵素の候補として、ブロモペルオキシダーゼ (BPO) をウラソゾから部分精製し 4)、1 の推定生合成前駆体 laurediol (2) 5) を用いた臭素付加・環形成実験に供した。その結果、部分精製 BPO は、2 から deacetyllaurencin (3) への臭素付加・環形成を触媒することが示された (Scheme 1) 4)。酵素生成物である 3 は、1 の生合成最終前駆体であることから、1 の臭素付加・環形成過程は、BPO により触媒されることが示唆された。一方で、ウラソゾ BPO の構造および生化学的知見は、現在に至るまで明らかにされていない。 他の紅藻 Corallina 属などでは、BPOの結晶構造が解明されており、活性中心にバナジン酸 (VO43-) を要求するバナジウム依存型 BPO (VBPO) であると報告されている 6)。そこで、本研究では、ソゾ由来の臭素付加酵素の同定のため、ウラソゾより VBPO 遺伝子クローニングを行った。また、ウラソゾ VBPO組み換えタンパク質を調製し、生化学的特性の評価とソゾ由来臭素化合物の推定前駆体を用いた in vitro 臭素付加反応を行い、生合成における役割を評価した。 Scheme 1. In vitro enzymatic bromination of laurediol using partially purified BPO from L. nipponica 4). ウラソゾ由来 VBPO の cDNA クローニングと組み換えタンパク質の調製 RACE PCR 法によって、ウラソゾ VBPO cDNA クローニングを行った結果、二種類のウラソゾVBPO 全長配列 (LnVBPO1およびLnVBPO2, 95% identity) を取得した。両遺伝子を、それぞれ大腸菌発現系 BL21 (DE3) pLysS に導入後、可溶画分を抽出し、硫安沈殿と DE52 陰イオン交換クロマトグラフィによって、LnVBPO1 および LnVBPO2組み換えタンパク質を精製した。得られたタンパク質をSDS-PAGE に供したところ、いずれも 77 kDa の位置に単一のバンドとして泳動された。また、両組み換えタンパク質は、ゲルろ過において最大で750 kDa 程度であり、10 量体を形成することが推定された。VBPO においては、紅藻 Corallina 由来 VBPO も 12 量体を形成することが知られている 7,8) 。 次に、藻体由来の BPO と LnVBPOs 組み換えタンパク質との同一性を検証するため、同様な精製方法を用いて、ウラソゾ藻体から BPO の精製を試みた。藻体由来 BPO は、色素成分との分離が困難であり、部分精製に留まった。組み換え LnVBPOs と部分精製 BPO をSDS-PAGE に供したところ、ともに 75 kD (View PDFfor the rest of the abstract.)
  • S. Kesel, F. Moormann, I. G�mperlein, A. Mader, M. Morikawa, O. Lieleg, M. Opitz
    Genome Announcements 2 6 e01163-14  2014年 [査読有り][通常論文]
     
    We report here the draft genome sequence of the Bacillus subtilis strain B-1, a strain known to form biofilms. The biofilm matrix mainly consists of the biopolymer γ-polyglutamate (γ-PGA). The sequence of the genome of this strain allows the study of specific genes involved in biofilm formation.
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  • Jamroonsri Poomtien, Jiraporn Thaniyavarn, Pairoh Pinphanichakarn, Sasitorn Jindamorakot, Masaaki Morikawa
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 77 12 2362 - 2370 2013年12月 [査読有り][通常論文]
     
    Cyberlindnera samutprakarnensis JP52(T), isolated from cosmetic industrial wastes in Thailand, was found to be an efficient biosurfactant-producing yeast when cultured in a medium containing (2% (w/v) glucose and 2% (v/v) palm oil at 30 degrees C, 200 rpm for 7 d. The crude biosurfactant had the ability to reduce the surface tension from 55.7 to 30.9 mN/m at 25 degrees C with a critical micelle concentration (CMC) of 0.046%. Physicochemical analysis of the crude biosurfactant revealed that it had wide ranges of optimum pH and pH stability at 6-9 and 3-10 respectively. It was also thermostable and retained 80% activity even after heat treatment, and it tolerated NaCI at 1.0-10%. Furthermore, it effectively emulsified various vegetable oils with an E24 value of over 80%. A partially purified biosurfactant fraction was analyzed for its structure by MALDI-TOF MS and NMR. This revealed that the biosurfactant mainly contained sophorolipids in C18-(MW 574) and C16-diaceltylated (MW 662) forms.
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  • Yoshikane Itoh, Keiko Sakagami, Yoshihito Uchino, Chanita Boonmak, Tetsuro Oriyama, Fuyumi Tojo, Mitsufumi Matsumoto, Masaaki Morikawa
    MICROBES AND ENVIRONMENTS 28 4 432 - 435 2013年12月 [査読有り][通常論文]
     
    A thermotolerant ammonia-oxidizing bacterium strain JPCCT2 was isolated from activated sludge in a thermal power station. Cells of JPCCT2 are short non-motile rods or ellipsoidal. Molecular phylogenetic analysis of 16S rRNA gene sequences demonstrated that JPCCT2 belongs to the genus Nitrosomonas with the highest similarity to Nitrosomonas nitrosa Nm90 (100%), Nitrosomonas sp. Nm148 (99.7%), and Nitrosomonas communis Nm2 (97.7%). However, G+C content of JPCCT2 DNA was 49.1 mol% and clearly different from N. nitrosa Nm90, 47.9%. JPCCT2 was capable of growing at temperatures up to 48 degrees C, while N. nitrosa Nm90 and N. communis Nm2 could not grow at 42 degrees C. Moreover, JPCCT2 grew similarly at concentrations of carbonate 0 and 5 gL(-1). This is the first report that Nitrosomonas bacterium is capable of growing at temperatures higher than 37 degrees C.
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  • Chanita Boonmak, Yasunori Takahasi, Masaaki Morikawa
    Genome Announcements 1 6 e00944-13  2013年 [査読有り][通常論文]
     
    Here, we report the draft genome sequence of Geobacillus thermoleovorans strain B23, which was isolated from a deep subterranean petroleum reservoir in Japan. An array of genes related to unique long-chain alkane degradation pathways in G. thermoleovorans B23 has been identified by whole-genome analyses of this strain.
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  • Toyama T, Ojima T, Tanaka Y, Mori K, Morikawa M
    Water Sci. Technol. 68 3 522 - 529 2013年 [査読有り][通常論文]
     
    The efficacy of two rhizobacteria (Sphingobium fuliginis TIK1 and Sphingobium sp. IT4) of Phragmites australis for the sustainable treatment of water polluted with phenolic endocrine-disrupting chemicals (EDCs) was investigated. Strains TIK1 and IT4 have recently been isolated from Phragmites rhizosphere and shown to degrade various 4-alkylphenols-TIK1 via phenolic ring hydroxylation and meta-cleavage and IT4 via ipso-hydroxylation. The two strains also degraded bisphenol A (BPA), bisphenol B, bisphenol E, bisphenol F, bisphenol P and bisphenol S (BPS). Thus, strains TIK1 and IT4 have wide degradation spectra for phenolic EDCs. The two strains utilized Phragmites root extracts as a sole carbon source and sustainably colonized Phragmites roots, where they degraded phenolic EDCs. In sequencing batch reactor experiments using Phragmites in association with TIK1 or IT4, both associations repeatedly removed phenolic EDCs from polluted secondary effluent water (BPA, BPS, 4-tert-butylphenol, 4-tert-octylphenol and 4-nonylphenol) from polluted secondary effluent water. The results suggest that hydroponic systems using Phragmites-TIK and Phragmites-IT4 associations would be useful for sustainable treatment of polluted waters containing various phenolic EDCs.
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  • バイオフィルムをしらべてみよう
    森川 正章
    生物工学会誌 90 246 - 250 2012年05月 [査読無し][招待有り]
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  • Kohei Shimada, Yoshikane Itoh, Kenji Washio, Masaaki Morikawa
    CHEMOSPHERE 87 3 226 - 233 2012年04月 [査読有り][通常論文]
     
    In natural environments, bacteria often exist in close association with surfaces and interfaces. There they form "biofilms", multicellular aggregates held together by an extracellular matrix. The biofilms confer on the constituent cells high resistance to environmental stresses and diverse microenvironments that help generate cellular heterogeneity. Here we report on the ability of Pseudomonas stutzeri T102 biofilm-associated cells, as compared with that of planktonic cells, to degrade naphthalene and survive in petroleum-contaminated soils. In liquid culture system. T102 biofilm-associated cells did not degrade naphthalene during initial hours of incubation but then degraded it faster than planktonic cells, which degraded naphthalene at a nearly constant rate. This delayed but high degradation activity of the biofilms could be attributed to super-activated cells that were detached from the biofilms. When the fitness of T102 biofilm-associated cells was tested in natural petroleum-contaminated soils, they were capable of surviving for 10 wk; by then T102 planktonic cells were mostly extinct. Naphthalene degradation activity in the soils that had been inoculated with T102 biofilms was indeed higher than that observed in soils inoculated with T102 planktonic cells. These results suggest that inoculation of contaminated soils with P. stutzeri T102 biofilms should enable bioaugmentation to be a more durable and effective bioremediation technology than inoculation with planktonic cells. (C) 2012 Elsevier Ltd. All rights reserved.
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  • 飯島沙織, 岡原良太, 鷲尾健司, 森川正章
    海水学会誌 66 4 186 - 190 The Society of Sea Water Science, Japan 2012年 [査読無し][通常論文]
  • Kenji Washio, Siew Ping Lim, Niran Roongsawang, Masaaki Morikawa
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 75 10 1880 - 1888 2011年10月 [査読有り][通常論文]
     
    Arthrofactin is a biosurfactant produced by Pseudomonas sp. MIS38. We have reported that transposon insertion into spoT (spoT::Tn5) causes moderate accumulation of guanosine 3',5'-bispyrophosphate (ppGpp) and abrogates arthrofactin production. To analyze the linkage of SpoT function and ablation of arthrofactin production, we examined the spoT::Tn5 mutation. The results showed that spoT::Tn5 is not a null mutation, but encodes separate segments of SpoT. Deletion of the 3' region of spoT increased the level of arthrofactin production, suggesting that the C-terminal region of SpoT plays a suppressive role. We evaluated the expression of a distinct segment of SpoT. Forced expression of the C-terminal region that contains the ACT domain resulted in the accumulation of ppGpp and abrogated arthrofactin production. Expression of the C-terminal segment also reduced MIS38 swarming and resulted in extensive biofilm formation, which constitutes the phenocopy of the spoT::Tn5 mutant.
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  • Niran Roongsawang, Kenji Washio, Masaaki Morikawa
    INTERNATIONAL JOURNAL OF MOLECULAR SCIENCES 12 1 141 - 172 2011年01月 [査読有り][通常論文]
     
    Lipopeptide biosurfactants (LPBSs) consist of a hydrophobic fatty acid portion linked to a hydrophilic peptide chain in the molecule. With their complex and diverse structures, LPBSs exhibit various biological activities including surface activity as well as anti-cellular and anti-enzymatic activities. LPBSs are also involved in multi-cellular behaviors such as swarming motility and biofilm formation. Among the bacterial genera, Bacillus (Gram-positive) and Pseudomonas (Gram-negative) have received the most attention because they produce a wide range of effective LPBSs that are potentially useful for agricultural, chemical, food, and pharmaceutical industries. The biosynthetic mechanisms and gene regulation systems of LPBSs have been extensively analyzed over the last decade. LPBSs are generally synthesized in a ribosome-independent manner with megaenzymes called nonribosomal peptide synthetases (NRPSs). Production of active-form NRPSs requires not only transcriptional induction and translation but also post-translational modification and assemblage. The accumulated knowledge reveals the versatility and evolutionary lineage of the NRPSs system. This review provides an overview of the structural and functional diversity of LPBSs and their different biosynthetic mechanisms in Bacillus and Pseudomonas, including both typical and unique systems. Finally, successful genetic engineering of NRPSs for creating novel lipopeptides is also discussed.
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  • Tojo F, Itoh Y, Okabe S, Morikawa M
    J. Environ. Biotechnol. 11 1-2 77 - 81 環境バイオテクノロジー学会 2011年 [査読有り][通常論文]
  • Masaaki Morikawa
    APPLIED MICROBIOLOGY AND BIOTECHNOLOGY 87 5 1595 - 1603 2010年08月 [査読有り][通常論文]
     
    The most significant aspect in microbial metabolisms, especially those of bacteria and archaea, is their marvelously wide acceptability of substrate electron donors and acceptors. This feature makes them to be attractive catalysts for environmental biotechnology in terms of degradation of harmful recalcitrant compounds, including hydrocarbons. Transformation of highly reduced and inert hydrocarbon compounds is with no doubt a challenging biochemical reaction for a single enzyme. However, several multi-component enzyme systems enable microorganisms to utilize hydrocarbons as carbon and energy (electron) sources. Initial biological attack to hydrocarbons is, in most cases, the hydroxylation that requires molecular dioxygen as a co-substrate. Dioxygen also contributes to the ring cleavage reaction of homo- and hetero-cyclic aromatic hydrocarbons. Although the molecular dioxygen is omnipresent and highly soluble in water, activation and splitting this triplet ground-state molecule to wed with difficult hydrocarbons need special devices. Non-heme iron, heme iron, or flavin nucleotide was designated as a major hidden dagger for this purpose.
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  • Fumiko Yamaga, Kenji Washio, Masaaki Morikawa
    ENVIRONMENTAL SCIENCE & TECHNOLOGY 44 16 6470 - 6474 2010年08月 [査読有り][通常論文]
     
    Phenol-degrading bacteria were isolated from the rhizosphere of duckweed (Lemna aoukikusa) using an enrichment culture method. One of the isolates, P23, exhibited an excellent ability to degrade phenol and attach to a solid surface under laboratory conditions. Phylogenetic analysis revealed that P23 belongs to the genera Acinetobacter and has the highest similarity to Acinetobacter calcoaceticus. P23 rapidly colonized on the surface of sterilized duckweed roots and formed biofilms, indicating that the conditions provided by the root system of duckweed are favorable to P23. A long-term performance test (160 h) showed that continuous removal of phenol can be attributed to the beneficial symbiotic interaction between duckweed and P23 P23 is the first growth-promoting bacterium identified from Lemna aoukikusa. The results in this study suggest the potential usefulness of dominating a particular bacterium in the rhizosphere of duckweeds to achieve efficient and sustainable bioremediation of polluted water
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  • Kenji Washio, Siew Ping Lim, Niran Roongsawang, Masaaki Morikawa
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 74 5 992 - 999 2010年05月 [査読有り][通常論文]
     
    Pseudomonas sp. MIS38 produces an effective biosurfactant named arthrofactin, which is a cyclic lipopeptide synthesized by a mega complex composed of three nonribosomal peptide synthetases. In order to gain insight into the control mechanism of arthrofactin production, a Tn5 mutant library was constructed and screened for arthrofactin-deficient mutants. Along with a number of mutations that occurred in the arthrofactin synthetase operon, three other mutants harbored distinct Tn5 insertions in the genes encoding SyrF-like protein (arfF), heat shock protein (htpG), and (p)ppGpp synthetase/hydrolase (spoT). Epistasis analyses revealed that spoT functions early in the arthrofactin production pathway. We also found that spoT affects MIS38 swarming, biofilm formation, and the cell morphology.
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  • Kaihei Oki, Kenji Washio, Daigo Matsui, Shinichi Kato, Yoshihiko Hirata, Masaaki Morikawa
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 74 3 583 - 589 2010年03月 [査読有り][通常論文]
     
    Urolith, which consists of dirty yellow-colored attachments on the toilet bowl, is associated with a variety of odorous chemicals, including ammonia, and causes disadvantages in daily life. Although largely it is derived from microorganisms, little is known about the microbial processes underlying the formation of urolith. In order to gain insight into the types and the activities of microorganisms present in urolith, culturable bacteria were isolated, identified, and physiologically characterized. One of the isolates exhibited higher ability to produce ammonia when it was grown in artificial urine medium. Phylogenetic and physiological analyses indicated that this strain (T-02) belonged to a new group of Staphylococcus species, showing combined phenotypes as between S. lentus and S. xylosus. T-02 exhibited high urease activity and was capable of growing in the urinary condition by forming robust biofilms. The results of this study indicate that T-02 has successfully adapted itself to the environment of urolith.
  • 坂口直史, Taha, A.I.B.H.M, 牧 秀明, 濱田誠一, 森川正章, 奥山英登志
    生物工学会誌 88 4 150 - 157 日本生物工学会 2010年 [査読有り][通常論文]
     
    2008年ロシア・サハリン島の油田開発は商業段階に入った.北海道沿岸域はサハリン油田開発を原因とする油井の暴噴,パイプラインやタンカーなど船舶の事故による汚染の危険に曝されている.石油により汚染された海域,海岸域の回復にはさまざまな対応が必要である.本総説では,これまで起こった主にタンカーの石油流出事故とそれに対する生物学的処理法(バイオレメディエーション,BR)による対応,特に北海道の冷涼な気候とBRについてその有用性を考慮しながら紹介した.北海道オホーツク海沿岸ではすでに石油汚染除去を想定したバイオスティミュレーション法(BS)が試験的に実施されている.BSは汚染現場に栄養塩などを与え土着の微生物の石油分解能を賦活化する方法である.一方,筆者らはBSと,別に取得した石油分解能力の高い細菌を汚染現場に投与するバイオオーグメンテーション法(BA)の特長を併せ持つ原地性バイオオーグメンテーション法(ABA)の有効性を検討している.サハリン油田が原因で汚染事故が起きた場合のABAの実用の可能性について論じた.
  • Tomohisa Kato, Asuka Miyanaga, Shigenori Kanaya, Masaaki Morikawa
    EXTREMOPHILES 14 1 33 - 39 2010年01月 [査読有り][通常論文]
     
    Geobacillus thermoleovorans B23 is capable of degrading long-chain alkanes at 70A degrees C. Bt-aldh, an aldehyde dehydrogenase gene in B23, was located in the upstream region of p21 whose expression level was dramatically increased when alkane degradation was started (Kato et al. 2009, BMC Microbiol 9:60). Like p21, transcription level of Bt-aldh was also increased upon alkane degradation. Bt-Aldh (497 aa, MW = 53,886) was overproduced in Escherichia coli, purified, and characterized biochemically. Bt-Aldh acted as an octamer, required NAD(+) as a coenzyme, and showed high activity against aliphatic long-chain aldehydes such as tetradecanal. The optimum condition for activity was 50-55A degrees C and pH 10.0. The activity was elevated to two- to threefold in the presence of 2 mM Ba2+, Ca2+, or Sr2+, while Mg2+ and Zn2+ inhibited the enzyme activity. Bt-Aldh represents thermophilic aldehyde dehydrogenases responsible for degradation of long-chain alkanes.
  • Reia Hosokawa, Motonori Nagai, Masaaki Morikawa, Hidetoshi Okuyama
    WORLD JOURNAL OF MICROBIOLOGY & BIOTECHNOLOGY 25 9 1519 - 1528 2009年09月 [査読有り][通常論文]
     
    Bioaugmentation for oil spills is a much more promising technique than is biostimulation. However, the effectiveness of bioaugmentation is variable, because the survival and the xenobiotic-degrading ability of introduced microorganisms are highly dependent on environmental conditions. As an alternative, autochthonous bioaugmentation (ABA) is proposed to overcome these difficulties. The ABA method is like a ready-made bioaugmentation technology. In ABA, microorganisms indigenous to the contaminated site or predicted contamination site that are well-characterized and potentially capable of degrading oils are used, and these microorganisms should be enriched under conditions where bioaugmentation will be conducted. It is possible to obtain information in advance on the chemical and physical characteristics of potential oil spill sites and of oils that might be spilled. The application of ABA in the coastal areas of Hokkaido Prefecture, Japan, is considered here, because Hokkaido is located south of Sakhalin Island, Russia, where development of oil fields is in progress. If oil spills in this region were well characterized in advance, ABA could be a feasible technology in the near future.
  • S. P. Lim, N. Roongsawang, K. Washio, M. Morikawa
    JOURNAL OF APPLIED MICROBIOLOGY 107 1 157 - 166 2009年07月 [査読有り][通常論文]
     
    To obtain further insights into transportation mechanisms of a most effective biosurfactant, arthrofactin in Pseudomonas sp. MIS38. A cluster genes arfA/B/C encodes an arthrofactin synthetase complex (ArfA/B/C). Downstream of the arfA/B/C lie genes encoding a putative periplasmic protein (ArfD, 362 aa) and a putative ATP-binding cassette transporter (ArfE, 651 aa), namely arfD and arfE, respectively. The arfA/B/C, arfD, and arfE form an operon suggesting their functional connection. Gene knockout mutants ArfD:Km, ArfE:Km, ArfD:Tc/ArfE:Km, and gene overexpression strains MIS38(pME6032_arfD/E) and ArfE:Km(pME6032_arfD/E) were prepared and analysed for arthrofactin production profiles. It was found that the production levels of arthrofactin were temporally reduced in the mutants or increased in the gene overexpression strains, but they eventually became similar level to that of MIS38. Addition of ABC transporter inhibitors, glibenclamide and sodium ortho-vanadate dramatically reduced the production levels of arthrofactin. This excludes a possibility that arthrofactin is exported by diffusion with the aid of its own high surfactant activity. ArfD/E is not an exclusive but a primary exporter of arthrofactin during early growth stage. Reduction in the arthrofactin productivity of arfD and arfE knockout mutants was eventually rescued by another ABC transporter system. Effects of arfD and arfE overexpression were evident only for 1-day cultivation. Multiple ATP dependent active transporter systems are responsible for the production of arthrofactin. Pseudomonas bacteria are characterized to be endued with multiple exporter and efflux systems for secondary metabolites including antibiotics, plant toxins, and biosurfactants. The present work demonstrates exceptionally flexible and highly controlled transportation mechanisms of a most effective lipopeptide biosurfactant, arthrofactin in Pseudomonas sp. MIS38. Because lipopeptide biosurfactants are known to enhance efficacy of bioactive compounds and arfA/B/C/D/E orthologous genes are also found in plant pathogenic P. fluorescens and P. syringae strains, the knowledge would also contribute to develop a technology controlling plant diseases.
  • Saori Iijima, Kenji Washio, Ryota Okahara, Masaaki Morikawa
    MICROBIAL BIOTECHNOLOGY 2 3 361 - 369 2009年05月 [査読有り][通常論文]
     
    In order to save natural resources and supply good fishes, it is important to improve fish-farming techniques. The survival rate of fish fry appears to become higher when powders of foraminifer limestone are submerged at the bottom of fish-farming fields, where bacterial biofilms often grow. The observations suggest that forming biofilms can benefit to keep health status of breeding fishes. We employed culture-based methods for the identification and characterization of biofilm-forming bacteria and assessed the application of their properties for fish farming. Fifteen bacterial strains were isolated from the biofilm samples collected from fish farm sediments. The 16S rRNA gene sequences indicated that these bacteria belonged to the genera, Pseudoalteromonas (seven strains), Vibrio (seven strains) and Halomonas (one strain). It was found that Pseudoalteromonas strains generally formed robust biofilms in a laboratory condition and produced extracellular proteases in a biofilm-dependent manner. The results suggest that Pseudoalteromonas bacteria, living in the biofilm community, contribute in part to remove excess proteineous matters from the sediment sludge of fish farms.
  • Tomohisa Kato, Asuka Miyanaga, Shigenori Kanaya, Masaaki Morikawa
    BMC MICROBIOLOGY 9 60  2009年03月 [査読有り][通常論文]
     
    Background: Initial step of beta-oxidation is catalyzed by acyl-CoA dehydrogenase in prokaryotes and mitochondria, while acyl-CoA oxidase primarily functions in the peroxisomes of eukaryotes. Oxidase reaction accompanies emission of toxic by-product reactive oxygen molecules including superoxide anion, and superoxide dismutase and catalase activities are essential to detoxify them in the peroxisomes. Although there is an argument about whether primitive life was born and evolved under high temperature conditions, thermophilic archaea apparently share living systems with both bacteria and eukaryotes. We hypothesized that alkane degradation pathways in thermophilic microorganisms could be premature and useful to understand their evolution. Results: An extremely thermophilic and alkane degrading Geobacillus thermoleovorans B23 was previously isolated from a deep subsurface oil reservoir in Japan. In the present study, we identified novel membrane proteins (P16, P21) and superoxide dismutase (P24) whose production levels were significantly increased upon alkane degradation. Unlike other bacteria acyl-CoA oxidase and catalase activities were also increased in strain B23 by addition of alkane. Conclusion: We first suggested that peroxisomal beta-oxidation system exists in bacteria. This eukaryotic-type alkane degradation pathway in thermophilic bacterial cells might be a vestige of primitive living cell systems that had evolved into eukaryotes.
  • Development of bioremediation by utilizing biofilms.
    MORIKAWA, Masaaki
    IFO Res. Commun. 23 99 - 115 2009年 [査読有り][通常論文]
  • Daisuke Takei, Kenji Washio, Masaaki Morikawa
    BIOTECHNOLOGY LETTERS 30 8 1447 - 1452 2008年08月 [査読有り][通常論文]
     
    Rhodococcus sp. TMP2 is an alkane-degrading strain that can grow with a branched alkane as a sole carbon source. TMP2 degrades considerable amounts of pristane at 20 degrees C but not at 30 degrees C. In order to gain insights into microbial alkane degradation, we characterized one of the key enzymes for alkane degradation. TMP2 contains at least five genes for membrane-bound, non-heme iron, alkane hydroxylase, known as AlkB (alkB1-5). Phylogenetical analysis using bacterial alkB genes indicates that TMP2 is a close relative of the alkane-degrading bacteria, such as Rhodococcus erythropolis NRRL B-16531 and Q15. RT-PCR analysis showed that expressions of the genes for AlkB1 and AlkB2 were apparently induced by the addition of pristane at a low temperature. The results suggest that TMP2 recruits certain alkane hydroxylase systems to utilize a branched alkane under low temperature conditions.
  • Jiraporn Thaniyavarn, Tanusta Chianguthai, Polakit Sangvanich, Niran Roongsawang, Keji Washio, Masaaki Morikawa, Suthep Thaniyavarn
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 72 8 2061 - 2068 2008年08月 [査読有り][通常論文]
     
    Biosurfactant production by Pichia anomala PY1, a thermotorelant strain isolated from fermented food, was examined as grown in media containing various carbon and nitrogen sources. The optimal conditions for biosurfactant production included 4% soybean oil as carbon source at pH 5.5 at 30 degrees C for 7d. Under these conditions, the surface tension of the medium decreased to 28mN/m with oil displacement measured at 69.43 cm(2). Comparative studies of biosurfactant production in media containing glucose or soybean oil were performed. The biosurfactants obtained were isolated and purified by chromatographic methods. The molecular weights of samples were further investigated by mass spectrometry. In medium containing glucose, biosurfactants of molecular weights of 675, 691, and 707 were obtained, while those isolated from medium containing soybean oil were of molecular weights of 658, 675, and 691. These results reveal that sophorolipid compounds containing fatty acids of C20 and C18:1 were produced from both media.
  • Hitoshi Ito, Reia Hosokawa, Masaaki Morikawa, Hidetoshi Okuyama
    INTERNATIONAL BIODETERIORATION & BIODEGRADATION 61 3 223 - 232 2008年04月 [査読有り][通常論文]
     
    A microbial consortium capable of degrading turbine oil (TuO), which consisted mainly of recalcitrant cycloalkanes and isoalkanes, was obtained from a soil sample collected from oil fields using repeated enrichment. When this consortium, named Atsuta A, was cultured in minimal salts medium containing 0.5% (w/v) TuO, it degraded 90% of TuO at 30 degrees C and pH 7 over 5 days. Although nine bacterial strains were isolated from the Atstita A consortium, TuO degradation by the individual isolates and by a mixture of them was negligible. The community structure of the consortium, which was investigated by PCR-denaturing gradient gel electrophoresis (DGGE) targeting 16S rRNA genes, changed significantly during the degradation of TuO. Four major bands (F, K, N and T) out of at least 23 DGGE bands significantly increased in intensity over time during incubation. The DGGE bands F, K and N corresponded to those of previously isolated species. However, DGGE band T did not correspond to any isolated strain. The 16S rRNA gene sequence collected from band T was 98% homologous to that of an unculturable strain belonging to the gamma-Proteobacteria. The degradation of TuO in the consortium may occur by cooperation between the unculturable species corresponding to band T and other strains in the consortium, including species corresponding to bands F, K and N. (C) 2007 Elsevier Ltd. All rights reserved.
  • 山賀文子, 鷲尾健司, 森川正章
    化学と生物 46 10 682 - 688 Japan Society for Bioscience, Biotechnology, and Agrochemistry 2008年 [査読有り][通常論文]
     
    微生物活性を利用した環境浄化法は,地球への負荷が少ない技術として広く認知されている.しかし,実用的技術としては,有用微生物の現場での定着率の低さによるコスト高や浄化後に危惧される微生物の異常増殖や生態系の攪乱などの問題が常に指摘されてきた.近年,この問題を解決する一つの方向性として根圏微生物の活用が注目されている.植物の光合成作用と微生物の汚染物質分解活性をリンクさせるこの手法の一例を紹介するとともに,今後の可能性を展望する.
  • Boonsri Jongsareejit, Amaret Bhumiratana, Masaaki Morikawa, Shigerri Kanaya
    ScienceAsia 33 4 389 - 395 2007年12月 [査読有り][通常論文]
     
    A 546-bp fragment of the sz-hasA gene encoding hyaluronan synthase (szHAS) from Streptococcus zooepidemicus (group C Streptococcus, GCS) was amplified by PCR with oligonucleotidesdesigned based on the conserved amino acid sequences of HASs from other organisms as primers. The entire sz-hasA gene was identified and cloned by Southern and colony hybridizations using this 546-bp fragment as a probe. Determination of the nucleotide sequence indicated that this gene encoded a protein with 417 amino acid residues (calculated molecular mass, 47.77 kDa). The amino acid sequence of szHAS was 74.2% identical to that of HAS from Strep. equisimilis. The overexpression of sz-hasA in Escherichia coli was detected by SDS-PAGE and confirmed by LC/MS-MS. To examine whether E. coli cells acquire an ability to synthesize hyaluronic acid (HA) upon transformation with plasmids bearing the sz-hasA gene, theplasmids pHAS-1 and pHAS-2, in which sz-hasA and sz-hasA with rare codon modifications at the 5′-terminus were ligated into the Ndel-BamHI sites of pET-28a, respectively, were constructed and used to transform E. coli BL21 (DE3), E. coli BL21 (codon+), and E. coli HMS 174 (DE3) plysS. Cultivation of these transformants, followed by induction for gene expression, revealed that the E. coli BL21 (codon+) transformants with pHAS-1 and E. coli HMS 174 (DE3) plysS transformants with pHAS-2 produced HA after 4 hr induction time at the maximum yield 16 μg/ml and 32.5 μg/ml, respectively. These are higher than the background levels in control bacteria, which were 5 μg/ml and 21.3 μg/ml, respectively.
  • Slew Ping Lim, Niran Roongsawang, Kenji Washio, Masaaki Morikawa
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 71 8 2002 - 2009 2007年08月 [査読有り][通常論文]
     
    Fluorescent Pseudomonas sp. MIS38 produces a cyclic lipopeptide, arthr4actin. Arthrofactin is synthesized by a unique nonribosomal peptide synthetase (NRPS) with dual C/E-domains. In this study, another class of cyclic peptide, pyoverdine, was isolated from MIS38, viz., Pvd38. The main fraction of Pvd38 had an m/z value of 1,064.57 and contained Ala, Glu, Gly, (OHOrn), Ser, and Thr at a ratio of 2:1:1:(1):1:1 in the peptide part, suggesting a new structure compound. A gene encoding NRPS for the chromophore part of Pvd38 was identified, and we found that it contained a conventional E-domain. Gene disruption completely impaired the production of Pvd38, demonstrating that the synthetase is functional. This observation allows us to conclude that different NRPS systems with dual C/Edomains (in arthrofactin synthetase) and a conventional E-domain (in pyoverdine synthetase) are both functional in MIS38.
  • Niran Roongsawang, Kenji Washio, Masaaki Morikawa
    CHEMBIOCHEM 8 5 501 - 512 2007年03月 [査読有り][通常論文]
     
    Mocrocyclization of a peptide or a lipopeptide occurs at the last step of synthesis and is usually catalyzed by a single C-terminal thioesterase (Te) domain. Arthrofactin synthetase WO from Pseudomonas sp. MIS38 represents a novel type of nonribosomal peptide synthetase that contains unique tandem C-terminal Te domains, ArfC_Te1 and ArfC_Te2. In order to analyze their function in vivo, site-directed mutagenesis was introduced at the putotive active-site residues in ArfC_Te1 and ArfC_Te2. It was found that both Te domains were functional. Peaks corresponding to arthrofactin and its derivatives were absent in ArfC_Te1.S89A, ArfC_Te1.-S89T, and ArfC_Te1:E26G/F27A mutants, and the production of arthrofactin by ArfC_7e2:S92A, ArfC_7e2:S92A/D118A, and AnFC Delta 7e2 was reduced by 95% without an alteration of the cyclic lipoundecapeptide structure. These results suggest that Ser89 in ArfC_Te1 is essential for the completion of macrocyclization and the release of product. Glu26 and Phe27 residues are also part of the active site of ArfC_Te1. ArfC_7e2 might hove been added during the evolution of Arf in order to improve macrocyclization efficiency.
  • バイオフィルムの功罪
    森川 正章
    食品衛生学雑誌 48 J389 - J396 2007年 [査読有り][通常論文]
  • Shin-ichi Hirano, Masaaki Morikawa, Kazufumi Takano, Tadayuki Imanaka, Shigenori Kanaya
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 71 1 192 - 199 2007年01月 [査読有り][通常論文]
     
    A putative gentisate 1,2-dioxygenase was encoded in the dibenzothiophene degradation gene cluster (dbd) from Xanthobacter polyaromaticivorans 127W. The deduced amino acid sequence showed high sequence similarity with gentisate dioxygenases from Pseudomonas alealigenes (AAD49427, 65% identical), Bradyrhizobium japonicum (NP766750, 64%), and P. aeruginosa (ZP_00135722, 54%), and moderate similarity with 1-hydroxy-2-naphthoate dioxygenase from Nocardioides sp. KP7 (BAA31235, 33%) and salicylate dioxygenase from Pseudaminobacter salicylatoxidans (AAQ91293, 33%). The enzyme, GDOxp, was heterologously produced in Escherichia coli and purified to homogeneity. GDOxp formed a tetramer and exhibited high dioxygenase activity against 1,4-dihydroxy 2-naphthoate as well as gentisate, suggesting unusually broad substrate specificity. GDOxp easily released ferrous ion under unfavorable temperature and pH conditions to become an inactive monomer protein. An inactive monomer protein can reconstitute a tetramer structure and restore enzyme activity in a cooperative manner upon the addition of ferrous ion. Chymotryptic digestion and protein truncation experiments suggested that the N-terminal region is important for the tetramerization of GDOxp.
  • Kenji Washio, Masaaki Morikawa
    BIOCHIMICA ET BIOPHYSICA ACTA-GENE STRUCTURE AND EXPRESSION 1759 10 478 - 490 2006年10月 [査読有り][通常論文]
     
    During germination of cereal seeds, aleurone cells respond to gibberellins (GA) by synthesizing and secreting hydrolytic enzymes that mobilize the reserved nutrients. It has been shown that products of early GA response genes, like a transcription factor GAMyb, act as key molecules leading to this regulation. Pivotal roles of GAMyb on expression of hydrolase genes have been well documented, whereas regulation of GAMyb expression itself remains obscure. In order to understand virtual mechanisms of the GA-mediated expression of genes, it is important to know how GA control expression of early GA response genes. Using an aleurone transient expression system of rice (Oryza sativa L.), we examined GA responsive domains of early GA response genes in the aleurone, such as GAMyb and OsDof3. The upstream promoter could not confer GA response. Extensive analyses revealed the presence of enhancer-like activities in a large first intron. In Arabidopsis, intron enhancers have been identified in MADS-box homeotic genes, AGAMOUS (AG) and FLOWERING LOCUS C (FLC), in which large introns should not only confer proper gene expressions, but also associate with gene silencing by covalent modifications of both DNA and historic. These evidences prompt us to assign that chromatin-based control might be important for initial GA action. Based on this assumption, we have identified DNA methylation of the GAMyb locus in germinated rice seeds. (c) 2006 Elsevier B.V All rights reserved.
  • Morikawa Masaaki, Kagihiro Shinji, Haruki Mitsuru, Takano Kazufumi, Branda Steve, Kolter Roberto, Kanaya Shigenori
    Microbiology 152 9 2801 - 2807 Society for General Microbiology 2006年09月 [査読有り][通常論文]
     
    The extracellular matrix produced by Bacillus subtilis B-1, an environmental strain that forms robust floating biofilms, was purified, and determined to be composed predominantly of -polyglutamate (-PGA), with a molecular mass of over 1000 kDa. Both biofilm formation and -PGA production by B. subtilis B-1 increased with increasing Mn2+ or glycerol concentration. -PGA was produced in a growth-associated manner in standing culture, and floating biofilms were formed. However, -PGA was produced in a non-growth-associated manner in shaking culture conditions. When B. subtilis B-1 was grown in a ...
  • Jiraporn Thaniyavarn, Aree Chongchin, Nopparat Wanitsuksombut, Suthep Thaniyavarn, Pairoh Pinphanichakarn, Natthanant Leepipatpiboon, Masaaki Morikawa, Shigenori Kanaya
    JOURNAL OF GENERAL AND APPLIED MICROBIOLOGY 52 4 215 - 222 2006年08月 [査読有り][通常論文]
     
    Biosurfactant production by Pseudomonas aeruginosa A41, a strain isolated from seawater in the gulf of Thailand, was examined when grown in defined medium containing 2% vegetable oil or fatty acid as a carbon source in the presence of vitamins, trace elements and,0.4% NH4NO3, at pH 7 and 30 C with 200 rpm-shaking for 7 days. The yield of biosurfactant steadily increased even after a stationary phase. Under such conditions the surface tension of the medium was lowered from 55-70 mN/m to 27.8-30 mN/m with every carbon source tested. However, types of carbon sources were found to affect biosurfactant yield. The yields of rhamnolipid biosurfactant were 6.58g/L, 2.91 g/L and 2.93g/L determined as rhamnose content when olive oil, palm oil and coconut oil, respectively, were used as a carbon source. Among them, biosurfactant obtained from palm oil was the best in lowering surface tension of the medium. Increase in biosurfactant activities in terms of oil displacement test and rhamnose, content were observed to be higher with shorter chain fatty acids than that of the longer chains (C12 > C14 > C16). In addition, we found that C18:2, highly unsaturated fatty acid, showed higher oil displacement activity and rhamnose content than that of C18:1. The optimal oil displacement activity was found at pH 7-9 and in the presence of 0.5-3% NaCl. The oil displacement activity was stable to temperatures up to 100 C for 15 h. Surface tension reduction activity was relatively stable at pH 2-12 and 0-5% of NaCl. Emusification activity tested with various types of hydrocarbons and vegetable oils showed similarity of up to 60% stability. The partially purified biosurfactant via TLC and silica gel column chromatography gave three main peaks on HPLC with mass spectra of 527, 272, and 661 m/z respectively, corresponding to sodium-monorhamnodecanoate, hydroxyhexadecanoic acid and an unknown compound, respectively.
  • M Pulido, K Saito, SI Tanaka, Y Koga, M Morikawa, K Takano, S Kanaya
    APPLIED AND ENVIRONMENTAL MICROBIOLOGY 72 6 4154 - 4162 2006年06月 [査読有り][通常論文]
     
    Subtilisin from the hyperthermophilic archaeon Thermococcus kodakaraensis KOD1 is a member of the subtilisin family. T. kodakaraensis subtilisin in a proform (T. kodakaraensis pro-subtilisin), as well as its propeptide (T. kodakaraensis propeptide) and mature domain (T. kodakaraensis mat-subtilisin), were independently overproduced in E. coli, purified, and biochemically characterized. T. kodakaraensis pro-subtilisin was inactive in the absence of Ca2+ but was activated upon autoprocessing and degradation of propeptide in the presence of Ca2+ at 80 degrees C. This maturation process was completed within 30 min at 80 degrees C but was bound at an intermediate stage, in which the propeptide is autoprocessed from the mature domain (T. kodakaraensis mat-subtilisin*) but forms an inactive complex with T. kodakaraensis mat-subtilisin*, at lower temperatures. At 80 degrees C, approximately 30% of T. kodakaraensis pro-subtilisin was autoprocessed into T. kodakaraensis propeptide and T. kodakaraensis mat-subtilisin*, and the other 70% was completely degraded to small fragments. Likewise, T. kodakaraensis mat-subtilisin was inactive in the absence of Ca2+ but was activated upon incubation with Ca2+ at 80 degrees C. The kinetic parameters and stability of the resultant activated protein were nearly identical to those of T. kodakaraensis mat-subtilisin*, indicating that T. kodakaraensis mat-subtilisin does not require T. kodakaraensis propeptide for folding. However, only similar to 5% of T. kodakaraensis mat-subtilisin was converted to an active form, and the other part was completely degraded to small fragments. T. kodakaraensis propeptide was shown to be a potent inhibitor of T. kodakaraensis mat-subtilisin* and noncompetitively inhibited its activity with a K-i of 25 +/- 3.0 nM at 20 degrees C. T. kodakaraensis propeptide may be required to prevent the degradation of the T. kodakaraensis mat-subtilisin molecules that are activated later by those that are activated earlier.
  • S Hirano, M Haruki, K Takano, T Imanaka, M Morikawa, S Kanaya
    APPLIED MICROBIOLOGY AND BIOTECHNOLOGY 69 6 672 - 681 2006年02月 [査読有り][通常論文]
     
    Xanthobacter polyaromaticivorans sp. nov. 127W is a bacterial strain that is capable of degrading a wide range of cyclic aromatic compounds such as dibenzothiophene, biphenyl, naphthalene, anthracene, and phenanthrene even under extremely low oxygen [dissolved oxygen (DO)<= 0.2 ppm] conditions (Hirano et al., Biosci Biotechnol Biochem 68:557-564, 2004). A major protein fraction carrying dibenzothiophene degradation activity was purified. Based on its partial amino acid sequences, dbdCa gene encoding alpha subunit terminal oxygenase (DbdCa) and its flanking region were cloned and sequenced. A phylogenetic analysis based on the amino acid sequence demonstrates that DbdCa is a member of a terminal oxygenase component of group IV ring-hydroxylating dioxygenases for biphenyls and monocyclic aromatic hydrocarbons, rather than group III dioxygenases for polycyclic aromatic hydrocarbons. Gene disruption in dbdCa abolished almost of the degradation activity against biphenyl, dibenzothiophene, and anthracene. The gene disruption also impaired degradation activity of the strain under extremely low oxygen conditions (DO <= 0.2 ppm). These results indicate that Dbd from 127W represents a group IV dioxygenase that is functional even under extremely low oxygen conditions.
  • 鷲尾健司, 森川正章
    化学と生物 44 2 85 - 92 Japan Society for Bioscience, Biotechnology, and Agrochemistry 2006年 [査読有り][通常論文]
  • 森川正章, 河合良尚, 相原 悠, 鷲尾健司, 高野和文, 金谷茂則
    生物工学会誌 84 12 488 - 490 日本生物工学会 2006年 [査読有り][通常論文]
  • T Yamamoto, T Matsuda, T Inoue, H Matsumura, M Morikawa, S Kanaya, Y Kai
    PROTEIN SCIENCE 15 1 152 - 161 2006年01月 [査読有り][通常論文]
     
    TATA-binding protein (TBP)-interacting protein from the hyperthermophilic archaeon Thermococcus kodakaraensis strain KODI (Tk-TIP26) is a possible transcription regulatory protein in Thermococcales. Here, we report the crystal structure of Tk-TIP26 determined at 2.3 angstrom resolution with multiple-wavelength anomalous dispersion (MAD) method. The overall structure of Tk-TIP26 consists of two domains. The N-terminal domain forms an alpha/beta structure, in which three alpha-helices enclose the central beta-sheet. The topology of this domain is similar to that of holliday junction resolvase Hjc from Pyrococcus furiosus. The C-terminal domain comprises three alpha-helices, six beta-strands, and two 3(10)-helices. In the dimer structure of Tk-TIP26, two molecules are related with the crystallographic twofold axis, and these molecules rigidly interact with each other via hydrogen bonds. The complex of Tk-TIP26/Tk-TBP is isolated and analyzed by SDS-PAGE and gel filtration column chromatography, resulting in a stoichiometric ratio of the interaction between Tk-TIP26 and Tk-TBP of 4:2, i.e., two dimer molecules of Tk-TIP26 formed a complex with one dimeric TBP. The electrostatic surfaces of Tk-TIP26 and TBP from Pyrocuccus woesei (PwTBP) allowed us to build a model of the Tk-TIP26/TBP complex, and to propose the inhibition mechanism where two dimer molecules of Tk-TIP26 bind to a dimeric TBP, preventing its binding to TATA-DNA.
  • M Morikawa
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 101 1 1 - 8 2006年01月 [査読有り][通常論文]
     
    Biofilms are densely packed multicellular communities of microorganisms attached to a surface or interface. Bacteria seem to initiate biofilm formation in response to specific environmental cues, such as nutrient and oxygen availability. Biofilms undergo dynamic changes during their transition from free-living organisms to sessile biofilm cells, including the specific production of secondary metabolites and a significant increase in the resistivity to biological, chemical, and physical assaults. Bacillus subtilis is an industrially important bacterium exhibiting developmental stages. It forms rough biofilms at the air-liquid interface rather than on the surface of a solid phase in a liquid, due to the aerotaxis of the cells. Biofilm formation by B. subtilis and related species permits the control of infection caused by plant pathogens, the reduction of mild steel corrosion, and the exploration of novel compounds. Although it is obviously important to control harmful biofilm formation, the exploitation of beneficial biofilms formed by such industrial bacteria may lead to a new biotechnology.
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  • N Roongsawang, SP Lim, K Washio, K Takano, S Kanaya, M Morikawa
    FEMS MICROBIOLOGY LETTERS 252 1 143 - 151 2005年11月 [査読有り][通常論文]
     
    Condensation (C) domains in the nonribosomal peptide synthetases are capable of catalyzing peptide bond formation between two consecutively bound various amino acids. C-domains coincide in frequency with the number of peptide bonds in the product peptide. In this study, a phylogenetic approach was used to investigate structural diversity of bacterial C-domains. Phylogenetic trees show that the C-domains are clustered into three functional groups according to the types of substrate donor molecules. They are L-peptidyl donors, D-peptidyl donors, and N-acyl donors. The fact that C-domain structure is not subject to optical configuration of amino acid acceptor molecules supports an idea that the conversion from L to D-form of incorporating amino acid acceptor occurs during or after peptide bond formation. L-peptidyl donors and D-peptidyl donors are suggested to separate before separating the lineage of Gram-positive and Gram-negative bacteria in the evolution process. (c) 2005 Federation of European Microbiological Societies. Published by Elsevier B.V. All rights reserved.
  • Y Suzuki, Y Mizutani, T Tsuji, N Ohtani, K Takano, M Haruki, M Morikawa, S Kanaya
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 69 2 364 - 373 2005年02月 [査読有り][通常論文]
     
    The gene encoding alkaline phosphatase from the psychrotrophic bacterium Shewanella sp. SIB1 was cloned, sequenced, and overexpressed in Escherichia coli. The recombinant protein was purified and its enzymatic properties were compared with those of E. coli alkaline phosphatase (APase), which shows an amino acid sequence identity of 37%. The optimum temperature of SIB1 APase was 50degreesC, lower than that of E. coli APase by 30degreesC. The specific activity of SIB1 APase at 50degreesC was 3.1 fold higher than that of E. coli APase at 80degreesC. SIB1 APase lost activity with a half-life of 3.9min at 70degreesC, whereas E. coli APase lost activity with a half-life of >6h even at 80degreesC. Thus SIB1 APase is-well adapted to low temperatures. Comparison of the amino acid sequences of SIB1 and E. coli APases suggests that decreases in electrostatic interactions and number of disulfide bonds are responsible for the cold-adaptation of SIB1 APase.
  • N Kunihiro, M Haruki, K Takano, M Morikawa, S Kanaya
    JOURNAL OF BIOTECHNOLOGY 115 2 129 - 136 2005年01月 [査読有り][通常論文]
     
    Branched alkanes including 2,6,10,14-tetramethylpentadecane (pristane) are more resistant to biological degradation than straight-chain alkanes especially under low-temperature conditions, such as 10 degreesC. Two bacterial strains, TMP2 and T12, that are capable of degrading pristane at 10 degreesC were isolated and characterized. Both strains grew optimally at 30 degreesC and were identified as Rhodococcus sp. based on the 16S rRNA gene sequences. Strain T12 degraded comparable amounts of pristane in a range of temperatures from 10 to 30 degreesC and strain TMP2 degraded pristane similarly at 10 and 20 degreesC but did not degrade it at 30 degreesC. These data suggest that the strains have adapted their pristane degradation system to moderately low-temperature conditions. (C) 2004 Elsevier B.V. All rights reserved.
  • Kitauchi F, Hirano S, Haruki M, Imanaka T, Morikawa M, Kanaya S
    J. Environ. Biotechnol 4 2 117 - 120 環境バイオテクノロジー学会 2005年 [査読有り][通常論文]
  • Toshihiko Akiba, Noriyuki Ishii, Naeem Rashid, Masaaki Morikawa, Tadayuki Imanaka, Kazuaki Harata
    Nucleic acids research 33 10 3412 - 23 2005年 [査読有り][通常論文]
     
    The X-ray crystal structure of RadB from Thermococcus kodakaraensis KOD1, an archaeal homologue of the RecA/Rad51 family proteins, have been determined in two crystal forms. The structure represents the core ATPase domain of the RecA/Rad51 proteins. Two independent molecules in the type 1 crystal were roughly related by 7-fold screw symmetry whereas non-crystallographic 2-fold symmetry was observed in the type 2 crystal. The dimer structure in the type 1 crystal is extended to construct a helical assembly, which resembles the filamentous structures reported for other RecA/Rad51 proteins. The molecular interface in the type 1 dimer is formed by facing a basic surface patch of one monomer to an acidic one of the other. The empty ATP binding pocket is located at the interface and barely concealed from the outside similarly to that in the active form of the RecA filament. The model assembly has a positively charged belt on one surface bordering the helical groove suitable for facile binding of DNA. Electron microscopy has revealed that, in the absence of ATP and DNA, RadB forms a filament with a similar diameter to that of the hypothetical assembly, although its helical properties were not confirmed.
  • A Mukaiyama, K Takano, M Haruki, M Morikawa, S Kanaya
    BIOCHEMISTRY 43 43 13859 - 13866 2004年11月 [査読有り][通常論文]
     
    Equilibrium and kinetic studies were carried out under denaturation conditions to clarify the energetic features of the high stability of a monomeric protein, ribonuclease HIT, from a hyperthermophile, Thermococcus kodakaraensis (Tk-RNase HII). Guanidine hydrochloride (GdnHCl)-induced unfolding and refolding were measured with circular dichroism at 220 nm, and heat-induced denaturation was studied with differential scanning calorimetry. Both GdnHCl- and heat-induced denaturation are very reversible. It was difficult to obtain the equilibrated unfolding curve of Tk-RNase HIT below 40 degreesC, because of the remarkably slow unfolding. The two-state unfolding and refolding reactions attained equilibrium at 50 degreesC after 2 weeks. The Gibbs energy change of GdnHCl-induced unfolding (DeltaG(H2O)) at 50 degreesC was 43.6 kJ mol(-1). The denaturation temperature in the DSC measurement shifted as a function of the scan rate; the denaturation temperature at a scan rate of 90 degreesC h(-1) was higher than at a scan rate of 5 degreesC h(-1). The unfolding and refolding kinetics of Tk-RNase HIT were approximated as a first-order reaction. The ln k(u) and ln k(r) values depended linearly on the denaturant concentration between 10 and 50 degreesC. The DeltaG(H2O) value obtained from the rate constant in water using the two-state model at 50 degreesC, 44.5 kJ mol(-1), was coincident with that from the equilibrium study, 43.6 kJ mol(-1), suggesting the two-state folding of Tk-RNase HII. The values for the rate constant in water of the unfolding for Tk-RNase HII were much smaller than those of E. coli RNase HI and Thermus thermophilus RNase HI, which has a denaturation temperature similar to that of Tk-RNase HII. In contrast, little difference was observed in the refolding rates among these proteins. These results indicate that the stabilization mechanism of monomeric protein from a hyperthermophile, Tk-RNase HII, with reversible two-state folding is characterized by remarkably slow unfolding.
  • Cornista J, Ikeuchi S, Haruki M, Kohara A, Takano K, Morikawa M, Kanaya S
    Biosci. Biotechnol. Biochem. 68 10 2128 - 2137 2004年10月 [査読有り][通常論文]
     
    Pitrilysin from Escherichia coli was overproduced, purified, and analyzed for enzymatic activity using 14 peptides as a substrate. Pitrilysin cleaved all the peptides, except for two of the smallest, at a limited number of sites, but showed little amino acid specificity. It cleaved beta-endorphin (beta-EP) most effectively, with a K-m value of 0.36 mum and a k(cat) value of 750 min(-1). beta-EP consists of 31 residues and was predominantly cleaved by the enzyme at Lys(19)-Asn(20). Kinetic analyses using a series of beta-EP derivatives with N and/or C-terminal truncations and with amino acid substitutions revealed that three hydrophobic residues (Leu(14), Val(15), and Leu(17)) and the region 22-26 in beta-EP are responsible for high-affinity recognition by the enzyme. These two regions are located on the N- and C-terminal sides of the cleavage site in beta-EP, suggesting that the substrate binding pocket of pitrilysin spans its catalytic site.
  • H Chon, R Nakano, N Ohtani, M Haruki, K Takano, M Morikawa, S Kanaya
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 68 10 2138 - 2147 2004年10月 [査読有り][通常論文]
     
    The gene encoding RNase HIII from the thermophilic bacterium Bacillus stearothermophilus was cloned and overexpressed in Escherichia coli, and the recombinant protein (Bst-RNase HIII) was purified and biochemically characterized. Bst-RNase HIII is a monomeric protein with 310 amino acid residues, and shows an amino acid sequence identity of 47.1% with B. subtilis RNase HIII (Bsu-RNase HIII). The enzymatic properties of Bst-RNase HIII, such as pH optimum, metal ion requirement, and cleavage mode of the substrates, were similar to those of Bsu-RNase HIII However, Bst-RNase HIII was more stable than Bsu-RNase HIII, and the temperature (T-1/2) at which the enzyme loses half of its activity upon incubation for 10min was 55degreesC for Bst-RNase HIII and 35degreesC for Bsu-RNase HIII. The optimum temperature for Bst-RNase HIII activity was also shifted upward by roughly 20degreesC as compared to that of Bsu-RNase HIII. The availability of such a thermostable enzyme will facilitate structural studies of RNase HIII.
  • K Takano, M Saito, M Morikawa, S Kanaya
    JOURNAL OF BIOCHEMISTRY 135 6 701 - 708 2004年06月 [査読有り][通常論文]
     
    It is known that several naturally occurring substances known as osmolytes increase the conformational stability of proteins. Bolen and co-worker proposed the osmophobic theory, which asserts the osmolyte effect occurs because of an unfavorable interaction of osmolytes mainly with the protein backbone, based on the results on the transfer Gibbs energy of amino acids (Deltag) [Bolen and Baskakov (2001) J. Mol. Biol. 310, 955-963]. In this paper, we report the effect of sarcosine on the conformational stability (DeltaG) of RNase Sa (96 residues and one disulfide bond) and four mutant proteins. The thermal denaturation curves for RNase Sa in sarcosine fitted a two-state model on nonlinear least-squares analysis. All the RNase Sa proteins were stabilized by sarcosine. For example, the increase in stability of the wild-type protein in 4 M sarcosine due to the osmolyte effect (Delta(o)DeltaG) is 3.2 kcal/mol. Mutational analysis of the osmolyte effect indicated that the changed Delta(o)DeltaG values upon mutation (Delta(m)Delta(o)DeltaG), as estimated from the Deltag values, are similar to the experimental values. Structural-based analysis of the osmolyte effect was also performed using model denatured structures: (a) a fully extended model (single chain) with no disulfide bond, (b) two-part, unfolded models (two chains) with a disulfide bond constructed through molecular dynamic (MD) simulation, and (c) a two-part, folded model (two chains). The two-part, unfolded models were expected to be more suitable as denatured structures. The Delta(o)DeltaG values calculated using the two-part, unfolded models were more consistent with experimental values than those calculated using the fully extended and two-part, folded models. This suggests that MD simulation is useful for testing denatured structures. These results indicate that the osmophobic theory can explain the osmolyte effect on protein stability.
  • Y Suzuki, M Haruki, K Takano, M Morikawa, S Kanaya
    EUROPEAN JOURNAL OF BIOCHEMISTRY 271 7 1372 - 1381 2004年04月 [査読有り][通常論文]
     
    A psychrotrophic bacterium Shewanella sp. strain SIB1 was grown at 4 and 20 degreesC, and total soluble proteins extracted from the cells were analyzed by two-dimensional polyacrylamide gel electrophoresis. Comparison of these patterns showed that the cellular content of a protein with a molecular mass of 28 kDa and an isoelectric point of four greatly increased at 4 degreesC compared to that at 20 degreesC. Determination of the N-terminal amino acid sequence, followed by the cloning and sequencing of the gene encoding this protein, revealed that this protein is a member of the FKBP family of proteins with an amino acid sequence identity of 56% to Escherichia coli FKBP22. This protein was overproduced in E. coli in a His-tagged form, purified, and analyzed for peptidyl-prolyl cis-trans isomerase activity. When this activity was determined by the protease coupling assay using N-succinyl-Ala-Leu-Pro-Phe-p-nitroanilide as a substrate at various temperatures, the protein exhibited the highest activity at 10 degreesC with a k(cat)/K-m value of 0.87 muM(-1).s(-1). When the peptidyl-prolyl cis-trans isomerase activity was determined by the RNase T-1 refolding assay at 10 and 20 degreesC, the protein exhibited higher activity at 10 degreesC with a k(cat)/K-m value of 0.50 muM(-1).s(-1). These k(cat)/K-m values are lower but comparable to those of E. coli FKBP22. We propose that a FKBP family protein is involved in cold-adaptation of psychrotrophic bacteria.
  • SI Hirano, F Kitauchi, M Haruki, T Imanaka, M Morikawa, S Kanaya
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 68 3 557 - 564 2004年03月 [査読有り][通常論文]
     
    Two bacterial strains, 127W and T102, were isolated from anoxic crude oil tank sludge as effective degraders of dibenzothiophene (DBT), a model sulfur containing heterocyclic aromatic compound in crude oil. Strain 127W was more tolerant to oxygen limitation than T102 and was capable of degrading two- and three-ring polycyclic and heterocyclic aromatic compounds under both aerobic and low oxygen conditions. Strain 127W degraded 0.082, 0.055, and 0.064 mm of DBT, naphthalene, and anthracene, respectively, in one week with dissolved oxygen </=0.2ppm (0.006mm). Degradation by 127W cell-free extracts for DBT was increased by addition of sodium hydrogencarbonate under this oxygen concentration. Phylogenetic analysis of the 16S rRNA gene sequence and physiological characteristics indicate that the strains 127W and T102 belong to new species of the genus Xanthobacter and Pseudomonas stutzeri, respectively. We propose X. polyaromaticivorans sp. nov. 127W.
  • 次世代のペプチド合成法
    森川正章, 金谷茂則
    日本化学会バイオテクノロジー部会ニュースレター 8 5 - 7 2004年 [査読有り][通常論文]
  • Haruyuki Atomi, Toshiaki Fukui, Tamotsu Kanai, Masaaki Morikawa, Tadayuki Imanaka
    Archaea 1 4 263 - 267 2004年 [査読有り][通常論文]
     
    A hyperthermophilic archaeal strain, KOD1, isolated from a solfatara on Kodakara Island, Japan, has previously been reported as Pyrococcus sp. KOD1. However, a detailed phylogenetic tree, made possible by the recent accumulation of 16S rRNA sequences of various species in the order Thermococcales, indicated that strain KOD1 is a member of the genus Thermococcus. We performed DNA-DNA hybridization tests against species that displayed high similarity in terms of 16S ribosomal DNA sequences, including Thermococcus peptonophilus and Thermococcus stetteri. Hybridization results and differences in growth characteristics and substrate utilization differentiated strain KOD1 from T. peptonophilus and T. stetteri at the species level. Our results indicate that strain KOD1 represents a new species of Thermococcus, which we designate as Thermococcus kodakaraensis KOD1 sp. nov.
  • N Roongsawang, K Hase, M Haruki, T Imanaka, M Morikawa, S Kanaya
    CHEMISTRY & BIOLOGY 10 9 869 - 880 2003年09月 [査読有り][通常論文]
     
    Arthrofactin is a potent cyclic lipopeptide-type biosurfactant produced by Pseudomonas sp. MIS38. In this work, an arthrofactin synthetase gene cluster (arf) spanning 38.7 kb was cloned and characterized. Three genes termed arfA, arfB, and arfC encode ArfA, ArfB, and ArfC, containing two, four, and five functional modules, respectively. Each module bears condensation, adenylation, and thiolation domains, like other nonribosomal peptide synthetases. However, unlike most of them, none of the 11 modules possess the epimerization domain responsible for the conversion of amino acid residues from L to D form. Possible L-and D-Leu adenylation domains specifically recognized only L-Leu. Moreover, two thioesterase domains are tandemly located at the C-terminal end of ArfC. These results suggest that ArfA, ArfB, and ArfC assemble to form a unique structure. Gene disruption of arfB impaired arthrofactin production, reduced swarming activity, and enhanced biofilm formation.
  • J Thaniyavarn, N Roongsawang, T Kameyama, M Haruki, T Imanaka, M Morikawa, S Kanaya
    BIOSCIENCE BIOTECHNOLOGY AND BIOCHEMISTRY 67 6 1239 - 1244 2003年06月 [査読有り][通常論文]
     
    A biosurfactant-producing strain, Bacillus licheniformis F2.2, was isolated from a fermented food in Thailand. The strain was capable of producing a new biosurfactant, BL1193, as well as two kinds of popular lipopeptide biosurfactants, plipastatin and surfactin. Mass spectrometry and FT-IR analysis indicated that BL1193 had a molecular mass of 1,193 Da with no peptide portion in the molecule. While plipastatin and surfactin were abundantly produced in a nutrient YPD medium, BL1193 was produced only in a synthetic DF medium containing no amino acids. According to an oil displacement activity test, the specific activity of BL1193 (6.53 kBS units/mg) is equivalent to that of surfactin (5.78-6.83 kBS units/mg).
  • Y Tsunaka, M Haruki, M Morikawa, M Oobatake, S Kanaya
    BIOCHEMISTRY 42 11 3366 - 3374 2003年03月 [査読有り][通常論文]
     
    The activities of the eight mutant proteins of Escherichia coli RNase HI, in which the four carboxylic amino acids (Asp(10), Glu(48), Asp(70), and Asp(134)) involved in catalysis are changed to Asn (Gln) or Ala, were examined in the presence of Mn2+. Of these proteins, the E48A, E48Q, D134A, and D134N proteins exhibited the activity, indicating that Glu(48) and Asp(134) are dispensable for Mn2+-dependent activity. The maximal activities of the E48A and D134A proteins were comparable to that of the wild-type protein. However, unlike the wild-type protein, these mutant proteins exhibited the maximal activities in the presence of > 100 muM MnCl2, and their activities were not inhibited at higher Mn2+ concentrations (up to 10 mM). The wild-type protein contains two Mn2+ binding sites and is activated upon binding of one Mn2+ ion at site 1 at low (similar to1 muM) Mn2+ concentrations. This activity is attenuated upon binding of a second Mn2+ ion at site 2 at high (> 10 muM) Mn2+ concentrations. The cleavage specificities of the mutant proteins, which were examined using oligomeric substrates at high Mn2+ concentrations, were identical to that of the wild-type protein at low Mn2+ concentrations but were different from that of the wild-type protein at high Mn2+ concentrations. These results suggest that one Mn2+ ion binds to the E48A, E48Q, D134A, and D134N proteins at site 1 or a nearby site with weaker affinities. The binding analyses of the Mn2+ ion to these proteins in the absence of the substrate support this hypothesis. When Mn2+ ion is used as a metal cofactor, the Mn2+ ion itself, instead of Glu(48) and Asp(134), probably holds water molecules required for activity.
  • T Yamamoto, T Matsuda, N Sakamoto, H Matsumura, T Inoue, M Morikawa, S Kanaya, Y Kai
    ACTA CRYSTALLOGRAPHICA SECTION D-BIOLOGICAL CRYSTALLOGRAPHY 59 2 372 - 374 2003年02月 [査読有り][通常論文]
     
    The 26 kDa TBP (TATA-binding protein) interacting protein from the hyperthermophilic archaeon Thermococcus kodakaraensis KOD1 (Tk-TIP26) is a possible transcriptional regulatory protein in Thermococcales. Here, the crystallization of both the native and selenomethionine-substituted proteins and data collection are described. The native crystals belong to the tetragonal space group P4(1)2(1)2 or P4(3)2(1)2, with unit-cell parameters a = 73.83, c = 86.41 Angstrom, and diffract to 2.2 Angstrom using synchrotron radiation. MAD data was collected and a Bijvoet difference Patterson map showed strong peaks sufficient to determine the positions of the Se atoms.
  • 掘り起こせ宝の山−微生物のしたたかな戦略バイオフィルム
    森川 正章
    バイオサイエンスとインダストリー 61 2003年 [査読有り][通常論文]
  • 森川 正章
    化学と生物 41 1 32 - 37 Japan Society for Bioscience, Biotechnology, and Agrochemistry 2003年 [査読有り][通常論文]
  • H Adachi, K Takano, M Morikawa, S Kanaya, M Yoshimura, Y Mori, T Sasaki
    ACTA CRYSTALLOGRAPHICA SECTION D-BIOLOGICAL CRYSTALLOGRAPHY 59 Pt1 194 - 196 2003年01月 [査読有り][通常論文]
     
    A new method of protein crystallization, the floating-drop vapour-diffusion technique, has been developed. The method combines the traditional sitting-drop vapour-diffusion technique and a novel two-liquid system. A crystallization drop composed of a mixture of sample and reagent floats on an insoluble and very dense liquid. Protein crystals are grown by vapour diffusion at the interface of the two liquids. The method makes it possible to remove the crystals easily without causing mechanical damage. This approach also significantly reduces the time and cost compared with the hanging-drop technique, which is presently the most popular method for protein crystallization.
  • Adachi H, Takano K, Hosokawa Y, Inoue T, Mori Y, Matsumura H, Yoshimura M, Tsunaka Y, Morikawa M, Kanaya S, Masuhara H, Kai Y, Sasaki T
    Jpn. J. Appl. Phys. 42 7B L798 - L800 Japan Society of Applied Physics 2003年 [査読有り][通常論文]
     
    We succeeded in the first ever generation of protein crystals by laser irradiation. We call this process Laser Irradiated Growth Technique (LIGHT). Effective crystallization was confirmed by applying an intense femtosecond laser. The crystallization period was dramatically shortened by LIGHT. In addition, protein crystals were obtained by LIGHT from normally uncrystallized conditions. These results indicate that intense femtosecond laser irradiation generates crystal nuclei; protein crystals can then be grown from the nuclei that act as seeds in a supersaturated solution. The nuclei formation is possible primarily due to nonlinear nucleation processes of an intense femtosecond laser with a peak intensity of over a gigawatt (GW).
  • 向山 厚, 高野 和文, 春木 満, 森川 正章, 金谷 茂則
    生物物理 43 S68  一般社団法人 日本生物物理学会 2003年
  • N Roongsawang, J Thaniyavarn, S Thaniyavarn, T Kameyama, M Haruki, T Imanaka, M Morikawa, S Kanaya
    EXTREMOPHILES 6 6 499 - 506 2002年12月 [査読有り][通常論文]
     
    Twenty-three halotolerant and biosurfactant producing strains were collected from salty conditions in central Thailand. One of the strains designated BBK-1 produced the biosurfactants with the highest activity. BBK-1 was isolated from fermented foods and was identified as B. subtilis based on its physiological characteristics and 16S rRNA gene sequence. We show that the strain grows in media containing NaCl up to 16% (w/v) and produces biosurfactants in NaCl up to 8%. We found that B. subtilis BBK-1 produces three kinds of surface-active lipopeptides simultaneously. By their respective molecular weights and amino acid compositions, it is indicated that these lipopeptides are bacillomycin L, plipastatin, and surfactin. In order to analyze the production mechanism of lipopeptides further in the strain, a generally important biosynthetic gene encoding 4'-phosphopantetheinyl transferase was cloned and sequenced. The gene existed in a single copy in the genome and the deduced amino acid sequence was almost identical to that of Lpa-14 from B. subtilis strain RB14, which co-produces iturin A and surfactin.
  • T Kanamori, N Rashid, M Morikawa, H Atomi, T Imanaka
    FEMS MICROBIOLOGY LETTERS 217 2 255 - 261 2002年12月 [査読有り][通常論文]
     
    A Gram-negative bacterium was previously isolated from an oil field in Shizuoka, Japan, and designated strain HD-1. Here we have performed detailed characterization of the strain, and have found that it represents a novel genus. The 16S rRNA sequence of strain HD-1 displayed highest similarity to various uncultured species (86.7 similar to 99.7%), along with 86.2 similar to 88.2% similarity to sequences from Azospirillum, Methylobacterium, Rhizobium, and Hyphomicrobium, all members of the alpha-Proteobacteria. Phylogenetic analysis revealed that HD-1 represented a deep-branched lineage among the alpha-Proteobacteria. DNA-DNA hybridization analysis with Azospirillum lipoferum and Hyphomicrobium vulgare revealed low levels of similarity among the strains. We further examined the biochemical properties of the strain under aerobic conditions. Among carbon sources, ethanol, n-propanol, n-butanol, and n-tetradecanol were the most preferred, while acetate, propionate, and pyruvate also supported high levels of growth. The strain could also grow on aromatic compounds such as toluene, benzene and phenol, and aliphatic hydrocarbons such as n-octane and n-tetradecane. In contrast, glycerol and various sugars, including glucose, fructose, maltose, and lactose, failed to support growth of HD-1. Under an anaerobic gas phase with butanol as the carbon source, little increase in cell weight was observed with the addition of several possible electron acceptors. As strain HD-1 represents a novel genus in the a-Proteobacteria, we designated the strain as Oleomonas sagaranensis gen. nov., sp. nov., strain HD-1. (C) 2002 Federation of European Microbiological Societies. Published by Elsevier Science B.V. All rights reserved.
  • M Haruki, Y Tsunaka, M Morikawa, S Kanaya
    FEBS LETTERS 531 2 204 - 208 2002年11月 [査読有り][通常論文]
     
    We have analyzed the cleavage specificities of various prokaryotic Type 2 ribonucleases H (RNases H) on chimeric DNA-RNA-DNA/DNA substrates containing one to four ribonucleotides. RNases HII from Bacillus subtilis and Thermococcus kodakaraensis cleaved all of these substrates to produce a DNA segment with a 5'-monoribonucleotide. Consequently, these enzymes cleaved even the chimeric substrate containing a single ribonucleotide at the DNA-RNA junction (5'-side of the single ribonucleotide). In contrast, Escherichia coli RNase HI and B. subtilis RNase HIII did not cleave the chimeric substrate containing a single ribonucleotide. These results suggest that bacterial and archaeal RNases MI are involved in excision of a single ribonucleotide misincorporated into DNA. (C) 2002 Federation of European Biochemical Societies. Published by Elsevier Science B.V. All rights reserved.
  • H Chon, Y Tsunaka, M Haruki, M Morikawa, S Kanaya
    PROTEIN ENGINEERING 15 8 683 - 688 2002年08月 [査読有り][通常論文]
     
    A series of DNA-linked RNases H, in which the 15-mer DNA is cross-linked to the Thermus thermophilus RNase HI (TRNH) variants at positions 135, 136, 137 and 138, were constructed and analyzed for their abilities to cleave the complementary 15-mer RNA. Of these, that with the DNA adduct at position 135 most efficiently cleaved the RNA substrate, indicating that position 135 is the most appropriate cross-linking site among those examined. To examine whether DNA-linked RNase H also site-specifically cleaves a highly structured natural RNA, DNA-linked TRNHs with a series of DNA adducts varying in size at position 135 were constructed and analyzed for their abilities to cleave MS2 RNA. These DNA adducts were designed such that DNA-linked enzymes cleave MS2 RNA at a loop around residue 2790. Of the four DNA-linked TRNHs with the 8-, 12-, 16- and 20-mer DNA adducts, only that with the 16-mer DNA adduct efficiently and site-specifically cleaved MS2 RNA. Primer extension revealed that this DNA-linked TRNH cleaved MS2 RNA within the target sequence.
  • HJ Kwon, M Haruki, M Morikawa, K Omori, S Kanaya
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 93 2 157 - 164 2002年02月 [査読有り][通常論文]
     
    A family 1.3 lipase from Pseudomonas sp. MIS38 (PML) contains 12 repeats of a nine-residue sequence motif in the C-terminal region. To elucidate the role of these repetitive sequences, mutant proteins PML5, PML4, PML1, and PML0, in which 7, 8, 11, and all 12 of the repetitive sequences are deleted, and PMLDelta19, in which 19 C-terminal residues are truncated, were constructed. Escherichia coli DH5 cells carrying the Serratia marcescens Lip system permitted the secretion of the wild-type and all of the mutant proteins except for PMLDelta19, although they were partially accumulated in the cells in an insoluble form as well. Both the secretion level and cellular content of the proteins decreased in the order PML>PML5>PML4>PML1>PML0, indicating that repetitive sequences are not required for secretion of PML but are important for its stability in the cells. All the mutant proteins were purified in a refolded form and their biochemical properties were characterized. CD spectra, the Ca2+ contents, and susceptibility to chymotryptic digestion strongly suggested that the five repetitive sequences remaining in PML5 are sufficient to form a P-roll structure, whereas the four in PML4 are not. PML5 and PMLDelta19 showed both lipase and esterase activities, whereas PML4, PML1, and PML0 were inactive. These results suggest that the enzymatic activity of PML is not seriously affected by a deletion or truncation at the C-terminal region as long as a succession of repetitive sequences can build a beta-roll structure.
  • A Muroya, R Nakano, N Ohtani, M Haruki, M Morikawa, S Kanaya
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 93 2 170 - 175 2002年02月 [査読有り][通常論文]
     
    The gene encoding ribonuclease HII from Bacillus stearothermophilus was cloned and expressed in Escherichia coli. The overproduced protein, Bst-RNase HII, was purified and biochemically characterized. Bst-RNase HII, which consists of 259 amino acid residues, showed the highest amino acid sequence identity (50.2%) to Bacillus subtilis R-Nase HII. Like B. subtilis RNase HII, it exhibited Mn2+-dependent RNase H activity. It was, however, more thermostable than B. subtilis RNase HII. When the Bst-RNase HII amino acid sequence is compared with that of Thermococcus kodakaraensis RNase HII, to which it shows 29.8% identity, 30 residues are observed to be truncated from the C-terminus and there is an extension of 71 residues at the N-terminus. The C-terminal truncation results in the loss of the alpha9 helix, which is rich in basic amino acid residues and is therefore important for substrate binding. A truncated protein, Delta59-Bst-RNase HII, in which most of the N-terminal extension was removed, completely lost its RNase H activity. Surface plasmon resonance analysis indicated that this truncated protein did not bind to the substrate. These results suggest that the N-terminal extension of Bst-RNase HII is important for substrate binding. Because B. subtilis RNase HII has an N-terminal extension of the same length and these extensions contain a region in which basic amino acid residues are clustered, the Bacillus enzymes may represent a novel type of RNase H which possesses a substrate-binding domain at the N-terminus.
  • 特殊環境微生物の環境修復への応用と限界
    森川 正章
    創造と実践—大阪大学全学共通教育機構— 2 66 - 71 2002年 [査読有り][通常論文]
  • N Ohtani, M Haruki, M Morikawa, S Kanaya
    PROTEIN ENGINEERING 14 12 975 - 982 2001年12月 [査読有り][通常論文]
     
    The rnhA gene encoding RNase HI from a psychrotrophic bacterium, Shewanella sp. SIB1, was cloned, sequenced and overexpressed in an rnh mutant strain of Escherichia coli. SIB1 RNase HI is composed of 157 amino acid residues and shows 63% amino acid sequence identity to E.coli RNase HI. Upon induction, the recombinant protein accumulated in the cells in an insoluble form. This protein was solubilized and purified in the presence of 7 M urea and refolded by removing urea. Determination of the enzymatic activity using M13 DNA-RNA hybrid as a substrate revealed that the enzymatic properties of SIB 1 RNase HI, such as divalent cation requirement, pH optimum and cleavage mode of a substrate, are similar to those of E.coli RNase HI. However, SIB1 RNase HI was much less stable than E.coli RNase HI and the temperature (T-1/2) at which the enzyme loses half of its activity upon incubation for 10 min was similar to25degreesC for SIB1 RNase HI and similar to60degreesC for E.coli RNase HI. The optimum temperature for the SIB1. RNase HI activity was also shifted downward by 20 C compared with that of E.coli RNase HI. Nevertheless, SIB1. RNase HI was less active than E.coli RNase HI even at low temperatures. The specific activity determined at 10 C was 0.29 units/mg for SIB1 RNase HI and 1.3 units/mg for E.coli RNase HI. Site-directed mutagenesis studies suggest that the amino acid substitution in the middle of the alphaI-helix (Pro52 for SIB1 RNase HI and Ala52 for E.coli RNase HI) partly accounts for the difference in the stability and activity between SIB1 and E.coli RNases HI.
  • K Amada, HJ Kwon, M Haruki, M Morikawa, S Kanaya
    FEBS LETTERS 509 1 17 - 21 2001年11月 [査読有り][通常論文]
     
    In order to understand a role of the Ca2+ ion on the structure and function of a Ca2+-dependent family 1.3 lipase from Pseudomonas sp. MIS38, apo-PML, holo-PML, holo-PML*, and the N-terminal domain alone (N-fragment) were prepared and biochemically characterized. Apo-PML and holo-PML represent refolded proteins in the absence and presence of the Ca2+ ion, respectively. Holo-PML* represents a holo-PML dialyzed against 20 mM Tris-HCl (pH 7.5). The results suggest that the C-terminal domain of PML is almost fully unfolded in the apo-form and its folding is induced by Ca2+ binding. The folding of this C-terminal domain may be required to make a conformation of the N-terminal catalytic domain functional. (C) 2001 Federation of European Biochemical Societies. Published by Elsevier Science B.V. All rights reserved.
  • T Kato, M Haruki, T Imanaka, M Morikawa, S Kanaya
    APPLIED MICROBIOLOGY AND BIOTECHNOLOGY 55 6 794 - 800 2001年06月 [査読有り][通常論文]
     
    Four psychrotrophic strains, which grew at 4 degreesC but not at 37 degreesC, were isolated from Japanese oil-reservoir water (strains SIB1, SIC1, SIS1) and Canadian oil sands (strain CAB1). Strains SIB1, SIS1, and CAB1 had a maximum growth rate at 20 degreesC and grew to the highest cell densities at the cultivation temperature of 0-4 degreesC. Strain SIS1 was capable of growing even at -5 degreesC. The growth profile of strain SIC I was rather similar to that of a mesophilic bacterium. Strains SIB1, SIC1, and SIS1 were identified as members of the genus Shewanella, and strain CAB1 was a member of the genus Arthrobacter. All these strains exhibited weak degradation ability against catechol, a hydroxylated aromatic hydrocarbon, and tributyrin. These strains are expected to be of potential use in the in situ bioremediation technology of hazardous hydrocarbons and esters under low-temperature conditions.
  • Y Kannan, Y Koga, Y Inoue, M Haruki, M Takagi, T Imanaka, M Morikawa, S Kanaya
    APPLIED AND ENVIRONMENTAL MICROBIOLOGY 67 6 2445 - 2452 2001年06月 [査読有り][通常論文]
     
    The gene encoding subtilisin-like protease T, kodakaraensis subtilisin was cloned from a hyperthermophilic archaeon Thermococcus kodakaraensis KOD1. T. kodakaraensis subtilisin is a member of the subtilisin family and composed of 422 amino acid residues with a molecular weight of 43,783, It consists of a putative presequence, prosequence, and catalytic domain. Like bacterial subtilisins, T. kodakaraensis subtilisin was overproduced in Escherichia coli in a form with a putative prosequence in inclusion bodies, solubilized in the presence of 8 M urea, and refolded and converted to an active molecule. However, unlike bacterial subtilisins, in which the prosequence was removed from the catalytic domain by autoprocessing upon refolding, T, kodakaraensis subtilisin was refolded in a form with a putative prosequence. This refolded protein of recombinant T. kodakaraensis subtilisin which is composed of 398 amino acid residues (Gly(-82) to Gly(316)), was purified to give a single band on a sodium dodecyl sulfate (SDS)-polyacrylamide gel and characterized for biochemical and enzymatic properties. The good agreement of the molecular weights estimated by SDS-polyacrylamide gel electrophoresis (44,000) and gel filtration (40,000) suggests that T. kodakaraensis subtilisin exists in a monomeric form. T. kodakaraensis subtilisin hydrolyzed the synthetic substrate N-succinyl-Ala-Ala-Pro-Phe-p-nitroanilide only in the presence of the Ca2+ ion with an optimal pH and temperature of pH 9.5 and 80 degreesC, Like bacterial subtilisins, it showed a broad substrate specificity, with a preference for aromatic or large nonpolar P1 substrate residues. However, it was much more stable than bacterial subtilisins against heat inactivation and lost activity with half-lives of > 60 min at 80 degreesC, 20 min at 90 degreesC, and 7 min at 100 degreesC.
  • T Matsuda, R Fujikawa, M Haruki, XF Tang, S Ezaki, T Imanaka, M Morikawa, S Kanaya
    EXTREMOPHILES 5 3 177 - 182 2001年06月 [査読有り][通常論文]
     
    Interactions of TBP-interacting protein (TIP26), TBP, and TFB from a hyperthermophilic archaeon Thermococcus kodakaraensis KOD1 with TATA-DNA were examined by electrophoretic mobility shift assay. Tk-TFB formed a ternary complex with Tk-TBP and TATA-DNA. Tk-TIP26 did not inhibit the formation of this ternary complex, but interacted with it to form a TIP26/TFB/TBP/DNA quaternary complex. This interaction is rather weak, and a large excess of Tk-TIP26 over Tk-TBP is required to fully convert the TFB/TBP/DNA ternary complex to the quaternary complex. However, determination of the concentration of Tk-TIP26 and Tk-TBP in KOD1 cells by Western blotting analysis indicated that the concentration of Tk-TIP26 is approximately ten times that of Tk-TBP, suggesting that the quaternary complex might also form in vivo.
  • Y Koga, M Haruki, M Morikawa, S Kanaya
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 91 6 551 - 556 2001年06月 [査読有り][通常論文]
     
    Glycerol kinases from Thermococcus kodakaraensis KOD1 (Tk-GK) and Escherichia coli (Ec-GK) greatly differ in thermostability. The temperature (T-1/2) at which the enzymes lose half of their activity upon incubation for 20 min is 50-55 degreesC for Ec-GK and similar to 95 degreesC for Tk-GK. To examine whether the amino acid substitutions that make Tk-GK more stable than Ec-GK are localized in a limited region, the chimeras of two parental genes encoding Tk-GK and Ec-GK were constructed by DNA shuffling. E. coli cells were transformed with a plasmid library harboring these chimeras and screened for those that produce chimeric enzymes which are more stable than Ec-GK. Four chimeric enzymes were isolated and purified, and their biochemical properties characterized. Replacement of 83 or 93 residues in the C-terminus of Ec-GK with the corresponding ones of Tk-GK increased the T-1/2 value of Ec-GK by 25-30 degreesC. In contrast, replacement of 85 residues in the N-terminus of Ec-GK with the corresponding ones of Tk-GK reduced the T-1/2 value by 5-10 degreesC. In addition, replacement of 10 residues in the C-terminus of Tk-GK with the corresponding ones of Ec-GK reduced the T-1/2 value of Tk-GK by similar to 15 degreesC. Measurement of the far-UV CD spectra indicates that the three-dimensional structures of the chimeric enzymes, as well as those of the parent enzymes, are similar to one another. These results suggest that the amino acid substitutions responsible for the high stability of Tk-GK are largely localized in the C-terminal region.
  • H. J. Kwon, K. Amada, M. Haruki, M. Morikawa, S. Kanaya
    FEBS Letters 497 2-3 174  2001年05月25日 [査読有り][通常論文]
  • Y Tsunaka, M Haruki, M Morikawa, S Kanaya
    BIOCHIMICA ET BIOPHYSICA ACTA-PROTEIN STRUCTURE AND MOLECULAR ENZYMOLOGY 1547 1 135 - 142 2001年05月 [査読有り][通常論文]
     
    The biochemical properties of the mutant protein D10R/E48R of Escherichia coli RNase HI, in which Asp(10) and Glu(48) are both replaced by Arg, were characterized. This mutant protein has been reported to have metal-independent RNase H activity at acidic pH [Casareno et al. (1995) J. Am. Chem. Sec. 117, 11011-11012]. The far- and near-UV CD spectra of this mutant protein were similar to those of the wild-type protein, suggesting that the protein conformation is not markedly changed by these mutations. Nevertheless, we found that this mutant protein did not show any RNase H activity in vitro. Instead, it showed high-nucleic-acid-binding affinity. Protein footprinting analyses suggest that DNA/RNA hybrid binds to or around the presumed substrate-binding site of the protein. In addition, this mutant protein did not complement the temperature-sensitive growth phenotype of the rnhA mutant strain, E. coli MIC3001, even at pH 6.0, suggesting that it does not show RNase H activity in vivo as well. These results are consistent with a current model for the catalytic mechanism of the enzyme, in which Glu(48) is not responsible for Mg2+ binding but is involved in the catalytic function. (C) 2001 Elsevier Science B.V. All rights reserved.
  • A Muroya, D Tsuchiya, M Ishikawa, M Haruki, M Morikawa, S Kanaya, K Morikawa
    PROTEIN SCIENCE 10 4 707 - 714 2001年04月 [査読有り][通常論文]
     
    The catalytic center of an archaeal Type 2 RNase H has been identified by a combination of X-ray crystallographic and mutational analyses. The crystal structure of the Type 2 RNase H from Thermococcus kodakaraensis KOD1 has revealed that the N-terminal major domain adopts the RNase H fold, despite the poor sequence similarity to the Type 1 RNase H. Mutational analyses showed that the catalytic reaction requires four acidic residues, which are well conserved in the Type 1 RNase H and the members of the polynucleotidyl transferase family. Thus, the Type 1 and Type 2 RNases H seem to share a common catalytic mechanism, except for the requirement of histidine as a general base in the former enzyme. Combined with the results from deletion mutant analyses, the structure suggests that the C-terminal domain of the Type 2 RNase H is involved in the interaction with the DNA/RNA hybrid.
  • バイオレメディエーション
    森川 正章
    学研ハイベスト教科事典「生物と環境」 223  2001年 [査読有り][通常論文]
  • M Morikawa, T Imanaka
    HYPERTHERMOPHILIC ENZYMES, PT A 330 424 - 433 2001年 [査読有り][通常論文]
  • T Kato, M Haruki, T Imanaka, M Morikawa, S Kanaya
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 91 1 64 - 70 2001年01月 [査読有り][通常論文]
     
    Two extremely thermophilic alkane-degrading bacterial strains, B23 and H41, were respectively isolated from deep subterranean petroleum reservoirs in the Minami-aga (Niigata) and Yabase (Akita) oil fields. Both strains were able to grow at temperatures ranging from 50 to 80 degreesC, with optimal growth at 70 degreesC for B23 and 65 degreesC for H41. From 16S rRNA gene sequence analysis and physiological characterization, both strains were identified as Bacillus thermoleovorans (identities of 99.5% and 99.6% to strain DSM 5366, and 98.3% and 98.7% to the type strain LEH-1(TS), respectively). Strains B23 and H41 effectively (>60%) degraded n-alkanes longer than C12 and C15, respectively, at 70 degreesC, while strain LEH-1(TS) degraded undecane (C11) most effectively. When B23 and H41 were cultivated in the presence of heptadecane, heptadecanoate and pentadecanoate were specifically accumulated in the cells. These results strongly suggest that the two strains degraded n-alkanes by a terminal oxidation pathway, followed by a beta -oxidation pathway.
  • T Kato, A Miyanaga, M Haruki, T Imanaka, M Morikawa, S Kanaya
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 91 1 100 - 102 2001年01月 [査読有り][通常論文]
     
    The gene encoding an alcohol dehydrogenase (Bt-ADH) was cloned from a newly isolated thermophilic alkane-degrading Bacillus thermoleovorans, strain B23. The gene conferred 1-tetradecanol dehydrogenase activity on Escherichia coli cells. Bt-ADH is composed of 249 amino acid residues and the calculated molecular mass is 27,196 Da. A tyrosine residue in the active site and a glycine-rich sequence (GGXXGI/LG) constituting probable nicotinamide adenine dinucleotide (NAD(+)) or nicotinamide adenine dinucleotide phosphate (NADP(+)) binding site were completely conserved in the Bt-ADH sequence at positions 155 and 11, respectively. A phylogenetic analysis of Bt-ADH suggested that the enzyme belongs to the zinc-independent ADH Group II. Its highest similarity (48% identical) was to a hypothetical oxidoreductase from a hyperthermophile, Thermotoga maritima.
  • N Rashid, M Morikawa, S Kanaya, H Atomi, T Imanaka
    HYPERTHERMOPHILIC ENZYMES, PT C 334 261 - 270 2001年 [査読有り][通常論文]
  • M Haruki, T Nogawa, N Hirano, H Chon, Y Tsunaka, M Morikawa, S Kanaya
    PROTEIN ENGINEERING 13 12 881 - 886 2000年12月 [査読有り][通常論文]
     
    To construct a DNA-linked RNase H, which cleaves RNA site-specifically at high temperatures, the 15-mer DNA, which is complementary to the polypurine-tract sequence of human immunodeficiency virus-1 RNA (PPT-RNA), was cross-linked to the unique thiol group of Cys135 in the Thermus thermophilus RNase HI variant. The resultant DNA-linked enzyme (d15-C135/TRNH), as well as the d15-C135/ERNH, in which the RNase H portion of the d15C135/TRNH is replaced by the Escherichia coli RNase HI variant, cleaved the 15-mer PPT-RNA site-specifically. The mixture of the unmodified enzyme and the unlinked 15-mer DNA also cleaved the PPT-RNA but in a less strict manner, In addition, this mixture cleaved the PIT-RNA much less effectively than the DNA-linked enzyme. These results indicate that the cross-linking limits but accelerates the interaction between the enzyme and the DNA/RNA substrate. The d15-C135/TRNH cleaved the PPT-RNA more effectively than the d15-C135/ERNH at temperatures higher than 50 degreesC, The d15-C135/TRNH showed the highest activity at 65 degreesC, at which the d15-C135/ERNH showed little activity. Such a thermostable DNA-linked RNase H may be useful to cleave RNA molecules with highly ordered structures in a sequence-specific manner.
  • M Haruki, Y Tsunaka, M Morikawa, S Iwai, S Kanaya
    BIOCHEMISTRY 39 45 13939 - 13944 2000年11月 [査読有り][通常論文]
     
    To investigate the role of the phosphate group 3' to the scissile phosphodiester bond of the substrate in the catalytic mechanism of Escherichia coli ribonuclease HI (RNase HI), we have used modified RNA-DNA hybrid substrates carrying a phosphorothioate substitution at this position or lacking this phosphate group for the cleavage reaction. Kinetic parameters of the H(124)A mutant enzyme, in which His(124) was substituted with Ala, as well as those of the wild-type RNase HI, were determined. Substitution of the pro-R-p-oxygen of the phosphate group 3' to the scissile phosphodiester bond of the substrate with sulfur reduced the k(cat) value of the wild-type RNase HI by 6.9-fold and that of the H(124)A mutant enzyme by only 1.9-fold. In contrast, substitution of the pro-Sb-oxygen of the phosphate group at this position with sulfur had little effect on the k(cat) value of the wild-type and H(124)A mutant enzymes. The results obtained for the substrate lacking this phosphate group were consistent with those obtained for the substrates with the phosphorothioate substitutions. In addition, a severalfold increase in the K-m value was observed by the substitution of the pro-R-p-oxygen of the substrate with sulfur or by the substitution of His(124) of the enzyme with Ala, suggesting that a hydrogen bond is formed between the pro-R-p-oxygen and His(124) These results allow us to propose that the pro-R-p-oxygen contributes to orient His(124) to the best position for the catalytic function through the formation of a hydrogen bond.
  • M Morikawa, Y Hirata, T Imanaka
    BIOCHIMICA ET BIOPHYSICA ACTA-MOLECULAR AND CELL BIOLOGY OF LIPIDS 1488 3 211 - 218 2000年11月 [査読有り][通常論文]
     
    Arthrofactin (AF) and surfactin (SF) are the most effective cyclic lipopeptide biosurfactants ever reported. Linear AF and linear SF were prepared by saponification of lactone ring. The oil displacement activities decreased to one third of their respective original values. When residues of both an aspartic acid and a glutamic acid of SF were methylated or amidated, the activity increased by 20%, although their water solubility was lost. When these amino acid residues were modified by aminomethane sulfonic acid, the activity was drastically decreased probably owing to charge repulsion and structural distortion inhibiting micelle formation. Both AF and SF expressed higher activity under alkaline conditions than acidic conditions. AF was more resistant to acidic conditions than SF and it kept high activity even under pH 0.5. Although SF drastically reduced its activity under acidic conditions, surfactin-Asp/Glu-amido ester and snrfactin-Asp/Glu-methyl ester retained similar activities irrespective of the pH change. A couple of conformers of SF prepared by reverse-phase HPLC showed the same oil displacement activity but different surface tension-reducing activity. AF was produced as a series of different fatty acid chain lengths (from C8 to C12). Among them, AF with fatty acid chain length of C10, which was the main product of the strain, showed the highest activity. (C) 2000 Elsevier Science B.V. All rights reserved.
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  • N Hirano, M Haruki, M Morikawa, S Kanaya
    BIOCHEMISTRY 39 43 13285 - 13294 2000年10月 [査読有り][通常論文]
     
    A genetic method for isolating a mutant enzyme of ribonuclease HI (RNase HI) from Thermus thermophilus HB8 with enhanced activity at moderate temperatures was developed. T. thermophilus RNase HI has an ability to complement the RNase H-dependent temperature-sensitive (ts) growth phenotype of Escherichia coli MIC3001. However, this complementation ability was greatly reduced by replacing Asp(134) which is one of the active site residues, with His, probably due to a reduction in the catalytic activity. Random mutagenesis of the gene encoding the resultant D134H enzyme, followed by screening for second-site revertants, allowed us to isolate three single mutations (Ala(12) --> Ser, Lys(75) --> Met, and Ala(77) --> Pro) that restore the normal complementation ability to the D134H enzyme. These mutations were individually or simultaneously introduced into the wild-type enzyme, and the kinetic parameters of the resultant mutant enzymes for the hydrolysis of a DNA-RNA-DNA/DNA substrate were determined at 30 degreesC. Each mutation increased the k(cat)/K-m value of the wild-type enzyme by 2.1-4.8-fold. The effects of the mutations on the enzymatic activity were roughly cumulative, and the combination of these three mutations increased the k(cat)/K-m value of the wild-type enzyme by 40-fold (5.5-fold in k(cat)). Measurement of thermal stability of the mutant enzymes with circular dichroism spectroscopy in the presence of 1 M guanidine hydrochloride and 1 mM dithiothreitol showed that the T-m value of the triple mutant enzyme, in which all three mutations were combined, was comparable to that of the wild-type enzyme (75.0 vs 77.4 degreesC). These results demonstrate that the activity of a thermophilic enzyme can be improved without a cost of protein stability.
  • K Hyun-Ju, K Amada, M Haruki, M Morikawa, S Kanaya
    FEBS LETTERS 483 2-3 139 - 142 2000年10月 [査読有り][通常論文]
     
    A lipase from Pseudomonas sp, MIS38 (PML) is a member of the lipase family 1.3. We analyzed the roles of the five histidine residues (His(30), His(274), His(291), His(313), and His(365)) and five acidic amino acid residues (Glu(253), Asp(255), ASp(262), Asp(275), and Asp(290)), which are fully conserved in the amino acid sequences of family 1.3 lipases, by site-directed mutagenesis, We showed that the mutation of His(313) or Asp(255) to Ala almost fully inactivated the enzyme, whereas the mutations of other residues to Ala did not seriously affect the enzymatic activity. Measurement of the far- and near-UV circular dichroism spectra suggests that inactivation by the mutation of His(313) Or Asp(255) is not due to marked changes in the tertiary structure, We propose that His(313) and Asp(255), together with Ser(207), form a catalytic triad in PML. (C) 2000 Federation of European Biochemical Societies. Published by Elsevier Science B.V. All rights reserved.
  • K Amada, M Haruki, T Imanaka, M Morikawa, S Kanaya
    BIOCHIMICA ET BIOPHYSICA ACTA-PROTEIN STRUCTURE AND MOLECULAR ENZYMOLOGY 1478 2 201 - 210 2000年05月 [査読有り][通常論文]
     
    Determination of the nucleotide sequence of the gene encoding a lipase from Pseudomonas sp. MIS38 (PML) revealed that PML is a member of the lipase family I.3 and is composed of 617 amino acid residues with a calculated molecular weight of 64 510. Recombinant PML (rPML) was overproduced in Escherichia coli in an insoluble form, solubilized in the presence of 8 M urea, purified in a urea-denatured form and refolded by removing urea in the presence of the Ca2+ ion. Gel filtration chromatography suggests that this refolded protein is monomeric. rPML showed relatively broad substrate specificities and hydrolyzed glyceryl tributyrate and olive oil with comparable efficiencies. rPML was active only in the form of a holoenzyme, in which at least 12 Ca2+ ions bound. These Ca2+ ions bound too tightly to be removed from the protein upon dialysis, but were removed from it upon EDTA treatment. The resultant ape-enzyme was fully active in the presence of 10 mM CaCl2, but was inactive in the absence of the Ca2+ ion. PML has a GXSXG motif, which is conserved in lipases/esterases and generally contains the active-site serine. The mutation of Ser(207) within this motif to Ala completely inactivated PML, suggesting that Ser(207) is the active-site serine of PML. (C) 2000 Elsevier Science B.V. All rights reserved.
  • N Ohtani, M Haruki, A Muroya, M Morikawa, S Kanaya
    JOURNAL OF BIOCHEMISTRY 127 5 895 - 899 2000年05月 [査読有り][通常論文]
     
    Escherichia coli RNase HII is composed of 198 amino acid residues. The enzyme has been overproduced in an insoluble form, purified in a urea-denatured form, and refolded with poor yield [M. Itaya (1990) Proc. Natl. Acad. Sci. USA 87, 8587-8591]. To facilitate the preparation of the enzyme in an amount sufficient for physicochemical studies, we constructed an overproducing strain in which E. coli RNase HII is produced in a soluble form. The enzyme was purified from this strain and its biochemical and physicochemical properties were characterized. The good agreement in the molecular weights estimated from SDS-PAGE (23,000) and gel filtration (22,000) suggests that the enzyme acts as a monomer. From the far-UV circular dichroism spectrum, its helical content was calculated to be 23%. The enzyme showed Mn2+-dependent RNase H activity. Its specific activity determined using H-3-labeled M13 RNA/DNA hybrid as a substrate was comparable to but slightly higher than that of the refolded enzyme, indicating that the enzyme overproduced and purified in a soluble form is more suitable for structural and functional analyses than the refolded enzyme.
  • Thermophilic bacteria isolated from a subterranean petroleum reservoir.
    M. Morikawa, T. Kato, M. Haruki, T. Imanaka, S. Kanaya
    In Gratama Workshop 2000 conference report 202 - 203 2000年 [査読有り][通常論文]
  • Decarbonylase, an enzyme which transforms aldehyde to alkene.
    H. Takagi, M. Haruki, N. Murakami, T. Imanaka, M. Morikawa, S. Kanaya
    In Proceedings of Fifth International Symposium on Environmental Biotechnology 2000年 [査読有り][通常論文]
  • Aldehyde dehydrogenase and esterase from a petroleum-degrading bacterium HD-1.
    S. Kanaya, N. Okibe, S. Mizuguchi, M. Haruki, T. Imanaka, M. Morikawa
    In Proceedings of Fifth International Symposium on Environmental Biotechnology 2000年 [査読有り][通常論文]
  • An extremely thermophile which degrades petroleum under high termperature conditions.
    T. Kato, A. Miyanaga, M. Haruki, T. Imanaka, M. Morikawa, S. Kanaya
    In Proceedings of Fifth International Symposium on Environmental Biotechnology 2000年 [査読有り][通常論文]
  • Enzymes from a psychrophilic Shewanella sp. SIB1.
    M. Haruki, N. Ohtani, K. Miura, Y. Suzuki, T. Kato, M. Morikawa, S. Kanaya
    In Proceedings of Fifth International Symposium on Environmental Biotechnology 2000年 [査読有り][通常論文]
  • Petroleum Degradation by an extremely thermophilic bacteria.
    M. Morikawa, T. Kato, A. Miyanaga, M. Haruki, T. Imanaka, S. Kanaya
    In Proceedings of Fifth International Symposium on Environmental Biotechnology 2000年 [査読有り][通常論文]
  • 新規抗菌物質の探索
    森川正章, 金谷茂則, 藤本善久
    大阪大学先端科学技術共同研究センター年報 6 18 - 20 2000年 [査読有り][通常論文]
  • 微生物にもとめる火事場の...?
    森川 正章
    The News of Engineering. Osaka University. 9 2000年 [査読有り][通常論文]
  • Kazuaki Harata, Noriyuki Ishii, Naeem Rashid, Masaaki Morikawa, Tadayuki Imanaka
    Acta Crystallographica Section D: Biological Crystallography 56 5 648 - 649 2000年 [査読有り][通常論文]
     
    Pk-REC is a protein which binds to DNA and catalyzes the central step of recombination and repair. The protein was crystallized using the hanging-drop vapour-diffusion method with PEG as a precipitant. Two orthorhombic crystal forms I and II with the same space group P212121 were obtained at pH 8.0 using PEG 3000 and PEG 550 monomethylether, respectively. The unit-cell parameters were a = 151, b = 174, c = 241 Å for form I and a = 151, b = 176, c = 300 Å for form II, indicating that the asymmetric unit contains more than 20 molecules.
  • S Mizuguchi, K Amada, M Haruki, T Imanaka, M Morikawa, S Kanaya
    JOURNAL OF BIOCHEMISTRY 126 4 731 - 737 1999年10月 [査読有り][通常論文]
     
    The gene encoding an esterase (HDE) was cloned from an oil-degrading bacterium, strain HD-I. HDE is a member of the hormone-sensitive lipase family and composed of 317 amino acid residues with a molecular weight of 33,633, The HDE-encoding gene was expressed in Escherichia coli, and the recombinant protein was purified and characterized. Amino acid sequence analysis indicated that the methionine residue was removed from its NH2-terminus, The good agreement of the molecular weights estimated by SDS-PAGE (35,000) and gel filtration (38,000) suggests that it acts in a monomeric form. HDE showed hydrolytic activity towards p-nitrophenyl esters of fatty acids with an acyl chain length of 2 to 14 and tributyrin, whereas it showed little hydrolytic activity towards p-nitrophenyl oleate (C-18), tricaprylin and triolein, Determination of the kinetic parameters for the hydrolyses of the p-nitrophenyl substrates from C-2 to C-14 indicated that HDE shows a relatively broad substrate specificity. However, comparison of the k(cat)/K-m values indicated that the C-10-C-14 substrates are the most preferred ones, Such a preference for substrates with long acyl chains may be a characteristic of HDE.
  • T Matsuda, M Morikawa, M Haruki, H Higashibata, T Imanaka, S Kanaya
    FEBS LETTERS 457 1 38 - 42 1999年08月 [査読有り][通常論文]
     
    We have isolated TBP (TATA-binding protein)interacting protein (TIP) from cell lysates of a hyperthermophilic archaeon, Pyrococcus kodakaraensis KOD1, by affinity chromatography with TBP-agarose. Based on the internal amino acid sequence information, PCR primers were synthesized and used to amplify the gene encoding this protein (Pk-TIP). Determination of the nucleotide sequence and characterization of the recombinant protein revealed that Pk-TIP is composed of 224 amino acid residues (molecular weight of 25558) and exists in a dimeric form. BIAcore analyses for the interaction between recombinant Pk-TIP and recombinant Pk-TBP indicated that they interact with each other with an equilibrium dissociation constant, K-D, of 1.24-1.46 mu M. A gel mobility shift assay indicated that Pk-TIP inhibited the interaction between Pk-TBP and a TATA-DNA. Pk-TIP may be one of the archaeal factors which negatively regulate transcription. (C) 1999 Federation of European Biochemical Societies.
  • N Ohtani, M Haruki, M Morikawa, S Kanaya
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 88 1 12 - 19 1999年07月 [査読有り][通常論文]
     
    RNase H is an enzyme that specifically cleaves RNA hybridized to DNA. The enzyme is ubiquitously present in various organisms. Single bacterial and eucaryotic tells often contain two RNases H, whereas single archaeal cells contain only one. To determine whether there is a physiologicaI significance in the ubiquity and multiplicity of the enzyme, and whether all enzymes are evolutionarily diverged from a common ancestor, we carried out phylogenetic analyses of the RNase H sequences. In this report, we demonstrated that RNases H are classified into two major families, Type 1 and Type 2 RNases H, of which only the Type 2 enzymes are present in all Living organisms, including bacteria, archaea, and eucaryotes, suggesting that they represent an ancestral form of RNases H. Based on this information, we discuss the evolutionary relationships and possible cellular functions of RNases H.
  • NQ Huy, S Jin, K Amada, M Haruki, NB Huu, DT Hang, DTC Ha, T Imanaka, M Morikawa, S Kanaya
    JOURNAL OF BIOSCIENCE AND BIOENGINEERING 88 1 100 - 102 1999年07月 [査読有り][通常論文]
     
    Four petroleum-degrading bacterial strains, 2TN-NB, 6TBX-CL, MVK2-5, and XCK, were isolated from various oil-contaminated sites in Vietnam. Determination of the nucleotide sequence of the gene encoding 16S rRNA allowed 2TN-NB to be identified as Acinetobacter sp, and the other three stains as Pseudomonas sp. Among the four isolates, 2TN-NB was most effective in degrading crude oil: in 1 d, it degraded 95% of the crude oil in the culture medium (5%, v/v). The isolated strains could also degrade a sulfur-containing aromatic hydrocarbon, dibenzothiophene (DBT), with low efficiency. Except for MVK2-5, which degraded crude oil least efficiently, the isolates produced biosurfactants in amounts sufficient for structural analysis. FT-IR measurement suggested that strains 6TBX-CL and XCK produced glycolipid-type biosurfactants while that produced by 2TN-NB was of the polysaccharide type.
  • M Haruki, Y Oohashi, S Mizuguchi, Y Matsuo, M Morikawa, S Kanaya
    FEBS LETTERS 454 3 262 - 266 1999年07月 [査読有り][通常論文]
     
    Escherichia coli esterase (EcE) is a member of the hormone-sensitive lipase family. We have analyzed the roles of the conserved residues in this enzyme (His(103), Glu(128), Gly(163), Asp(164), Ser(165), Gly(167), Asp(262), Asp(266) and His(292)) by site-directed mutagenesis. Among them, Gly(163), Asp(164), Ser(165), and Gly(167) are the components of a G-D/E-S-A-G motif. We showed that Ser(165), Asp(262), and His(292) are the active-site residues of the enzyme. We also showed that none of the other residues, except for Asp(164), is critical for the enzymatic activity. The mutation of Asp(164) to Ala dramatically reduced the catalytic efficiency of the enzyme by the factor of 10(4) without seriously affecting the substrate binding. This residue is probably structurally important to make the conformation of the active-site functional. (C) 1999 Federation of European Biochemical Societies.
  • N Rashid, M Morikawa, S Kanaya, H Atomi, T Imanaka
    FEBS LETTERS 445 1 111 - 114 1999年02月 [査読有り][通常論文]
     
    A RecA/Rad51 homologue from Pyrococcus koda-karaensis KOD1 (Pk-REC) is the smallest protein among various RecA/Rad51 homologues, Nevertheless, Pk-Rec is a super multifunctional protein and shows a deoxyribonuclease activity. This deoxyribonuclease activity was inhibited by 3 mM or more ATP, suggesting that the catalytic centers of the ATPase and deoxyribonuclease activities are overlapped. To examine whether these two enzymatic activities share the same active site, a number of site-directed mutations were introduced into Pk-REC and the ATPase and deoxyribonuclease activities of the mutant proteins were determined. The mutant enzyme in which double mutations Lys-33 to Ala and Thr-34 to Ala were introduced, fully lost both of these activities, indicating that Lys-33 and/or Thr-34 are important for both ATPase and deoxyribonuclease activities. The mutation of Asp-112 to Ale slightly and almost equally reduced both ATPase and deoxyribonuclease activities. In addition, the mutation of Glu-54 to Gib did not seriously affect the ATPase, deoxyribonuclease, and UV tolerant activities. These results strongly suggest that the active sites of the ATPase and deoxyribonuclease activities of Pk-REC are common, It is noted that unlike Glu-96 in Escherichia coli RecA, which has been proposed to be a catalytic residue for the ATPase activity, the corresponding residual Glu-54 in Pk-REC is not involved in the catalytic function of the protein. (C) 1999 Federation of European Biochemical Societies.
  • 環境問題を大学で学ぶ
    森川 正章
    栄冠をめざしてSPECIAL.河合塾/全国進学情報センター 特別 1999年 [査読有り][通常論文]
  • 森川 正章
    生産技術 51 1 153 - 157 生産技術振興協会 1999年 [査読有り][通常論文]
  • N Ohtani, M Haruki, M Morikawa, RJ Crouch, M Itaya, S Kanaya
    BIOCHEMISTRY 38 2 605 - 618 1999年01月 [査読有り][通常論文]
     
    Database searches indicated that the genome of Bacillus subtilis contains three different genes encoding RNase H homologues. The ypdQ gene encodes an RNase HI homologue with 132 amino acid residues, whereas the rnh and ysgB genes encode RNase HII homologues with 255 and 313 amino acid residues, respectively. RNases HI and HII show no significant sequence similarity. These genes were individually expressed in Escherichia coli; the recombinant proteins were purified, and their enzymatic properties were compared with those of E. coli RNases HI and HII. We found that the ypdQ gene product showed no RNase H activity. The 2.2 kb pair genomic DNA containing this gene did not suppress the RNase H deficiency of an E, coli rnhA mutant, indicating that this gene product shows no RNase H activity in vivo as well. In contrast, the rnh (rnhB) gene product (RNase HII) showed a preference for Mn2+, as did E. coli RNase HII, whereas the ysgB (mhC) gene product (RNase HIII) exhibited a Mg2+-dependent RNase H activity. Oligomeric substrates digested with these enzymes indicate similar recognition of these substrates by B. subtilis and E. coli RNases HII. Likewise, B. subtilis RNase HIII and E. coli RNase HI have generated similar products. These results suggest that B. subtilis RNases HII and HIII may be functionally similar to E, coli RNases HII and HI, respectively. We propose that Mn2+-dependent RNase HII is universally present in various organisms and Mg2+-dependent RNase HIII, which may have evolved from RNase HII, functions as a substitute for RNase HI.
  • Naoko Okibe, Kei Amada, Shin Ichi Hirano, Mitsuru Haruki, Tadayuki Imanaka, Masaaki Morikawa, Shigenori Kanaya
    Journal of Bioscience and Bioengineering 88 1 7 - 11 1999年 [査読有り][通常論文]
     
    The hd-ald gene encoding aldehyde dehydrogenase (hd-ALDH) from an mixotrophic petroleum-degrading bacterium, strain HD-1 was cloned and sequenced, hd-ALDH (506 amino acids) is a member of the NAD+-dependent aldehyde dehydrogenase group. The hd-ald gene was expressed in Escherichia coli, and the recombinant enzyme was purified and characterized biochemically and enzymatically. The molecular weight of the enzyme was estimated to be 55,000 by SDS-PAGE, and 224,000 by gel filtration chromatography, suggesting that it acts as a tetramer. The CD spectrum suggests that the helical content of the enzyme is 10%. hd-ALDH was active on various aliphatic aldehyde substrates. The K(m) values of the enzyme were 6.4 μM for acetaldehyde, 4.2 μM for hexanal, 2.8 μM for octanal, and 0.84 μM for decanal, whereas the k(cat) values for these substrates were nearly equal (51-64 min-1). These results indicate that hd-ALDH acts preferentially on long-chain aliphatic aldehydes.
  • Y Koga, M Morikawa, M Haruki, H Nakamura, T Imanaka, S Kanaya
    PROTEIN ENGINEERING 11 12 1219 - 1227 1998年12月 [査読有り][通常論文]
     
    The Pk-glpK gene, which encodes glycerol kinase (GK) from a hyperthermophilic archaeon Pyrococcus kodakaraensis KOD1, was cloned and expressed in Escherichia coli, The amino acid sequence of this enzyme (Pk-GK) deduced from the nucleotide sequence showed 57% identity with that of E.coli GK and 37% identity with that of human GK, Pk-GK, which has a molecular weight of 55 902 (497 amino acid residues), was purified from E.coli and characterized, Despite the high sequence similarity, Pk-GK and E.coli GK are greatly divergent in structure and function from each other. Unlike E.coli GK, which exists as a tetramer, Pk-GK exists as a dimer, The preferred divalent cation for Pk-GK is Co2+, instead of Mg2+. The optimum pH and temperature for Pk-GK activity are 8.0 and 80 degrees C, respectively, Pk-GK call utilize other nucleoside triphosphates than ATP as a phosphoryl donor, It is fairly resistant to an allosteric inhibitor of E.coli GK, fructose-1,6-bisphosphate. Determination of the kinetic parameters indicates that the K-m value of the enzyme is 15.4 mu M for ATP and 111 mu M for glycerol and its k(cat) value is 930 s(-1). The enzyme was shown to be fairly resistant to irreversible heat inactivation and still retained 50% of its enzymatic activity even after heating at 100 degrees C for 30 min. Construction of a model for the three-dimensional structure of the enzyme suggests that the formation of extensive ion-pair networks is responsible for the high stability of this enzyme.
  • M Haruki, K Hayashi, T Kochi, A Muroya, Y Koga, M Morikawa, T Imanaka, S Kanaya
    JOURNAL OF BACTERIOLOGY 180 23 6207 - 6214 1998年12月 [査読有り][通常論文]
     
    We have cloned the gene encoding RNase HII (RNase HIIPk) from the hyperthermophilic archaeon Pyrococcus kodakaraensis KOD1 by screening of a library for clones that suppressed the temperature-sensitive growth phenotype of an mh mutant strain of Escherichia coli. This gene was expressed in an mh mutant strain off. call, the recombinant enzyme was purified, and its biochemical properties were compared with those of E. coli RNases HI and HII, RNase HIIPk is composed of 228 amino acid residues (molecular weight, 25,799) and acts as a monomer, Its amino acid sequence showed little similarity to those of enzymes that are members of the RNase HI family of proteins but showed 40, 31, and 25% identities to those of Methanococcus jannaschii, Saccharomyces cerevisiae, and E. coli RNase HII proteins, respectively. The enzymatic activity,vas determined at 30 degrees C and pH 8.0 by use of an M13 DNA-RNA hybrid as a substrate. Under these conditions, the most preferred metal ions were Co2+ for RNase HIIPk, Mn2+ for E. coli RNase HII, and Mg2+ for E. coli RNase HI. The specific activity of RNase HIIPk determined in the presence of the most preferred metal ion was 6.8-fold higher than that off. coli RNase HII and 4.5-fold lower than that off. coli RNase HI, Like E. coli RNase HI, RNase HIIPk and E. call RNase HII cleave the RNA strand of an RNA-DNA hybrid endonucleolytically at the P-O3' bond. In addition, these enzymes cleave oligomeric substrates in a similar manner. These results suggest that RNase HIIPk and E. coli RNases HI and HII are structurally and functionally related to one another.
  • Cloning of a ribonuclease HII gene from a hyperthermophilic archaeon: Purification and characterization of a recombinant enzyme.
    Haruki, M, Hayashi, K, Kouchi, T, Muroya, A, Koga, Y, Morikawa, M, Imanaka, T, Kanaya, S
    J. Bacteriol. 1998年12月 [査読有り][通常論文]
  • N Hirano, M Haruki, M Morikawa, S Kanaya
    BIOCHEMISTRY 37 36 12640 - 12648 1998年09月 [査読有り][通常論文]
     
    TO identify factors that contribute to the thermal stability of ribonuclease HI (RNase HI) from Thermus thermophilus HB8, protein variants with a series of carboxyl-terminal truncations and Cys Ala mutations were constructed, and their thermal denaturations were analyzed by CD. The results indicate that Cys(41) and Cys(149) contribute to the protein stability, probably through the formation of a disulfide bond. Peptide mapping analysis for the mutant protein with only two cysteine residues, at positions 41 and 149, indicated that this disulfide bond is partially formed in a protein purified from Escherichia coli in the absence of a reducing reagent but is fully formed in a thermally denatured protein. These results suggest that the thermal stability of T. thermophilus RNase HI, determined in the absence of a reducing reagent, reflects that of an oxidized form of the protein. Comparison of the thermal stabilities and the enzymatic activities of the wild-type and truncated proteins, determined in the presence and absence of a reducing reagent, indicates that the formation of this disulfide bond increases the thermal stability of the protein by 6-7 degrees C in T-m and similar to 3 kcal/mol in Delta G without seriously affecting the enzymatic activity. Since T. thermophilus RNase HT is present in a reducing environment in cells, this disulfide bond probably is not formed in vivo but is spontaneously formed in vitro in the absence of a reducing reagent.
  • M Morikawa, T Iwasa, K Nagahisa, S Yanagida, T Imanaka
    ADVANCES IN CHEMICAL CONVERSIONS FOR MITIGATING CARBON DIOXIDE 114 467 - 470 1998年 [査読有り][通常論文]
  • 森川正章, 金 沙, 金谷茂則, 今中忠行
    農芸化学会誌 72 4 532 - 534 1998年 [査読有り][通常論文]
  • 大学推進型新プロジェクトが創る夢
    森川 正章
    大阪大学工業会誌テクノネット 501 9  1998年 [査読有り][通常論文]
  • M Morikawa, T Iwasa, S Yanagida, T Imanaka
    JOURNAL OF FERMENTATION AND BIOENGINEERING 85 2 243 - 245 1998年 [査読有り][通常論文]
     
    A petroleum-degrading bacterium, strain HD-1, was grown anaerobically with CO2 and H-2 as Sole carbon and energy sources, respectively. Electron microscopic observation revealed that many granules were accumulated inside the cell. GC/MS analysis of the cell components showed that the bacterium fixed CO2 and produced alkanes/alkenes with carbon numbers from 14 to 30 besides fatty acids and poly-beta-hydroxyalkanoic acids. By employing HD-1 cell extract, fatty acid and fatty aldehyde were found to be utilized as substrates in the alkane/alkene biosynthetic pathways.
  • N Rashid, M Morikawa, K Nagahisa, S Kanaya, T Imanaka
    NUCLEIC ACIDS RESEARCH 25 4 719 - 726 1997年02月 [査読有り][通常論文]
     
    The Pk-rec gene, encoding a RecA/RAD51 homologue from the hyperthermophilic archaeon Pyrococcus sp. KOD1, was expressed in Escherichia coli, The recombinant Pk-REC was purified to homogeneity and was shown to be in a dimeric form. A striking property of the purified recombinant Pk-REC was the unusual DNase activity on both single- and double-stranded DNAs along with the ATPase activity, The reaction product of this DNase activity was mononucleotides, The optimum temperature and pH for the DNase activity were 60 degrees C and 8-8.5, respectively. In addition, the metal ion requirement for DNase activity was different from that for the ATPase activity. The protein exhibited no DNase activity in the presence of Zn2+ ion, which was one of the most preferable divalent cations for ATPase activity. Another unique characteristic of the recombinant protein was that the reaction product of ATPase activity was AMP instead of ADP. Pk-REC may represent a common prototype of the RecA family proteins with high RecA-like activity.
  • A new type of petroleum-degrading/producing bacterium HD-1.
    M. Morikawa, T. Imanaka
    In Proceedings of International Workshop on Ultra-Long-Term Cryogenic 51 - 60 1997年 [査読有り][通常論文]
  • Gene cloning and characterization of recombinant ribonuclease HII from a hyperthermophilic archaeon.
    Haruki M, Hayashi K, Kochi T, Muroya A, Koga Y, Morikawa M, Imanaka T, Kanaya S
    Annual reports of ICBiotech. 20 803 - 821 1997年 [査読有り][通常論文]
  • 超好熱菌の新機能解析と耐熱酵素に関する研究
    高木昌宏, 金谷茂則, 森川正章, 春木 満, 藤原伸介, 橘 佳永
    大阪大学先端科学共同研究センター年報 2 35 - 38 1997年 [査読有り][通常論文]
  • N Rashid, M Morikawa, T Imanaka
    JOURNAL OF FERMENTATION AND BIOENGINEERING 83 5 412 - 418 1997年 [査読有り][通常論文]
     
    The gene encoding ribose phosphate pyrophosphokinase (Pk-RPPK) from a hyperthermophilic archaeon, Pyrococcus sp. KOD1 (Pk), was cloned, sequenced and expressed in Escherichia coli. The recombinant Pk-RPPK (280 aa, 31,113 Da) was purified to homogeneity. The optimal temperature and pH for the enzymatic activity are 50 degrees C and 7.0, respectively. The half-life of the enzymatic activity is 55 min at 70 degrees C. A unique characteristic of the enzyme is that it can utilize CTP and GTP as substrates In addition to ATP. It was also found that Co2+ in particular and Ni2+ markedly enhance the specific activity of the enzyme, as does Mg2+ in the presence of Co2+ (182 units/mg protein).
  • T Imanaka, M Morikawa
    GLOBAL ENVIRONMENTAL BIOTECHNOLOGY 401 - 414 1997年 [査読有り][通常論文]
  • M Morikawa, T Imanaka
    GLOBAL ENVIRONMENTAL BIOTECHNOLOGY 585 - 596 1997年 [査読有り][通常論文]
  • N Rashid, M Morikawa, T Imanaka
    MOLECULAR & GENERAL GENETICS 253 3 397 - 400 1996年12月 [査読有り][通常論文]
     
    A gene encoding a RecA/RAD51 homologue from a hyperthermophilic archaeon, Pyrococcus sp. KOD1 (Pk), was cloned, sequenced and expressed in Escherichia coli. The deduced 210-amino acid sequence was compared to homologues from bacteria (RecA), eukaryotes (RAD51, DMC1) and archaea (RadA). The entire protein from Pk (Pk-REC) basically corresponds to the essential central domain of its counterparts and lacks the two smaller RecA subdomains at the N- and C-termini. The sequence comparison suggests that Pk-REC represents a common prototype of RecA, RAD51, DMC1 and RadA, with higher enzymatic activity. Recombinant Pk-REC was fully active and complemented the ultraviolet light sensitivity of an E. coli recA mutant strain.
  • T Imanaka, M Morikawa
    MOLECULAR BIOLOGY OF PSEUDOMONADS 289 - 297 1996年 [査読有り][通常論文]
  • RecA/RAD51 homologue from a hyperthermophilic archaeon maintains the major domain only.
    Rashid N, Morikawa M, Imanaka T
    Annual reports of ICBiotech. 19 713 - 718 1996年 [査読有り][通常論文]
  • 森川正章, 今中忠行
    生産技術 48 4 59 - 62 生産技術振興協会 1996年 [査読有り][通常論文]
  • M Morikawa, M Kanemoto, T Imanaka
    JOURNAL OF FERMENTATION AND BIOENGINEERING 82 3 309 - 311 1996年 [査読有り][通常論文]
     
    A petroleum assimilating facultative anaerobic bacterium (strain HD-1) was isolated from an oil field in Shizuoka. The cells were anaerobically grown on CO2 as the sole carbon source in the presence of H-2, and the growth was markedly enhanced by the addition of aromatic or aliphatic hydrocarbon [Morikawa, M, and Imanaka, T.: J. Ferment. Bioeng., 76, 280-283, 1993]. The strain degraded tetradecane (C14) under anaerobic conditions and one of the major metabolic intermediates was identified as 1-dodecene (C12). This result demonstrates that alkanes are biodegradable in the absence of molecular oxygen via a pathway different from that of beta-oxidation. The strain was found to grow on CO2 in the presence of tetradecane and absence of H-2 gas and Light. These findings strongly indicate that the bacterium is capable of anaerobically utilizing alkane as an energy source.
  • T Imanaka, M Morikawa
    ENVIRONMENTAL BIOTECHNOLOGY 16 - 27 1996年 [査読有り][通常論文]
     
    We isolated a new type of Gram-negative mixotrophic bacterium, Pseudomonas sp. HD-1, which is a facultative anaerobe. Cells were grown on CO2 as a sole carbon source in the presence of H-2. Anaerobic growth of the strain was enhanced by the addition of aliphatic as well as aromatic hydrocarbons. When cells were grown on n-alkane anaerobically, many oil vacuoles formed in the cells and about 40-50% of the dry cell weight was lipid and oil. The total increase in the hydrophilic components of the cells indicated the anaerobic assimilation of,aliphatic hydrocarbon. Electron microscopic observation showed that the cell surface was highly wavy and that the membrane had a multi-layer structure irrespective of the presence of oil. The strain can fix CO2 and produce n-alkane (C-10 to C-20) in the absence of oil. The strain has the following potentials from the viewpoint of bioremediation. 1) Dissolved the oil pollution problem by anaerobic degradation of hydrocarbons, 2) Dissolve the greenhouse effect by CO2 fixation, and 3) Microbial production of oil.
  • N RASHID, M MORIKAWA, T IMANAKA
    GENE 166 1 139 - 143 1995年12月 [査読有り][通常論文]
     
    The gene encoding the TATA-binding protein (PkTBP) from a hyperthermophilic archaeon, Pyrococcus sp, KOD1 (Pk), was cloned and sequenced. An open reading frame with homology to the conserved C-terminal core region of eukaryotic TBP was expressed in Escherichia coli. Specific DNA-binding activity of the recombinant PkTBP (190 amino acids, 21.36 kDa) was also demonstrated, Although it was composed of a structurally direct repeat sequence which is similar to eukaryotic TBP, the total net charge of archaeal TBP was amazingly negative (calculated isoelectric point (pI) was 4.66 and experimentally estimated pi was 4.8). A series of five Glu residues was found at the C terminus of archaeal TBP. These data strongly suggest that a positively charged protein is also involved in the transcription initiation event which might stabilize the structure of the genomic DNA under high-growth-temperature conditions.
  • バイオサーファクタント実用化の試み
    今中忠行, 平田善彦, 森川正章
    Rep. Chem. Mat. R & D Found. 10 103 - 106 1995年 [査読有り][通常論文]
  • 森川正章, 今中忠行
    高圧ガス 32 4 336 - 339 高圧ガス保安協会 1995年 [査読有り][通常論文]
  • 今中忠行, 森川正章
    燃料及燃焼 62 5 323 - 330 燃料及燃焼社 1995年 [査読有り][通常論文]
  • 森川正章
    日本農芸化学会誌 69 6 756 - 757 1995年 [査読有り][通常論文]
  • 森川正章, 今中忠行
    蛋白質 核酸 酵素 40 1 52 - 60 共立出版 1995年 [査読有り][通常論文]
  • DJ KIM, M MORIKAWA, M TAKAGI, T IMANAKA
    JOURNAL OF FERMENTATION AND BIOENGINEERING 79 2 87 - 94 1995年 [査読有り][通常論文]
     
    The peptidyl prolyl cis-trans isomerase (PPIase, EC 5.2.1.8) gene (ppiT) from Bacillus stearothermophilus SIC1 was cloned on the basis of a partial amino acid sequence of the purified enzyme. ppiT was found as an open reading frame (501 bases) which coded for a protein consisting of 167 amino acid residues (molecular weight, 18,349) (GenBank accession number D42050). The cloned ppiT was overexpressed in Eschelichia coil cells using pET-8c as an expression vector. The enzyme was purified by heat treatment and column chromatography on DEAE-Sepharose CL-6B. Purification was about 148-fold and the molecular weight of the enzyme was estimated to be about 18.0 kDa by SDS-PAGE. PPIase activity was determined using synthetic peptide as a substrate in a 2-step reaction coupled with chymotrypsin treatment. The enzyme was stable at pH 7.5-8.0. No heat denaturation was observed when the enzyme was treated at 60 degrees C for 30 min. The PPIase purified from recombinant E. coil has almost the same characteristics as that from B. stearothemophilus SIC1. In refolding solution, the PPIase enhanced the Isomerization rate of unfolded RNase T1.
  • M MORIKAWA, Y IZAWA, N RASHID, T HOAKI, T IMANAKA
    APPLIED AND ENVIRONMENTAL MICROBIOLOGY 60 12 4559 - 4566 1994年12月 [査読有り][通常論文]
     
    A hyperthermophilic archaeon strain, KOD1, was isolated from a solfatara at a wharf on Kodakara Island, Kagoshima, Japan. The growth temperature of the strain ranged from 65 to 100 degrees C, and the optimal temperature was 95 degrees C. The anaerobic strain was an S-0-dependent heterotroph. Cells were irregular cocci and were highly motile with several polar flagella. The membrane lipid was of the ether type, and the GC content of the DNA was estimated to be 38 mol%. The 16S rRNA sequence was 95% homologous to that of Pyrococcus abyssi. The optimum growth pH and NaCl concentration of the strain KOD1 were 7.0 and 3%, respectively. Therefore, strain KOD1 was identified as a Pyrococcus sp. Strain KOD1 produced at least three extracellular proteases. One of the most thermostable proteases was purified 21-fold, and the molecular size was determined to be 44 kDa by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and 45 kDa by gel filtration chromatography. The specific activity of the purified protease was 2,160 U/mg of protein. The enzyme exhibited its maximum activity at approximately pH 7.0 and at a temperature of 110 degrees C, with azocasein as a substrate. The enzyme activity was completely retained after heat treatment at 90 degrees C for 2 h, and the half-life of enzymatic activity at 100 degrees C was 60 min. The proteolytic activity was significantly inhibited by p-chloromercuribenzoic acid or E-64 but not by EDTA or phenylmethylsulfonyl fluoride. Proteolytic activity was enhanced threefold in the presence of 8 mM cysteine. These experimental results indicated that the enzyme was a thermostable thiol protease.
  • M MORIKAWA, H DAIDO, S PONGPOBPIBOOL, T IMANAKA
    APPLIED MICROBIOLOGY AND BIOTECHNOLOGY 42 2-3 300 - 303 1994年11月 [査読有り][通常論文]
     
    Arthrobacter sp. strain MIS38 was transformed with a shuttle vector containing the kanamycin resistant gene kan (derived from Tn5) by an electroporation method. This shuttle vector is from Brevibacterium lactofermentum and Escherichia coli, pULRS8. The following optimal condition of electroporation was determined. A square wave pulse of 1 kV/cm electric field strength for 0.5 ms duration yielded 3 x 10(5) transformants/mu g plasmid DNA. The number of transformants increased with the amount of DNA over the range 0.01-5 mu g. This host-vector system was then used successfully to clone and express a lipase gene from Arthrobacter sp. strain MIS38 into both Arthrobacter sp. MIS38 and E. coli JM109.
  • Lee S-P, Morikawa M, Takagi M, Imanaka T
    Appl. Environ. Microbiol. 60 10 3764 - 3773 1994年10月 [査読有り][通常論文]
     
    A thermophilic and alkaliphilic Bacillus sp. strain, XAL601, was isolated from soil. It produces a thermostable and alkaline-stable enzyme with both alpha-amylase and pullulanase activities. The alpha-amylase-pullulanase gene (aapT) from this Bacillus strain was cloned, and its nucleotide sequence was determined (GenBank accession number D28467). A very large open reading frame composed of 6,096 bases, which encodes 2,032 amino acid residues with an M(r) of 224,992, was found. The deduced amino acid sequence revealed that the four highly conserved regions that are common among amylolytic enzymes were well conserved. These include an active center and common substrate-binding sites of various amylases. In the C-terminal region, a six-amino-acid sequence (Gly-Ser-Gly-Thr-Thr-Pro) is repeated 12 times. The aapT gene was then subcloned in Escherichia coli and overexpressed under the control of the lac promoter. Purification of AapT from this recombinant E. coli was performed, and it was shown that the aapT gene product exhibits both or-amylase and pullulanase activities with one active site. The optimum temperature and pH for enzyme activity were found to be 70 degrees C and pH 9, respectively. Furthermore, AapT was found to strongly adsorb to crystalline cellulose (Avicel) and raw corn starch. Final hydrolyzed products from soluble starch range from maltose (G2) to maltotetraose (G4). Only maltotriose (G3) was produced from pullulan. The enzyme also hgdrolyzes raw starch under a broad range of conditions (60 to 70 degrees C and pH 8 to 9).
  • Cloning and analysis of 16S-rRNA gene and transcription factor (TF) IID gene from a hyperthermophilic archaeon strain KOD1.
    Rashid N, Morikawa M, Imanaka T
    Annual reports of ICBiotech. 17 255 - 270 1994年 [査読有り][通常論文]
  • 超好熱始原菌 KOD1 株チオール型プロテアーゼ(TT プロテアーゼ) 遺伝子の検索
    森川 正章
    アマシャムライフサイエンスHighlight 12月 1994年 [査読有り][通常論文]
  • 今中忠行, 森川正章
    バイオサイエンスとインダストリー 52 11 898 - 900 バイオインダストリ-協会 1994年 [査読有り][通常論文]
  • CO2を単一炭素源として生育する石油代謝細菌
    森川正章, 今中忠行
    化学と生物 32 690 - 691 1994年 [査読有り][通常論文]
  • M MORIKAWA, H DAIDO, T TAKAO, S MURATA, Y SHIMONISHI, T IMANAKA
    JOURNAL OF BACTERIOLOGY 175 20 6459 - 6466 1993年10月 [査読有り][通常論文]
     
    A biosurfactant termed arthrofactin produced by Arthrobacter species strain MIS38 was purified and chemically characterized as 3-hydroxydecanoyl-D-leucyl-D-asparagyl-D-threonyl-D-leucyl-D-l eucyl-D-seryl-L-leucyl-D-Seryl-L-isoleucyl-L-isoleucyl-L-asparagyl lactone. Surface activity of arthrofactin was examined, with surfactin as a control. Critical micelle concentration values of arthrofactin and surfactin were around 1.0 x 10(-5) M and 7.0 x 10(-5) M at 25-degrees-C, respectively. Arthrofactin was found to be five to seven times more effective than surfactin. The minimum surface tension value of arthrofactin was 24 mN/m at a concentration higher than the critical micelle concentration. According to the oil displacement assay, arthrofactin was a better oil remover than synthetic surfactants, such as Triton X-100 and sodium dodecyl sulfate. Arthrofactin is one of the most effective lipopeptide biosurfactants.
  • 森川正章, 今中忠行
    バイオサイエンスとインダストリー 51 5 33 - 37 バイオインダストリ-協会 1993年 [査読有り][通常論文]
  • 石油を分解する細菌
    森川正章, 今中忠行
    化学 48 692 - 693 1993年 [査読有り][通常論文]
  • M MORIKAWA, T IMANAKA
    JOURNAL OF FERMENTATION AND BIOENGINEERING 76 4 280 - 283 1993年 [査読有り][通常論文]
     
    We isolated a new type of Gram-negative mixotrophic bacterium, Pseudomonas sp. HD-1, which is a facultative anaerobe. Cells were grown on CO2 as a sole carbon source in the presence of H-2. Anaerobic growth of the strain was enhanced by the addition of aliphatic as well as aromatic hydrocarbons. When cells were grown on n-alkane anaerobically, many oil vacuoles formed in the cells and about 40-50% of the dry cell weight was lipid and oil. The total increase in the hydrophilic components of the cells indicated the anaerobic assimilation of aliphatic hydrocarbon. Electron microscopic observation showed that the cell surface was highly wavy and that the membrane had a multi-layer structure irrespective of the presence of oil.
  • M MORIKAWA, M ITO, T IMANAKA
    JOURNAL OF FERMENTATION AND BIOENGINEERING 74 5 255 - 261 1992年 [査読有り][通常論文]
     
    Two bacteria (A-1 and B-1) which exhibited large emulsified halos around their colonies on oil-L-agar plates were isolated. These bacteria produced the same biosurfactant, surfactin. Strain A-1 (Psf+: surfactin producing) was identified as Bacillus pumilus and could be transformed with plasmid DNA using an electroporation method. Several surfactin non-producing (Psf-) mutants were obtained by chemical mutagenesis of B. pumilus A-1. By using them as host cells and pC194 as a vector plasmid, we cloned DNA fragments which complemented Psf- alleles. One of them (2 kb HindIII fragment) could transform Bacillus subtilis MI113 (a derivative of Marburg strain 168 and Psf-) to a Psf+ cell as well. Nucleotide sequence of the 2 kb fragment was determined and three large open reading frames (ORF1, 2, 3) were found. Deletion analysis of the recombinant plasmid indicated that ORF3 (699 bp, 233 amino acid residues) is essential for surfactin production. The gene was designated as psf-1 and a 25 kDa translation product was detected. The nucleotide sequence of psf-1 exhibited high homology with an unknown open reading frame, orfX, upstream to the gramicidin S biosynthesis operon of Bacillus brevis. It is suggested that the deduced gene products of unknown orfX in B. brevis and psf-1 in B. pumilus may share the same function.
  • 森川正章, 今中忠行
    バイオサイエンスとインダストリー 49 9 969 - 972 バイオインダストリ-協会 1991年 [査読有り][通常論文]
  • Cloning in Bacillus subtilis of thermostable and alkalophilic amylase from a thermophilic Bacillus sp.
    Ganrong X, Lee S-P, Takagi M, Morikawa M, Imanaka T
    Annual reports of ICBiotech. 13 121 - 128 1990年 [査読有り][通常論文]
  • M MURAKI, M MORIKAWA, Y JIGAMI, H TANAKA
    EUROPEAN JOURNAL OF BIOCHEMISTRY 179 3 573 - 579 1989年02月 [査読有り][通常論文]
  • M MURAKI, M MORIKAWA, Y JIGAMI, H TANAKA
    PROTEIN ENGINEERING 2 1 49 - 54 1988年04月 [査読有り][通常論文]
  • M MURAKI, M MORIKAWA, Y JIGAMI, H TANAKA
    BIOCHIMICA ET BIOPHYSICA ACTA 916 1 66 - 75 1987年11月 [査読有り][通常論文]
  • M MURAKI, Y JIGAMI, M MORIKAWA, H TANAKA
    BIOCHIMICA ET BIOPHYSICA ACTA 911 3 376 - 380 1987年02月 [査読有り][通常論文]

MISC

書籍等出版物

  • Masaaki Morikawa (担当:単著)
    2023年01月
  • Masaaki Morikawa (担当:単著)
    Springer 2023年01月
  • Shunitz Tanaka, Masaaki Kurasaki, Masaaki Morikwa, Yuichi Kamiya (担当:共編者(共編著者))
    Springer 2023年01月
  • バイオサーファクタント”、第10章低炭素社会への取組み、「応用微生物学 第3版」
    森川 正章 
    文永堂出版 2016年
  • Chap. 12. Comparison of the degradation activity of biofilm-associated versus planktonic cells pp219-232
    Morikawa M, Washio K 
    Caister Academic Press 2016年
  • Chap. 13A Using microbial biofilms to enhance the phytoremediation of contaminants in soil and water – A trial for sustainable phenol degradation by duckweed-colonizing biofilms pp 233-240
    Morikawa M, Yamaga F, Suzuki K, Kurashina K, Miwa K, Washio K 
    Caister Academic Press 2016年
  • 植物機能のポテンシャルを活かした環境保全・浄化技術
    森川正章 (担当:分担執筆範囲:第4章3節 PGPR (Plant Growth Promoting Rhizobacteria) の環境保全・修復への利用 pp 169-176)
    シーエムシー出版 2011年
  • 微生物増殖学の現在・未来
    森川 正章 (担当:分担執筆範囲:バイオフィルム―微生物の生存戦略を生かすpp 444-454)
    地人書館 2009年
  • バイオフィルムの基礎と制御
    森川正章, 鷲尾健司 (担当:分担執筆範囲:将来展望 バイオフィルムがもたらすブレークスルーの可能性pp 389-399, バイオサーファクタントを利用したバイオフィルムの形成と阻害pp 278-287)
    エヌティーエス 2008年
  • ナノバイオ大事典
    森川 正章 (担当:分担執筆範囲:バイオフィルム pp 420-423)
    テクノシステム 2007年
  • バイオプロセスハンドブック
    森川 正章 (担当:分担執筆範囲:4章 微生物工学の基礎 pp 111-122)
    エヌティーエス 2007年
  • 環境修復の科学と技術
    森川 正章 (担当:分担執筆範囲:第4章3節 バイオレメディエーション pp150-186)
    北海道大学出版会 2007年
  • 生物学(上)
    森川 正章 (担当:共訳範囲:14章)
    培風館 2006年
  • 食品のストレス環境と微生物
    森川 正章 (担当:分担執筆範囲:第9章1節.バイオフィルムの生成と生存メカニズム pp 221-228)
    サイエンスフォーラム 2004年
  • 農芸化学の事典
    森川 正章 (担当:分担執筆範囲:6.3.2. 直鎖状炭化水素の分解 pp749-751)
    朝倉書店 2003年
  • 微生物利用の大展開
    森川正章, ロベルト・コルター (担当:分担執筆範囲:4.2.3. バイオサーファクタント pp 993-1002, 1.3.2. バイオフィルム–微生物たちの街 pp 178-181)
    エヌティーエス 2002年
  • 生命工学
    森川 正章 (担当:分担執筆範囲:第6章 微生物工学 pp155-179)
    共立出版 2000年
  • 生物工学実験書
    森川正章, 高木昌宏, 今中忠行 (担当:分担執筆範囲:第4章(4.4.2) 第5章(5.4.2))
    培風館 1992年

講演・口頭発表等

  • Enhanced Duckweed Biomass Production Utilizing Novel Plant Growth-Promoting Bacteria  [招待講演]
    森川 正章
    China-Japan Environmental Microbiology Forum 2016, Chongqing, China 2016年11月
  • 有用微生物の農作物への新しい展開とその将来像  [招待講演]
    森川 正章
    日本生物工学会2016年度大会シンポジウム 於、富山国際会議場 2016年09月
  • Insight into aquatic plant-microbe interaction  [招待講演]
    森川 正章
    Thai Research Expo, 2016, Bangkok, Thai 2016年08月
  • 海底メタン生産環境中の共生関係機構の解析  [招待講演]
    森川 正章
    日本農芸化学会2016年度大会シンポジウム 於、札幌コンベンションセンター 2016年03月
  • 微生物伝播の足場“バイオフィルム”  [招待講演]
    森川 正章
    日本細菌学会第89回総会シンポジウム 於、大阪国際交流センター 2016年03月
  • Mutualistic biofilms- benefits for plants and animals  [招待講演]
    森川 正章
    The 27th Annual Meeting of the Thai Society for Biotechnology and international conference (TSB2015) Bangkok, Thailand 2015年11月
  • A new plant breeding technology enforcing mutualistic interaction between aquatic plants and their associated bacteria  [招待講演]
    森川 正章
    International Symposium on Microbial Research and Biotechnology for Biomass Utilization. JR HAKATA CITY, Fukuoka, Japan 2015年11月
  • 根圏微生物共生系を活用した高次植生バイオプロセスの開発  [招待講演]
    森川 正章
    2015年度北日本支部仙台シンポジウム 於、仙台市 2015年09月
  • 水生植物と表層微生物の新しい共生メカニズム  [招待講演]
    森川 正章
    日本農芸化学会2015年度大会シンポジウム 於、岡山大学 2015年03月
  • Plant growth-promoting bacteria are natural and powerful tools for enhancement of duckweed production  [招待講演]
    森川 正章
    – Construction of an international research network for duckweed and scheme for the application to water environmental improvement –SPIRITS program Kyoto University Dept. Botany, Grad. Sch. Sci., Kyoto Univ. 2015年03月
  • 微生物に魅せられて  [招待講演]
    森川 正章
    日清オイリオグループ株式会社 研究所内講演会 於、横須賀市 2014年12月
  • 水生植物の高機能化による革新的植生浄化技術の開発  [招待講演]
    森川 正章
    日本水処理生物学会第51回大会 於、甲府市 2014年11月
  • Isolation and characterization of biosurfactant producing microorganisms from natural resources in Thailand  [招待講演]
    森川 正章
    New Core to Core Program Advanced Research Networks. Bangkok, Thailand 2014年08月
  • Development of effective bioremediation technology utilizing beneficial biofilms  [招待講演]
    森川 正章
    New Core to Core Program Advanced Research Networks. Brawijaya Univesity, Indonesia 2014年08月
  • 好熱菌の諸特性〜その特異な酵素から生態まで  [招待講演]
    森川 正章
    2014年度第一回バイオ単分子研究会 於、伊豆市 2014年07月
  • Application of Beneficial Plant-Microbe Interaction for Sustainable Industry  [招待講演]
    森川 正章
    Joint Symposium on Environmental Science 2013 –Bridging Finland and Japan – at University of Helsinki, Helsinki, Finland 2013年11月
  • バイオフィルム工学による効率的な環境汚染物質分解  [招待講演]
    森川 正章
    JSR株式会社社内講演会(四日市市) 2013年09月
  • 水生植物の根圏強化による省エネ型水質浄化  [招待講演]
    森川 正章
    2013年度 環境バイオテクノロジー学会シンポジウム 於、北九州国際会議場(北九州市) 2013年06月
  • High Temperature Petroleum Reservoir Microbiology  [招待講演]
    森川 正章
    Plenary Lecture. 42nd Convention Philippine Society for Microbiology, Tagaytay, Philippine 2013年04月
  • 教育講演 細菌の生存戦略としてのバイオフィルム形成  [招待講演]
    森川 正章
    47回緑膿菌感染症研究会 2013年02月
  • Upgrading the function of aquaplants utilizing non-legume rhizobacteria  [招待講演]
    森川 正章
    International Workshop for Plant Response to Mineral Stress 2012年12月 口頭発表(招待・特別)
  • Beneficial biofilm formation by environmental bacteria in oil contaminated soils and the rhizosphere of duckweeds  [招待講演]
    森川 正章
    Microbiology Seminars at University of Helsinki 2012年10月 口頭発表(招待・特別)
  • Could the utilization of biofilms, surface attached microbial communities, lead to a game-change in green biotechnology?  [招待講演]
    森川 正章
    Lecture of Environmental Biotechnology at Aalto University 2012年10月 口頭発表(招待・特別)
  • Could the utilization of biofilms, surface attached microbial communities, lead to a game-change in green biotechnology?  [招待講演]
    森川 正章
    Royal Swedish Academy of Engineering Sciences (IVA) Lecture 2012年10月 口頭発表(招待・特別)
  • Acinetobacter calcoaceticus P23のコウキクサの根圏への付着に関する検討  [通常講演]
    蜂谷祥之, QUACH Angela, 尾形有香, 黒田真史, 井上大介, 森川正章, 池道彦
    平成24年度生物工学会 2012年10月 口頭発表(一般)
  • Beneficial biofilm formation by environmental bacteria in oil contaminated soils and the rhizosphere of duckweeds  [招待講演]
    森川 正章
    Seminar at Uppsala Biocenter SLU 2012年10月 口頭発表(招待・特別)
  • Could the utilization of biofilms, surface attached microbial communities, lead to a game-change in green biotechnology?  [招待講演]
    森川 正章
    Lecture at Technical University of Denmark 2012年10月 口頭発表(招待・特別)
  • Cyclic lipopeptide antibiotics as Hsp90 inhibitors  [通常講演]
    H. Nakamoto, Y. Yokoyama, S. Minagawa, Y. Kondoh, K. Sueoka, H. Osada, M. Morikawa
    6th International Conference on the Hsp90 Chaperone Machine 2012年09月 ポスター発表
  • 低温菌Shewanella sp. SIB1由来エステラーゼの取得および特性解析  [通常講演]
    小林隆一, 平野展孝, 森川正章, 金谷茂則, 春木 満
    平成24年度化学系学協会東北大会 2012年09月 ポスター発表
  • How do bacteria treat with interfaces and surfaces?  [招待講演]
    森川 正章
    Invited seminar at L'Oréal Aulnay Research Center 2012年09月 口頭発表(招待・特別)
  • Characterization of an extremely thermophilic bacterium, Coprothermobacter sp. PM9-2, isolated from an undersea petroleum reservoir  [通常講演]
    W. Urushibata, T. Funayama, M. Morikawa
    Extremophiles2012 2012年09月 ポスター発表
  • Anammox 細菌Candidatus‘Brocadia sinica’の膜画分に高発現するタンパク質に関する研究  [招待講演]
    東條ふゆみ, 伊東義兼, 岡部 聡, 森川正章
    平成24年度環境バイオテクノロジー学会(学会奨励賞受賞講演) 2012年06月 口頭発表(招待・特別)
  • Nitrosomonas europaeaのアンモニア酸化活性を促進する因子の同定  [通常講演]
    折山徹郎, 坂上景子, 三輪京子, 森川正章
    平成24年度環境バイオテクノロジー学会 2012年06月 口頭発表(一般)
  • Beneficial biofilm formation by environmental bacteria  [招待講演]
    森川 正章
    Invited Seminar at Harvard Medical School 2012年06月 口頭発表(招待・特別)
  • Analysis of LadA-related long-chain alkane monooxygenase in an extremely thermophilic Geobacillus thermoleovorans B23  [通常講演]
    C. Boonmak, Y. Takahashi, M. Honma, M. Morikawa
    ASM2012 2012年06月 ポスター発表
  • バイオフィルムの形成〜微生物の優れた生存戦略  [招待講演]
    森川 正章
    バイオミメティクス研究会シンポジウム 2011年12月 口頭発表(招待・特別)
  • 海底油田から単離した高度好熱菌Coprothermobacter sp. PM9-2株の諸特性解析  [通常講演]
    漆畑亘, 船山哲, 森川正章
    第12回極限環境生物学会 2011年11月 口頭発表(一般)
  • Enhancement of water purification activity by reconstructing rhizobacterial community  [招待講演]
    森川 正章
    JST-NSFC “China-Japan Workshop on Novel Remediation Technologies for Wastewater Environment Conservation" 2011年10月 口頭発表(招待・特別)
  • 有益なバイオフィルムの環境技術への利用  [招待講演]
    森川 正章
    日本歯科保存学会2011年度秋季学術大会シンポジウム 2011年10月 口頭発表(招待・特別)
  • Analysis of LadA-related long-chain alkane monooxygenase in an extremely thermophilic Geobacillus thermoleovorans B23  [通常講演]
    C. Boonmak, Y. Takahashi, M. Morikawa
    第63回日本生物工学会大会 2011年09月 口頭発表(一般)
  • Marinobacter属細菌と共存する親属海洋細菌の混合バイオフィルム形成  [通常講演]
    森川正章, 栄木悠, 柞木田なつみ, 鷲尾健司
    第63回日本生物工学会大会 2011年09月 口頭発表(一般)
  • Functional characterization of Thermococcus kodakaraensis S-layer protein in E. coli  [通常講演]
    T. Agata, W. Urushibata, T. Kanai, H. Atomi, T. Imanaka, M. Morikawa
    Thermophiles 2011年09月 ポスター発表
  • Analysis of multiple alkB genes from Geobacillus thermoleovorans B23  [通常講演]
    C. Boonmak, Y. Takahashi, M. Morikawa
    IUMS2011 2011年09月 ポスター発表
  • Purification of azoreductase from a bacterium strain that degrades Orange G dye  [通常講演]
    S. Murakami, V. Gurning, Y. Itoh, M. Morikawa
    IUMS2011 2011年09月 ポスター発表
  • Isolation of an aerobic chemoheterotroph that positively affects the activity of ammonia-oxidizing bacteria  [通常講演]
    K. Sakagami, Y. Itoh, M. Matsumoto, M. Morikawa
    IUMS2011 2011年09月 ポスター発表
  • Isolation and characterization of Rhizobium sp. R8 that forms biofilms on a toilet bowl  [通常講演]
    T. Fukano, Y. Takahashi, M. Gomi, Y. Osaki, M. Morikawa
    IUMS2011 2011年09月 ポスター発表
  • A novel thermotolerant ammonia-oxidizing bacterium, Nitrosomonas thermotolerans JPCCT2, was isolated from activated sludge in a thermal power station in Japan  [通常講演]
    Y. Itoh, M. Matsumoto, M. Morikawa
    IUMS2011 2011年09月 ポスター発表
  • Identification of novel plant-growth promoting factor produced by Acinetobacter calcoaceticus P23, a rhizobacterium of Lemna aoukikusa  [通常講演]
    S. Chida, M. Morikawa
    IUMS2011 2011年09月 ポスター発表
  • An extremely thermophilic bacterium, Coprothermobacter sp. PM9-2, isolated from an offshore petroleum reservoir in the South China Sea  [通常講演]
    W. Urushibata, T. Funayama, M. Morikawa
    国際長期生体学研究ネットワーク(ILTER)年次会議2011 2011年09月 口頭発表(基調)
  • 生物界面活性剤と微生物膜  [招待講演]
    森川 正章
    室蘭工業大学工学研究科応用理化学系専攻 講演会 2011年07月 口頭発表(招待・特別)
  • Co-beneficial biofilms on the duckweed roots  [通常講演]
    森川 正章
    FEMS 2011 4th Congress of European Microbiologists 2011年06月 ポスター発表
  • 原油汚染土壌修復技術へのバイオフィルムの適用  [通常講演]
    森川正章, 高橋康徳
    環境バイオテクノロジー学会2011年度大会 2011年06月 ポスター発表
  • Isolation of a novel thermotolerant ammonia-oxidizing bacterium, Nitrosomonas thermotolerans JPCCT2, from activated sludge in a thermal power station in Japan  [通常講演]
    Y. Itoh, M. Matsumoto, M. Morikawa
    111th ASM General Meeting 2011年05月 ポスター発表
  • Analysis of the granule formation by Anammox bacteria  [通常講演]
    F. Tojo, Y. Itoh, S. Okabe, M. Morikawa
    第一回国際アナモックスシンポジウム 2011年05月 シンポジウム・ワークショップパネル(公募)
  • 好熱性アルカン分解細菌 Geobacillus thremoleovorans B23由来 alkB 遺伝子の多様性解析  [通常講演]
    高橋康徳, チャニター ブーンマク, 森川正章
    日本農芸化学会2011年度大会 2011年03月 ポスター発表
  • 耐熱性を有する新規アンモニア酸化細菌の単離ならびに諸性質  [通常講演]
    伊東義兼, 松本光史, 森川正章
    日本農芸化学会2011年度大会 2011年03月 ポスター発表
  • 便器表面初期付着細菌群の菌叢解析とバイオフィルム形成  [通常講演]
    深野透, 高橋康徳, 五味満裕, 大崎幸彦, 森川正章
    日本農芸化学会2011年度大会 2011年03月 ポスター発表
  • 根圏作用を高度利用した次世代型環境浄化技術の開発  [招待講演]
    森川 正章
    農芸化学会研究企画賞受賞講演 2011年03月 口頭発表(招待・特別)
  • 難分解性アゾ染料Orange Gを分解する細菌およびその還元酵素の精製  [通常講演]
    村上 峻, グルニング ボルタ, 伊東義兼, 森川正章
    生化学会 2010年12月 ポスター発表
  • 超好熱始原菌Thermococcus kodakaraensis KOD1由来細胞表層タンパク質Slpを発現する細菌の凝集性およびバイオフィルム形成能の評価  [通常講演]
    漆畑 亘, 阿形朋子, 金井 保, 跡見晴幸, 今中忠行, 森川正章
    生化学会 2010年12月 ポスター発表
  • 根圏作用を高度利用した光駆動型バイオ環境浄化技術の開発  [招待講演]
    森川 正章
    北海道大学大学院農学研究院寄付分野講演会 2010年12月 口頭発表(招待・特別)
  • ウキクサ根圏細菌を利用した持続的水質浄化技術  [招待講演]
    森川 正章
    北海道バイオ産業クラスターフォーラム 技術シーズ公開会 2010年10月 口頭発表(招待・特別)
  • Biofilm formation on the duckweed roots expands substrate specificity of alkane degrading rhizobacteria  [招待講演]
    M. Morikawa
    China-Japan Workshop on Novel Remediation Technologies for Wastewater Environment Conservation 2010年10月 シンポジウム・ワークショップパネル(指名)
  • The role of urease activity on biofilm and urolith formation by Staphylococcus sp. T-02 that was isolated from a toilet bowl.  [通常講演]
    K. Oki, K. Washio, D. Matsui, Y. Hirata, M. Morikawa
    IBS2010 2010年09月 ポスター発表
  • Origin of Peroxisomal Beta-oxidation Pathway Suggested by Extremely Thermophilic Alkane Degrading Bacteria  [招待講演]
    M. Morikawa
    BIT’s 1st Annual World Congress of Petromicrobiology 2010年07月 口頭発表(招待・特別)
  • Enhanced Production of Vitamin K2 by Bacillus subtilis natto Biofilms  [招待講演]
    M. Morikawa, K. Yamazaki, H. Aibara, K.Washio
    BIT’s 3rd Annual World Congress of Industrial Biotechnology 2010年07月 口頭発表(招待・特別)
  • 耐熱性を有する新規アンモニア酸化細菌の単離ならびにその諸性質  [通常講演]
    伊東義兼, 坂上景子, 松本光史, 鷲尾健司, 森川正章
    生化学会北海道支部例会 2010年07月 口頭発表(一般)
  • アンモニア酸化細菌のアンモニア酸化活性に影響を与える従属栄養細菌  [通常講演]
    坂上景子, 伊東義兼, 松本光史, 鷲尾健司, 森川正章
    生化学会北海道支部例会 2010年07月 口頭発表(一般)
  • Sustainable biodegradation of phenol by a symbiotic Acinetobacter calcoaceticus P23 that was isolated from the rhizosphere of duckweed Lemna aoukikusa  [通常講演]
    F. Yamaga, K. Washio, M. Morikawa
    110th ASM General Meeting 2010年05月 ポスター発表
  • (p)ppGppの合成・代謝酵素SpoTによる環状リポペプチドの生産制御  [通常講演]
    鷲尾健司, リムシューピン, ルーンサワンニラン, 森川正章
    日本農芸化学会 2010年03月 ポスター発表
  • フロックを形成するアンモニア酸化細菌の単離ならびにその諸性質  [通常講演]
    伊東義兼, 松本光史, 鷲尾健司, 森川正章
    日本農芸化学会 2010年03月 口頭発表(一般)
  • Nitrosomonas europaeaのアンモニア酸化活性に影響を与える従属栄養細菌  [通常講演]
    坂上景子, 伊東義兼, 松本光史, 鷲尾健司, 森川正章
    日本農芸化学会 2010年03月 ポスター発表
  • ウキクサから単離したアルカン分解根圏細菌の評価  [通常講演]
    鈴木和也, 山賀文子, 鷲尾健司, 森川正章
    日本農芸化学会 2010年03月 ポスター発表
  • Pseudomonas 属細菌の環状リポペプチド生産制御機構  [招待講演]
    森川 正章
    北海道大学シンポジウム「北大の研究者達がつむぐ微生物の世界」 2009年12月 口頭発表(招待・特別)
  • ウキクサと根圏細菌の相利共生作用による汚染浄化法  [招待講演]
    森川正章, 鷲尾健司
    水処理生物学会 2009年11月 口頭発表(招待・特別)
  • Characterization of crude oil degrading rhizobacteria  [通常講演]
    Kazuya SUZUKI
    Summary of 12th HU-SNU Joint Symposium 2009年11月 シンポジウム・ワークショップパネル(公募)
  • 超好熱性アーキアThermococcus kodakaraensis KOD1由来細胞表在タンパク質Slpの機能解析  [通常講演]
    阿形朋子, 鷲尾健司, 金井 保, 跡見晴幸, 今中忠行, 森川正章
    生化学会 2009年10月 ポスター発表
  • 火力発電所硝化槽より単離した新規メタノール資化細菌の諸特性解析  [通常講演]
    石川絵里奈, 伊東義兼, 鷲尾健司, 松本光史, 森川正章
    生化学会 2009年10月 ポスター発表
  • Biofilm formation and effective production of menaquinone-7 (Vitamin K2) by Bacillus subtilis: Lost of the world in environmental bacteria.  [招待講演]
    Kenji Washio, Masaaki Morikawa
    Workshop Argentina-Japan “Bioscience and Biotechnology for the Promotion of Agriculture and Food Production” 2009年08月 口頭発表(招待・特別)
  • Studies on a lipopeptide biosurfactant, arthrofactin – structure, biosynthesis, transportation  [招待講演]
    森川 正章
    Invited lecture at UC Berkeley, California, 2009年08月 口頭発表(招待・特別)
  • バイオフィルムに見られるナフタレン分解活性遅延の理由  [通常講演]
    嶋田恒平, 鷲尾健司, 森川正章
    環境バイオテクノロジー学会 2009年06月 ポスター発表
  • 微生物によるジクロロメタン分解に関する研究  [通常講演]
    岩崎一弘, 中杉奈央, 大川恵, 菅田曜, 森川正章, 宮崎英男, 坂間至朗
    環境バイオテクノロジー学会 2009年06月 ポスター発表
  • Genetic analysis of synthetic regulation and transportation of lipopeptide type biosurfactant.  [招待講演]
    N. Roongsawang, S. P. Lim, K. Washio, M. Morikawa
    Biosurfactant workshop 2009年04月 口頭発表(招待・特別)
  • 微生物から見た界面の世界—バイオサーファクタントとバイオフィルム  [招待講演]
    森川 正章
    日本化粧品技術者会 2009年04月 口頭発表(招待・特別)
  • バイオフィルム利用の将来展望  [招待講演]
    森川 正章
    農芸化学会大会 2009年03月 口頭発表(招待・特別)
  • Anammox細菌のグラニュール形成に関するプロテオミック解析  [通常講演]
    東條ふゆみ, 伊東義兼, 鷲尾健司, 岡部聡, 森川正章
    農芸化学会大会 2009年03月 ポスター発表
  • 根圏細菌Acinetobacter sp. P23株のバイオフィルム形成遺伝子の探索  [通常講演]
    羽山亨, 山賀文子, 鷲尾健司, 森川正章
    農芸化学会大会 2009年03月 ポスター発表
  • バイオフィルム形成能の高いアルカン分解細菌の探索  [通常講演]
    高橋康徳, 嶋田恒平, 鷲尾健司, 森川正章
    農芸化学会大会 2009年03月 ポスター発表
  • 枯草菌バイオフィルムによるメナキノンの菌体外生産  [通常講演]
    山崎和彦, 相原悠, 大胡康, 鷲尾健司, 森川正章
    農芸化学会大会 2009年03月 ポスター発表
  • Sustainable Bioremediation Technology by Utilizing Biofilms  [招待講演]
    Morikawa, F. Yamaga, K. Shimada, K. Washio
    International symposium on Biotechnological Approaches to Environmental Science for Energy Production and Sustainability. 2009年02月 口頭発表(招待・特別)
  • 環状リポペプチド、アルスロファクチンの産生を制御する (p)ppGpp合成・代謝酵素、SpoTの機能解析  [通常講演]
    鷲尾健司, リムシューピン, ルーンサワンニラン, 森川正章
    日本分子生物学会•日本生化学会合同大会2008 2008年12月 ポスター発表
  • Staphylococcus 属細菌のバイオフィルム形成における尿素分解酵素(ウレアーゼ)の役割  [通常講演]
    大木海平, 松井大悟, 平田善彦, 鷲尾健司, 森川正章
    日本分子生物学会•日本生化学会合同大会2008 2008年12月 ポスター発表
  • バイオフィルム研究の様々な切り口ー分子、細胞、生態ー  [招待講演]
    森川 正章
    日本微生物生態学会20年度大会 2008年11月 口頭発表(招待・特別)
  • Advances in Biofilm Research to Inhibit Biocorrosion  [招待講演]
    森川 正章
    ARO workshop 2008年09月 口頭発表(招待・特別)
  • 新規アゾ染料分解脱色細菌の探索  [通常講演]
    文 Volta, R. T. Gurning, 鷲尾健司, 森川正章
    環境バイオテクノロジー学会20年度大会 2008年06月 ポスター発表
  • Efficacy of biofilm formation by naphthalene degrading Pseudomonas stutzeri T102 toward bioremediation technology.  [通常講演]
    ASM 108th 2008年06月 ポスター発表
  • Biofilm formation by Bacillus subtilis 168, incompatible function of sfp  [通常講演]
    H. Aibara, K. Washio, M. Morikawa
    ASM 108th 2008年06月 ポスター発表
  • A lipopeptide biosurfactant produced by Pseudomonas sp. MIS38, characterization and functional analyses of the synthetase gene.  [招待講演]
    M. Morikawa
    Invited lecture at East China University of Science and Technology 2008年05月 口頭発表(招待・特別)
  • Efficacy of biofilm formation by naphthalene degrading Pseudomonas stutzeri T102 toward bioremediation technology.  [招待講演]
    M. Morikawa, K. Shimada, K. Washio
    iBIO2008 2008年05月 口頭発表(招待・特別)
  • 小便器内壁から単離した細菌のバイオフィルム形成能  [通常講演]
    大木海平, 松井大悟, 平田善彦, 鷲尾健司, 森川正章
    農芸化学会 2008年03月 ポスター発表
  • Pseudomonas stutzeri バイオフィルムのナフタレン分解活性と土壌安定性  [通常講演]
    嶋田恒平, 片岡剛文, 鷲尾健司, 森川正章
    農芸化学会 2008年03月 ポスター発表
  • 超好熱性アーキアThermococcus kodakaraensis KOD1 の浮遊細胞とコロニー細胞を用いたプロテオーム解析  [通常講演]
    阿形朋子, 松見理恵, 鷲尾健司, 金井保, 跡見晴幸, 今中忠行, 森川正章
    農芸化学会 2008年03月 ポスター発表
  • 食中毒原因細菌のバイオフィルムと浮遊細胞の加熱処理耐性比較  [通常講演]
    東條ふゆみ, 佐藤 禅, 鷲尾健司, 森川正章
    農芸化学会 2008年03月 ポスター発表
  • Pseudomonas sp. MIS38株由来の二つの環状リポペプチド類ABC-トランスポーター  [通常講演]
    Siew Ping Lim, Niran Roongsawang, 鷲尾健司, 森川正章
    生化学会 2007年12月 ポスター発表
  • フタル酸エステル分解細菌の単離と諸特性解析  [通常講演]
    菅原寛明, 陳 志銘, 鷲尾健司, 森川正章
    生化学会 2007年12月 ポスター発表
  • Pseudomonas sp. MIS38株の成長相とバイオサーファクタント生産  [通常講演]
    鷲尾健司, Siew-Ping Lim, Roongsawang Niran, 森川正章
    生化学会 2007年12月 ポスター発表
  • バイオフィルムってなんだろう  [招待講演]
    森川 正章
    地球環境科学研究院公開講座「快適な環境をまもる微生物のはたらきと姿」 2007年09月 口頭発表(招待・特別)
  • 微生物の生存戦略:バイオフィルムとバイオサーファクタント  [招待講演]
    森川 正章
    日清製粉基礎研究所セミナー 2007年07月 口頭発表(招待・特別)
  • 環境微生物の生存戦略ーバイオフィルムー  [招待講演]
    森川正章, 相原 悠, 山崎和彦, 鷲尾健司
    生化学会北海道支部シンポジウム 2007年07月 口頭発表(招待・特別)
  • Pseudomonas stutzeri バイオフィルムのナフタレン分解活性と土壌安定性  [通常講演]
    嶋田恒平, 片岡剛文, 鷲尾健司, 森川正章
    環境バイオテクノロジー学会 2007年06月 口頭発表(一般)
  • 細菌バイオフィルムと浮遊細胞の耐熱性比較  [通常講演]
    東條ふゆみ, 佐藤 禅, 鷲尾健司, 森川正章
    環境バイオテクノロジー学会 2007年06月 ポスター発表
  • フタル酸エステル分解細菌の単離と諸特性解析  [通常講演]
    菅原寛明, 陳 志銘, 鷲尾健司, 森川正章
    環境バイオテクノロジー学会 2007年06月 ポスター発表
  • 非リボソーム型ペプチド合成酵素の解析と機能改変  [招待講演]
    森川 正章
    第8回 酵素応用シンポジウム 2007年06月 口頭発表(招待・特別)
  • Genes Responsible for the Transportation of Arthrofactin (Arf) in Pseudomonas sp. MIS38  [通常講演]
    Lim SP, Roongsawang N, Washio K, Morikawa M
    ASM 107th Meeting 2007年05月 ポスター発表
  • バイオフィルムとバイオサーファクタント  [招待講演]
    森川 正章
    日清製粉研究所セミナー 2007年04月 口頭発表(招待・特別)
  • 水生植物からの汚染物質分解能を有する微生物の探索  [通常講演]
    山賀 文子, 竹井 大亮, 鷲尾 健司, 森川 正章
    農芸化学会 2007年03月 口頭発表(一般)
  • 海洋性細菌を用いた複数種バイオフィルム形成能の評価  [通常講演]
    柞木田 なつみ, 岡田 千尋, 鷲尾 健司, 森川 正章
    農芸化学会 2007年03月 口頭発表(一般)
  • 枯草菌バイオフィルム形成に与えるサーファクチン生産の影響  [通常講演]
    相原 悠, 鷲尾 健司, 森川 正章
    農芸化学会 2007年03月 口頭発表(一般)
  • Pseudomonas sp. MIS38株が産生する環状リポペプチドの生成機構の解析  [通常講演]
    鷲尾 健司, Lim Siew-Ping, Roongsawang Niran, 柞木田 なつみ, 森川正章
    農芸化学会 2007年03月 口頭発表(一般)
  • 人に役立つ微生物のちから  [招待講演]
    森川 正章
    ヤクルト講演会 2006年11月 口頭発表(招待・特別)
  • 枯草菌のバイオフィルム形成に関する遺伝子と分子  [招待講演]
    森川 正章
    日本農芸化学会北海道支部ミニシンポジウム『クオルモン利用の最前線』 2006年11月 シンポジウム・ワークショップパネル(指名)
  • Isolation of biofilm-forming bacteria from marine environments  [通常講演]
    M. Morikawa, C. Okada, K. Washio, K. Takano, S. Kanaya
    SGM 159th Meeting 2006年09月 口頭発表(一般)
  • Isolation and characterization of useful bacteria for bioremediation.  [通常講演]
    森川 正章
    Tong Hai University-Hokkaido University Joint seminar 2006年08月 口頭発表(一般)
  • Isolation and characterization of bacteria that degrade DEHP.  [通常講演]
    C-M. Chen, K. Washio, K. Takano, S. Kanaya, M. Morikawa
    Tong Hai University-Hokkaido University Joint seminar 2006年08月 口頭発表(一般)
  • バクテリアの個性と社会性 —微生物群集への新たな理解を求めてー「枯草菌のバイオフィルム形成機構」  [招待講演]
    森川 正章
    第16回 根圏ネットワーク講演会『バクテリアの個性と社会性』 2006年08月 口頭発表(招待・特別)
  • 疎水環境と微生物  [招待講演]
    森川 正章
    バイオウィーク in Sapporo 2006 2006年07月 口頭発表(招待・特別)
  • 特殊環境微生物の最新研究動向と産業利用「疎水環境と微生物」  [招待講演]
    森川 正章
    バイオウィーク in Sapporo 2006年07月 口頭発表(招待・特別)
  • 海洋細菌による混合バイオフィルム形成能の評価  [通常講演]
    柞木田なつみ, 岡田千尋, 鷲尾健司, 森川正章
    環境バイオテクノロジー学会 2006年06月 ポスター発表
  • A Novel Biofilm-Forming Rhizobiales Isolated from Seto Inland Sea  [通常講演]
    C. Okada, K. Washio, K. Takano, S. Kanaya, M. Morikawa
    ASM 106th Meeting 2006年05月 ポスター発表
  • Characterization of the C-terminal thioesterase domains in arthrofactin synthetase: a prototype of two internal thioesterases  [通常講演]
    Niran Roongsawang, Kenji Washio, Masaaki Morikawa
    SGM 158th Meeting 2006年04月 口頭発表(一般)
  • 瀬戸内海バイオフィルムから単離された新属細菌の報告  [通常講演]
    岡田千尋, 金谷茂則, 森川正章
    農芸化学会 2006年03月 ポスター発表
  • P12 Structural analysis of a biosurfactant, arthrofactin, produced by Pseudomonas sp. MIS38  [通常講演]
    近藤 泰史, 川上 徹, 森川 正章, 池上 貴久
    産業用酵素国際シンポジウム 2006年02月 口頭発表(一般)
  • NMRによるアルスロファクチンの構造解析  [通常講演]
    近藤泰史, 池上貴久, 森川正章
    日本生物物理学会 2005年11月 口頭発表(一般)
  • バイオフィルムの成因と生存メカニズム  [招待講演]
    森川 正章
    第12回HACCP・微生物制御に関する講演会 2005年09月 口頭発表(招待・特別)
  • Phylogenetic analysis of condensation domain in nonribosomal peptide synthetases suggests the evolutionary relationship in the peptide donor molecules  [通常講演]
    NIRAN ROONGSAWANG, KAZUFUMI TAKANO, SHIGENORI KANAYA, MASAAKI MORIKAWA
    SGM2005 2005年04月 口頭発表(一般)
  • バイオサーファクタント生産菌Pseudomonas sp. MIS38由来非リボソーム型ペプチド合成酵素のエピメラーゼドメインの同定  [通常講演]
    Siew Ping Lim, Niran Roongsawang, Kenji Washio, Kazufumi Takano, Shigenori Kanaya, Masaaki Morikawa
    日本農芸化学会2005年大会 2005年03月 口頭発表(一般)
  • 非リボソーム型ペプチド合成酵素縮合ドメインの系統解析によってペプチド供与分子部分に進化的関係が刻まれていることが分かる  [通常講演]
    Niran Roongsawang, Kazufumi Takano, Shigenori Kanaya, Masaaki Morikawa
    日本農芸化学会2005年大会 2005年03月 口頭発表(一般)
  • プラスチック可塑剤(DEHP)を分解する細菌 Gordonia sihwensis C4の諸特性の解析  [通常講演]
    陳 志銘, 森川正章, 高野和文, 金谷茂則
    日本農芸化学会2005年大会 2005年03月 口頭発表(一般)
  • 枯草菌野生株のバイオフィルム形成に関する研究  [通常講演]
    森川 正章, 金谷茂則, 今中忠行
    日本生物工学会 2004年11月 口頭発表(招待・特別)
  • Rhodococcus属細菌TMP2のアルカン分解遺伝子群に関する解析  [通常講演]
    竹井大亮, 国広波緒, 高野和文, 金谷茂則, 森川正章
    日本生物工学会 2004年11月 口頭発表(一般)
  • Pseudoalteromonas属細菌SB-B1のバイオフィルム形成とプロテアーゼ生産性  [通常講演]
    森川 正章, 飯島沙織, 岡原良太, 高野和文, 金谷茂則
    日本生物工学会 2004年11月 口頭発表(一般)
  • 好熱性油田細菌と超好熱菌に見る生命の渾沌とした姿  [招待講演]
    森川 正章
    日本植物学会北日本支部大会 2004年09月 口頭発表(招待・特別)
  • バイオフィルム  [招待講演]
    森川 正章
    サラヤ株式会社セミナー 2003年12月 口頭発表(招待・特別)
  • Complete sequence of arthrofactin biosynthesis operon with unique two carboxy-terminal thioesterase domains.  [通常講演]
    N. Roongsawang, M. Haruki, T. Imanaka, M. Morikawa, S. Kanaya
    ASM 103th 2003年05月
  • Terrahaemophilus aromaticivorans gen nov. sp. nov., a terrestrial Pasteurellaceae isolated from petroleum sludge.  [通常講演]
    S. Hirano, M. Haruki, T. Imanaka, M. Morikawa, S. Kanaya
    ASM 103th 2003年05月
  • Oleomonas sagaranensis gen. nov., sp. nov., represents a novel genus in the alpha-Proteobacteria.  [通常講演]
    T. Kanamori, N. Rashid, M. Morikawa, H. Atomi, T. Imanaka
    ASM 103th 2003年05月
  • Structural analysis of extracellular polymeric substances (EPS) from Bacillus subtilis that forms robust pellicles.  [通常講演]
    M. Morikawa, M. Kagihiro, T. Imanaka, R. Kolter, S. Kanaya
    ASM 103th 2003年05月
  • 生物の過酷環境への適応戦略ー低温適応を中心として「バイオフィルム形成と環境適応」  [通常講演]
    森川 正章
    大阪大学蛋白質研究所セミナー 2003年03月
  • Site-specific cleavage of MS2 RNA by a thermostable DNA-linked RNase H.  [通常講演]
    C. Hyongi, T. Nogawa, Y. Tsunaka, M. Haruki, M. Morikawa, S. Kanaya
    RNase H International Conference 2002 2002年09月
  • Structural and functional analyses of archaeal Type 2 ribonuclease H.  [通常講演]
    A. Muroya, D. Tsuchiya, M. Ishikawa, M. Haruki, M. Morikawa, S. Kanaya, K. Morikawa
    RNase H International Conference 2002 2002年09月
  • Cleavage of a double-stranded DNA containing a single ribonucleotide at the DNA-RNA junction with prokaryotic RNases HII  [通常講演]
    M. Haruki, Y. Tsunaka, M. Morikawa, S. Kanaya
    RNase H International Conference 2002 2002年09月
  • 環境に役立つ微生物たち  [招待講演]
    森川 正章
    ボストン日本人研究者交流会 2002年01月 口頭発表(招待・特別)
  • The world of extremophilic oil bacteria  [招待講演]
    MORIKAWA, Masaaki
    Seminar at Department of Molecular and Cellular Biology, Harvard University 2001年07月 口頭発表(招待・特別)
  • Long-chain-alkane degradation by extremely thermophilic Bacteria.  [通常講演]
    M. Morikawa, T. Kato, M. Haruki, T. Imanaka, S. Kanaya
    ASM 101th 2001年05月
  • 環境バイオテクノロジー:基礎研究の戦略と事業化への展開  [招待講演]
    森川 正章
    日本化学工学会シンポジウム 2001年04月 口頭発表(招待・特別)
  • Biological oil production from CO2.  [通常講演]
    T. Imanaka, M. Morikawa
    Pacifichem 2000 2000年12月
  • Gene cloning and characterization of an aldehyde dehydrogenase and an esterase from a petroleum degrading strain HD-1.  [通常講演]
    M. Morikawa, S. Mizuguchi, N. Okibe, M. Haruki, T. Imanaka, S. Kanaya
    Pacifichem 2000 2000年12月
  • An extreme-thermophile which degrades petroleum under high temperature conditions.  [通常講演]
    T. Kato, A. Miyanaga, M. Haruki, T. Imanaka, M. Morikawa, S. Kanaya
    Pacifichem 2000 2000年12月
  • Thermophilic bacteria isolated from a subterranean petroleum reservoir.  [通常講演]
    M. Morikawa, T. Kato, M. Haruki, T. Imanaka, S. Kanaya
    Gratama Workshop 2000 conference 2000年04月
  • CO2 fixation and alkane production by an oil-bacterium strain HD-1.  [招待講演]
    M. Morikawa, H. Atomi, T. Imanaka
    International Symposium on Autotrophy and Hydrogen Biotechnology 2000年02月 口頭発表(招待・特別)
  • CO2固定細菌を利用した地球環境修復システムの構築  [招待講演]
    森川 正章
    近畿バイオインダストリー振興会議第一回技術シーズ公開会 1999年09月 口頭発表(招待・特別)
  • 資源をつくる微生物  [招待講演]
    森川 正章
    日本農芸化学会ミニシンポジウム 1998年07月 口頭発表(招待・特別)
  • Isolation of a petroleum degrading/producing bacterium  [通常講演]
    M. Morikawa, S. Jin, K. Amada, M. Haruki, S. Kanaya, T. Imanaka
    International Congress on Extremophiles '98 1998年01月
  • Petroleum degrading/producing bacterium HD-1 with its unique characters.  [通常講演]
    M. Morikawa, S. Kanaya, T. Imanaka
    Asian Nitrogen-Fixation Symposium under JSPS and Monbusho Programme 1997年12月
  • A new type of petroleum-degrading/producing bacterium HD-1.  [通常講演]
    M. Morikawa, T. Imanaka
    International Workshop on Ultra-long term Cryogenic Preservation Network of Biological and Environmental Specimens 1997年11月
  • Production of alkane and alkene from CO2 by a petroleum-degrading bacterium strain HD-1.  [通常講演]
    M. Morikawa, T. Iwasa, S. Yanagida, T. Imanaka
    Fourth International Conference on Carbon Dioxide Utilization 1997年09月
  • Studies on the structure-function relationship of lipopeptide biosurfactants.  [通常講演]
    M. Morikawa, T. Imanaka
    International Society for Environmental Biotechnology 3rd International Symposium 1996年07月
  • A new mixotrophic bacterium which can fix CO2 and assimilate aliphatic and aromatic hydrocarbons anaerobically.  [通常講演]
    T. Imanaka, M. Morikawa
    International Society for Environmental Biotechnology 3rd International Symposium 1996年07月
  • 「極限環境における生体の分子論的応答」有機溶媒:バイオサーファクタントと石油代謝細菌  [招待講演]
    森川 正章
    大阪大学蛋白質研究所セミナー 1996年01月 口頭発表(招待・特別)
  • ヒト・リゾチームの構造・機能相関解析  [招待講演]
    森川 正章
    生物工学若手研究者の集い 1989年07月 口頭発表(招待・特別)

所属学協会

  • 環境バイオテクノロジー学会   日本生化学会   新資源生物変換研究会 常任幹事   米国微生物学会   日本農芸化学会   日本生物工学会   ポリリン酸研究会   NEDO技術委員   American Society for Microbiology   Study Group of Polyphosphate   Japan Society for Environmental Biotechnology   and Agrochemistry   Biotechnology   Japan Society for Bioscience   Japan Society for Biotechnology   

Works(作品等)

  • 平成23年度北海道大学大学院地球環境科学研究院公開講座 「生物の環境への適応」
    2011年
  • オープンキャンパス2011 (北大理学部)
    2011年
  • プロフェッサービジット2009
    2010年
  • プロフェッサービジット2010
    2010年
  • オープンキャンパス2010(北大理学部)
    2010年
  • ボストン日本人研究者交流会(於,マサチューセッツ工科大学) 「環境に役立つ微生物たち
    2002年
  • 日本化学工学会シンポジウム 環境バイオテクノロジー:基礎研究の戦略と事業化への展開 展望講演「CO2固定細菌と油田細菌の環境修復技術への可能性」
    2001年
  • International Symposium on Autotrophy and Hydrogen Biotechnology (於,東京YMCA)"CO2 fixation and alkane production by an oil-bacterium strain HD-1."
    2000年
  • 近畿バイオインダストリー振興会議第一回技術シーズ公開会 (於,大阪科学技術センター) 「CO2固定細菌を利用した地球環境修復システムの構築
    1999年
  • 日本農芸化学会ミニシンポジウム(於,大阪府立大学) 「資源をつくる微生物」
    1998年
  • 大阪大学蛋白質研究所セミナー(於,大阪大学) 「極限環境における生体の分子論的応答」 〜有機溶媒:バイオサーファクタントと石油代謝細菌
  • 平成16年度北海道大学大学院地球環境科学研究科公開講座 「地球環境をまもる微生物たち」

共同研究・競争的資金等の研究課題

  • 日本学術振興会:科学研究費助成事業 挑戦的研究(開拓)
    研究期間 : 2021年07月 -2024年03月 
    代表者 : 森川 正章
  • 科学技術振興機構/国際協力機構 (JST/JICA):SATREPS
    研究期間 : 2020年08月 
    代表者 : 森川正章
  • 科学技術振興機構 (JST):先端的低炭素化技術開発 (ALCA)
    研究期間 : 2016年09月 -2020年03月 
    代表者 : 森川正章
  • JSPS:科学研究補助金:挑戦的萌芽研究
    研究期間 : 2016年04月 -2018年03月 
    代表者 : 森川 正章
  • 科学技術振興機構 (JST):先端的低炭素化技術開発 (ALCA)
    研究期間 : 2011年10月 -2016年08月 
    代表者 : 森川 正章
  • 高度好熱菌性油田細菌のアルカン代謝および生態に関する研究
    JSPS:科学研究費基盤B一般
    研究期間 : 2010年 -2012年 
    代表者 : 森川 正章
  • バイオフィルム工学による微生物のデザイン化
    NEDO:受託研究「微生物機能を活用した環境調和型製造基盤技術開発」
    研究期間 : 2007年 -2011年 
    代表者 : 森川 正章
  • バイオフィルム形成分子機構を切り口とした微生物未知機能の解明
    JSPS:科学研究費基盤B一般
    研究期間 : 2007年 -2009年 
    代表者 : 森川 正章
  • バイオフィルムを利用した環境修復技術の開発
    (財)発酵研究所:発酵研究所研究助成
    研究期間 : 2006年 -2008年 
    代表者 : 森川 正章
  • 寒冷条件に対応した次世代汚染土壌修復技術の開発
    METI:受託研究 (中小企業ベンチャー挑戦支援事業)
    研究期間 : 2008年 
    代表者 : 森川 正章
  • 非リボソーム型ペプチド合成酵素の解析と機能改変
    (株)天野エンザイム:酵素応用シンポジウム奨励賞
    研究期間 : 2007年 
    代表者 : 森川 正章
  • 脂溶性機能性食品成分の菌体外分泌システム開発
    (財)食生活研究会:食生活研究会研究助成
    研究期間 : 2007年 
    代表者 : 森川 正章
  • バイオフィルム工学を利用した生物環境修復技術の開発
    J-Power:共同研究 (J-Power 50周年記念先端技術共同研究)
    研究期間 : 2005年 -2006年 
    代表者 : 森川 正章
  • Arthrofactin 合成反応の分子メカニズム
    JSPS:科学研究費基盤C一般
    研究期間 : 2005年 -2006年 
    代表者 : 森川 正章
  • 病原微生物データ分析実験作業
    (財)食品産業センター:受託研究 食品製造工程管理情報高度化促進事業
    研究期間 : 2006年 
    代表者 : 森川 正章
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 2004年 -2005年 
    代表者 : 森川 正章, ROONGSAWANG Niran
     
    非リボソーム型ペプチド合成酵素は生理活性のある非常に多様な複合/環状ペプチド類を合成することができる。合成最終段階の環状化反応と産物の遊離は合成酵素のC末端に存在するチオエステラーゼドメイン(TE)の働きにより進行する。Pseudomonas属細菌MIS38が有するarthrofactin合成酵素は3つのサブユニット(ArfA/B/C)から構成される。興味深いことにArfCのC末端には2つのTEが存在する。いずれのTE(TE1,TE2)も活性発現に必須のSr/Asp/Hisを有している。本研究では、これらのTEが合成反応にどのように係わっているのかを解明することを目的とした。 当該遺伝子部分を大腸菌用ベクターを用いてクローニングした後、PCR法を用いて部位特異的突然変異遺伝子を構築した。さらにこの変異遺伝子を相同性組み換え法によりMIS38染色体に戻した。こうして、S91A,S91T,S383A,S383/D410A変異株を作製した。塩基配列解析を行い、それぞれの位置以外に突然変異が導入されていないことを確認した。こうして得られた変異株のarthrofactin生産性を調べた。その結果、S91A,S91T変異株は生産性を完全に失っていた。一方、S383AおよびS383A/D410A変異株は野生株に比べて5±1%の活性を保持していた。またこれら変異株が生産するarthrofactinは野生株のものと同一の構造であることを確認した。以上の結果から、S91を含むTE1が環状化反応と産物の遊離に必須であり、TE2は本質的に重要ではないことが判明した。現在,この仮説を証明するためにTE2を完全に決失した変異株を作成中である。
  • 汚染土壌微生物生態を利用した環境修復技術の開発
    住友財団:
    研究期間 : 2005年 
    代表者 : 森川 正章
  • 革新的リボソーム非依存型複合ペプチド合成酵素に関する研究
    武田科学振興財団:武田科学振興財団奨励金一般研究
    研究期間 : 2005年 
    代表者 : 森川 正章
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 2003年 -2003年 
    代表者 : 谷田 純, 森川 正章
     
    空間符号モアレマッチング技術を基本としたゲノム解析手法の開発を通して,その有効性,特牲,問題点を明らかにするとともに,ゲノム情報処理分野における情報フォトニクス技術応用の可能性を探ることを目的とする.本年度に得られた知見は以下の通りである. 1.昨年度考案したカラー空間符号モアレマッチング技術を実装したプログラム(MTerm)により,各種細菌類を対象とした全ゲノム比較を行い,有効性,特性,問題点を評価した.ほとんどの比較において一様なモアレ縞が観測され,モアレ縞が観測されないほうがむしろ稀であることを確認した.また,出現頻度符号化を用いた場合,区切り枠の取り方により一致線が分裂する現象を見いだし,その対策として,MTermに区切り枠の調整機構を付加した. 2.ゲノム配列内に存在する逆位の検出性に対する検討を行った.配列塩基種の相補塩基への変換,塩基の配置方向の反転などの機能をMTerm付加した.大腸菌O157EDL933株と同sakai株に適用し,配列多重度10000においても逆位部位の検出が行えることを確認した. 3.配列一致部位の自動検出をめざして,出力モアレ縞画像に対する特徴抽出処理の検討を行った.移動平均法の多重適用,閾値処理による二値化,膨張・収縮処理によるノイズ成分除去の一連の処理により,良好な特徴抽出結果が得られることを確認した.さらに,処理画像に対する情報圧縮により,1/500程度の圧縮率が得られることを確認した.
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 2002年 -2003年 
    代表者 : 春木 満, 森川 正章
     
    当該研究は、フェノール処理などの操作を不要とすることにより、組換えDNA実験のグリーン化を進めることを目指し、熱失活性のApase、RNase A、制限酵素の開発を目的とする。また、通常低温で行われる連結反応の効率化を目指し、低温において高い活性を有するDNAリガーゼの開発を目的とする。 SIB1株由来のAPaseの諸特性を解析したところ、至適反応温度は約40℃であり、大腸菌由来酵素と比較して約20℃低温側にシフトしていた。また安定性も大腸菌由来酵素が80℃で1時間処理しても60%の活性を保持するのに対して本酵素は80℃で5分処理するだけで速やかに失活した。本酵素は40℃での酵素反応において大腸菌由来酵素と比べて5倍以上高い触媒効率を示し、20℃でも十分な活性を維持していることがわかった。 低温菌DNAリガーゼについては、近縁でゲノム配列の解読されているS.oneidensisのDNAリガーゼの遺伝子の配列をもとにPCRプライマーを合成し、SIB1株のゲノムDNAを鋳型としてPCRを行った結果、600bpの断片が増幅された。この断片の塩基配列を決定したところ、そのコードするアミノ酸配列は、S.oneidensisのDNAリガーゼと77%の同一性を示し、SIB株のDNAリガーゼ遺伝子の一部であることがあきらかとなった。 RNase Aおよび制限酵素Bg1IIの熱失活性変異体を取得するために、これらの酵素遺伝子に6×Hisタグ配列を付加し、M13ファージのpIIIコート蛋白質遺伝子のN末端に挿入した。構築した遺伝子をもつ大腸菌にヘルパーファージを感染させ、ファージ粒子を調製し、抗M13抗体を用いたELISA法により、Ni-NTAプレートへの結合を調べたが、プレートへの特異的結合はみられなかった。したがって、酵素がファージ上へうまくディスプレイされていないと考えられる。
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 2002年 -2002年 
    代表者 : 谷田 純, 森川 正章
     
    空間符号化法を用いた配列比較技術に対して,符号化法の改良や専用視覚化端末の開発を通し,全ゲノム配列比較への拡張手法に関する種々の検討を行った.また,これらの手法を各種大腸菌の全ゲノムやヒト染色体などの実配列に適用し,その有効性を評価した.その結果,以下に示す成果を得た. 1.単一ディスプレイ上でマッチング処理を実行するためのソフトウェアを開発し,これまでに考案した種々の符号化法を実装した.さらに,符号化画像の更新や選択配列部位の切り出しなどの様々な機能を付加させることにより,専用視覚端末の利便性を向上させた. 2.長大な2配列間のマッチング結果を同時に提示するため,対象配列を一定の長さを有する部分配列に分割し,部分配列内の各塩基要素を符号パターンに反映させる出現頻度符号化法を考案した.この符号化法を用いることで,数10万塩基長に及ぶ2配列間のマッチング結果を同時に表示できることを確認した. 3.出現頻度符号化法により得られる出力結果から,配列間の部分一致性や欠失・挿入だけでなく,配列内の塩基組成分布に関する様々な情報を抽出できることを新たに見出した.さらに,出現頻度符号の配色を工夫することで,DNA配列解析において重要であるGC含有量を出力結果から直感的に把握できることを実験的に確認した. 4.出現頻度符号化法、およびその部分配列長の可変機能を専用端末上に実装し,微視レベルから巨視レベルまでのマルチスケールな配列比較を統合して扱える環境を構築した.この符号化法を用いて,大腸菌K-12株と病原性大腸菌O-157:H7株を比較し,全ゲノム配列から部分一致性を抽出することに成功した.
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 2001年 -2001年 
    代表者 : 森川 正章
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 2001年 -2001年 
    代表者 : 谷田 純, 森川 正章
     
    配列情報の空間符号化を利用した配列間マッチング技術に対して,符号化規則の変更や出力モアレ縞の解釈によって得られるゲノム配列間の情報抽出法を検討した.これらの手法を,公開ゲノム配列データベースより取得したDNA及び,アミノ酸配列に適用し,評価を行った.その結果,以下に示す成果を得た. 1.モアレ情報端末の利用性向上のため,液晶ディスプレイ上に2配列の符号化画像を表示する方式を検討し,所望のマッチング結果を得ることに成功した.これより,コンピュータ制御による簡易視覚端末が実現できることを確認した. 2.アミノ酸配列間の類縁性を含めた比較情報を抽出するため,疎水性パラメータを空間符号に導入する手法を考案し,弱相関配列の検出を試みた.既存のホモロジー検索ツール,モチーフ抽出ツールとの比較から,アミノ酸配列比較技術としての有効性を示した. 3.ドットプロット法との比較により,提案手法が有する特長を明らかにした.モアレ現象の特性により適度な情報抽出が行われ,DNA配列に対してもフィルタリング処理なしで有用な情報が抽出できる点,表示に必要なデータ数を減少でき,高速かつ簡便にデータ更新が行える点,検査範囲が等しければ,より高い視認性で出力が得られる点などである. 4.高密度符号化法を開発し,10万要素の同時比較の可能性を示すことができた.いくつかの特定の縦列反復配列部位において観察される特徴的な2次元モアレパターンを明らかにした.また,処理手順を整理し,自己相関相互相関,反転相関の有用性を示した.これらの成果より,2配列間の類似性を鳥瞰的に視覚化する手法の体系化を行い,提案手法のもつ多様な情報抽出の可能性を提示した.
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 2000年 -2000年 
    代表者 : 谷田 純, 森川 正章
     
    光演算技術は,大容量情報に対する並列処理性と,人間の優れたパターン認識能力を誘起する情報可視性をあわせ持ち,それらの有効利用はゲノム情報処理の効率化に寄与しうる.本研究では,その具体的手法として,空間符号モアレ法による2配列間マッチング演算を対象とし,特性,および,有効性を評価した. 空間符号モアレ法では,符号パターンや実現方法により,出力情報の加工が可能である.相補配列の検出能力をもつ対称型符号パターンを用いて,ステムループ構造の抽出が行えることを確認した.次に,濃度反転符号と非反転符号の組合せによる一致信号の先鋭化技術を考案し,従来方式では不可能であった1塩基置換によるミスマッチの検出を実現した.また,3色の符号パターンにより,3配列間マッチング処理を実現した. 一方,検討手法の簡便な利用をめざして,マッチング情報端末を試作した.2台の液晶ディスプレイ画面を半透鏡で合成する方式と,1台の液晶ディスプレイ画面に印刷済透明シートを張り合わせる方式とを実装した.後者の方式は,データ操作の自由度では劣るものの,視認性の点で極めて優れている. 光演算技術に基づく情報システムとして,自由空間光インターコネクションによる配列マッチング専用プロセッサの基本構成を検討した.空間符号を時分割展開した時間符号が処理スループットの点で優れていることを見い出し,予備実験により原理確認を行った. 空間符号モアレ法は,ホモロジー検索の基本演算であるドット・プロット法と等価な信号を出力する.しかし,モアレ縞は,各要素のマッチング結果が継ぎ目なく表されるアナログ画像情報である.その結果,人間のパターン認識能力をより強く誘起しうる可能性をもつ.符号化については,視覚特性を考慮する必要がある.一つの展開方向として,動態視の利用によりマッチング識別能力を向上させる方式が考えられる.
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 1996年 -1997年 
    代表者 : 森川 正章
     
    油田から分離したHD-1株は好気・嫌気の両条件下において,脂肪族および芳香族炭化水素を資化する通性嫌気性の石油分解細菌である。本研究課題においてはHD-1株を始めとする細菌の嫌気(無酸素)条件下における石油分解機構の解析を目的として研究を進めた。HD-1株を用いてテトラデカン(アルカン)の無酸素条件下での分解を検討した結果、2種類のアルケンが代謝中間体として検出できた。このうちの主成分についてFT-IR,^1H-NMR,GC/MS法などを駆使して構造を決定したところ1-ドデセン(アルケン)であることが判った。この結果は本菌が無酸素条件下において脱水素反応によりアルカンを酸化分解することを示すものである。これまでにアルカンの嫌気分解については我々の研究以外にドイツで1例のみ報告されているが、代謝中間体を解析した結果は今回が始めてである。さらに、本菌は石油がなくともCO_2を単一炭素源として生育することが可能であり、その菌体内には石油成分であるアルカンが乾燥菌体重量当たり0.1%程度合成されることを見い出した。この代謝機構の詳細な検討は今後の課題である。また、最近、新たに無酸素条件下で石油を分解するTK-122株を石油備蓄タンクから分離した。本菌の石油分解能力はHD-1株に比べてはるかに高く、嫌気条件下においても石油成分であるアルカン(オクタンからヘキサデカンまで)を3日間で約70%分解した。さらに嫌気分解時における電子受容体を検討した結果、MoO4^<2->(VI)であることが判った。この結果は従来にない新しい石油分解酵素発見の可能性を示唆する。また16SrRNA遺伝子の塩基配列から本菌はEschericiha属あるいはCitrobacter属に近縁の細菌であることが予想されたが、生理学試験ではいずれも一致しなかった。 以上の結果、TK-122株は新属細菌であると思われる。
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 1995年 -1995年 
    代表者 : 森川 正章, 今中 忠行
     
    【1】アルカン/アルケン生合成経路の解明 まず、生物学的にCO_2からアルカン/アルケンを合成する経路のなかで最も研究が遅れており、実際反応律速になっている可能性が高いと思われる脂肪酸からアルカン/アルケンへの変換反応について検討した。緑藻類などを用いた研究結果からは脂肪酸から直接アルカン/アルケンを合成しているのではなく、脂肪酸からアルデヒドになった後アルカン/アルケンに変換される可能性が示唆されている。そこでHD-1株が最も多く蓄積していたヘキサデカン(C16)の前駆物質であると予想されるパルミチン酸あるいはヘキサデカナ-ルを使ってアルカン/アルケンの生成が実際に起こるかを調べた。^<14>C-パルミチン酸は市販のものを利用した。^<14>C-ヘキサデカナ-ルは入手不可能であったため^<14>C-パルミチン酸から化学合成した。アルカン/アルケンの生成反応は以下のようにして行った。基質である^<14>C-パルミチン酸あるいは^<14>C-ヘキサデカナ-ルを含むリン酸緩衝液(pH7.0)/1% Triton X-100をナスフラスコ内でArガス通気により脱酸素処理する。同様に脱酸素処理した細胞抽出液を嫌気性ボックス内で添加後密栓する。これを遮光した湯溶中で37℃24時間保温した。反応産物を含む疎水性画分をクロロホルム抽出し、気質のみで保温したコントロールと共にシリカゲル60TLC(ヘキサンおよびヘキサン,ジエチルエーテル,ギ酸)で展開し、脂肪酸あるいはアルデヒド画分(Rf=0.5-0.7)とアルカン/アルケン画分(Rf=0.9以上)を厳密に分けて回収した。液体シンチレーションカウンターによりそれぞれの放射活性を測定した。この結果から、微量ではあるが細胞抽出液を加えた場合にのみアルカン/アルケンの生成が確認できた。さらに脂肪酸にくらべてアルデヒドの方がアルカン/アルケンの生成率が良いことか、細菌においても脂肪酸はアルデヒドを経由してアルカン/アルケンに変換されることが強く示唆された。現在細胞抽出液をカラムクロマトグラフィーなどにより分画して、本酵素活性(アルデヒドデカルボニラーゼ)の精製を目指している。 【2】アルカン/アルケン合成能力の向上 本プロジェクトが実際に地球環境レベルで貢献できるにはHD-1株の生育速度を高めると共にアルカン/アルケンの蓄積量を飛躍的に増大する必要がある。そこで、人為的突然変異処理を繰り返してこの目的に合った変異株を効率良く選別する方法を検討した。突然変異処理法は細菌において最も強力で汎用的なニトロソグアニジン処理を採用した。処理条件は生存率10%〜50%を設定(100mg/1,37℃,30分間)した。アルカン/アルケンの合成能力の高くなった株はプレート上では元株と容易には区別できない。そこで比重の違いを利用した。すなわちアルカン/アルケンを含む疎水性成分の細胞内含量が高いものは他にくらべて軽くなっていると予想した。比重の違いで生体物質を分画するのに最も簡便な方法のひとつが密度勾配遠心分離法である。そこで細胞を分画するための無菌的密度勾配遠心分離の最適条件検討を策定した。遠心分離後、上層から注意深く溶液を10区画(No.1〜No.10)に分けて回収した。これをプレートに広げて単一細胞を単離して最も比重の軽い細胞(No.5)、中程度の細胞(No.7)、最も重い細胞(No.10)を選んでそれぞれの大量培養後、疎水性成分含量を比較した。取得したNo.5は変異剤未処理の約3倍の疎水性物質を蓄積していた。現在ガスクロマトグラフィーにより疎水性成分(アルカン/アルケン含量など)を分析中である。以上の結果から、突然変異処理(ニトロソグアニジンおよび紫外線照射)と密度勾配遠心分離による選別により、アルカン/アルケンの高生産性突然変異株の取得が可能であることが確認できた。今後、この操作を繰り返すことによってHD-1株のアルカン/アルケン生成能力を可能な限り増強させる予定である。
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 1993年 -1995年 
    代表者 : 今中 忠行, 森川 正章
     
    【1】HD-1株宿主-ベクター系の開発 HD-1株を宿主とした形質転換系を構築することを目的としてまず、各種抗生物質に対する耐性をしらべた。その結果、カナマイシン(Km)、テトラサイクリン(Tc)、アンピシリン(Ap)、クロラムフェニコール(Cm)、カルベニシリン(Cd)に対する耐性は全くなく(5μg/ml以下)、ストレプトマイシン(Sm)に対しては10μg/mlが生育限界濃度であった。続いてこれまでに開発されたPseudomonas属を含むグラム陰性細菌に広く利用されている広宿主域ベクターや大腸菌用のベクターなどを中心にエレクトロポレーション法によるHD-1株の形質転換実験を行った。それぞれのベクターにコードされている各種薬剤耐性を獲得した細胞を形質転換体として選択した。その結果、グラム陰性用広宿主域ベクターRSF1010によってHD-1株の形質転換が可能であることが判った。細胞を懸濁する溶液としては10%グリセロールが適していると思われた。実際に、Sm耐性株(形質転換体)からプラスミドを抽出してアガロースゲル電気泳動で調べた結果、RSF1010の存在が確認できた。この結果は、RSF1010はHD-1株細胞内で独立複製可能であることも示している。種々の条件を検討した結果、HD-1株の形質転換最適条件は以下の通りである。宿主(HD-1株),定常期前期菌体:ベクター,RSF1010(Sm^r):選択圧,Sm20μg/ml:電気パルス(方形波):電界強度,5kV/cm:パルス幅,1ms:遺伝子発現までの培養時間,3時間。以上の条件で得られる最大形質転換頻度は3.3×10^<-5>transformants/viable cell、最大形質転換効率は1.1×10^5transformants/μgDNAであった。 【2】アルカン/アルケン生合成経路の解明 まず、生物学的にCO_2からアルカン/アルケンを合成する経路のなかで最も研究が遅れており、実際反応律速になっている可能性が高いと思われる脂肪酸からアルカン/アルケンへの変換反応について検討した。緑藻類などを用いた研究成果からは脂肪酸から直接アルカン/アルケンを合成しているのではなく、脂肪酸からアルデヒドになった後アルカン/アルケンに変換される可能性が示唆されている。そこでHD-1株が最も多く蓄積していたヘキサデカン(C16)の前駆物質であると予想されるパルミチン酸あるいはヘキサデカナ-ルを使ってアルカン/アルケンの生成が実際に起こるかを調べた。^<14>C-パルミチン酸は市販のものを利用した。^<14>C-MEKISAデカナ-ルは入手不可能であったため^<14>C-パルミチン酸から化学合成した。アルカン/アルケンの生成反応は以下のようにして行った。基質である^<14>-パルミチン酸あるいは^<14>C-ヘキサデカナ-ルを含むリン酸緩衝液(pH7.0)/1%Triton X-100をナスフラスコ内でArガス通気により脱酸素処理する。同様に脱酸素処理した細胞抽出液を嫌気性ボックス内で添加後密栓する。これを遮光した湯浴中で37℃24時間保温した。反応産物を含む疎水性画分をクロロホルム抽出し、基質のみで保温したコントロールと共にシリカゲル60TLC(ヘキサンおよびヘキサン,ジエチルエーテル,ギ酸)で展開し、脂肪酸あるいはアルデヒド画分(Rf=0.5-0.7)をアルカン/アルケン画分(Rf=0.9以上)を厳密に分けて回収した。液体シンチレーションカウンターによりそれぞれの放射活性を測定した。この結果から、微量であるが細胞抽出液を加えた場合にのみアルカン/アルケの生成が確認できた。さらに脂肪酸にくらべてアルデヒドの方がアルカン/アルケンの生成率が良いことから、細菌においても脂肪酸はアルデヒドを経由してアルカン/アルケンに変換されることが強く示唆された。現在細胞抽出液をカラムクロマトグラフィーなどにより分画して、本酵素活性(アルデヒトデカルボニラーゼ)の精製を目指している。
  • 日本学術振興会:科学研究費助成事業
    研究期間 : 1994年 -1994年 
    代表者 : 森川 正章, 今中 忠行
     
    原材料をCO_2ガス、最終産物を石油成分(特にパラフィン系炭化水素)とする一連のプロセス(炭素物質循環系)の構築を前提として油田土壌から分離されたHP-1株代謝経路の解明ならびに菌株を改良することが本研究の目的である。本年度はHP-1株がCO_2から炭化水素を生成できることの確認とその代謝経路の推定、および遺伝子組み換え法により本菌株を改良するための基盤を確立することを目的とした。 先ず、CO_2を単一炭素源とする培地0.5%(NH_4_2SO_4,0.1%KH_2PO_4,0.05%MgCl_2・6H_2O/水道水(pH7.0)にCO_2を含む混合嫌気ガス(CO_2:H_2:N_2=5:5:90)を通気して37℃2週間培養した。増殖した菌体を遠心分離により回収・洗浄したのち凍結乾燥した。クロロホルム抽出によって調製した疎水性画分についてGC分析を行った結果、パラフィンに相当する位置にピークが検出されたため、さらにGC-MSによる質量数の決定ならびに構造の推定を行った。親イオンピークならびにフラグメントイオンピークの特徴から脂肪酸(パルミチン酸、ステアリン酸)以外に質量数278と226のパラフィン(それぞれ、エイコサジエンならびにヘキサデカン)が確認できた。以上の結果、HP-1株はCO_2とH_2から石油主成分であるパラフィンを生産することを確認した。 次に、本菌のCO_2固定能力ならびにパラフィン合成能力を強化するために遺伝子組み換え基盤技術の確立をめざした。汎用プラスミドベクター14種類についてエレクトロポレーション法によりHD-1株の形質転換を試みたところ、グラム陰性細菌用ベクターRSF1010(Sm^r)によりパルス条件10kV/cm 1 mses2回により2.3×10^3/μg DNA の頻度で形質転換可能であることを見いだした。本研究成果によりCO_2固定経路とパラフィン合成経路における律速段階を触媒する酵素遺伝子群を遺伝子工学的に強化できる見通しがついた言える。それぞれの代謝経路についてその機構を解析することが今後の課題である。
  • Petroleum degrading and producing bacteria (under low temperature, low oxygen conditions) Bioremediation technology (Encocrine disruptant degrading bacteria) Biosynthetic pathways of biosurfactant (Non-ribosomal peptide synthetase) Biofilm formation (M・・・
    Petroleum degrading and producing bacteria (under low temperature, low oxygen conditions) Bioremediation technology (Encocrine disruptant degrading bacteria) Biosynthetic pathways of biosurfactant (Non-ribosomal peptide synthetase) Biofilm formation (Marine bacteria, Bacillus, Hyperthermophiles)

産業財産権

  • 特願2014-148493:植物成長強化剤及びそれを用いた植物栽培方法  2014年07月22日
    鈴木 和歌子, 菅原 雅之, 三輪 京子, 森川 正章, 玉木 秀幸, 牧野 彩花, 鎌形 洋一
  • 特願WO2017002929A1:植物の生長を促進する方法、植物生長促進物質を製造する方法及びこれらに利用されるタンパク質  2015年06月30日
    森川正章, ジョグ ラフル, 菅原雅之, 三輪京子
  • 特許第4955039号:土壌汚染浄化方法    2012年03月23日
    長谷川武, 平本弘, 山本英樹, 岡崎修, 森川正章
  • 特開2011-030487:キノン類の製造方法  2011年02月17日
    森川正章, 大胡康, 鈴木良雄  
    特願2009-179141
  • 特開2009-247279:新規水草根圏微生物  2009年10月29日
    森川正章, 鷲尾健司, 山賀文子
  • 特許第3507890号:Shewanellasp.SIB1株由来の新規なアルカリフォスファターゼ    2004年01月09日
    金谷 茂則, 森川 正章, 春木 満
  • 特許第3120114号:アルカン類を分解する新規微生物、アルカン類を分解する方法  
    森川 正章, 加藤 智久
  • 特開2000-354496:核酸の増幅方法およびその試薬  2000年12月26日
    北林 雅夫, 荒川 琢, 井上 浩明, 川上 文清, 川村 良久, 今中 忠行, 高木 昌宏, 森川 正章
  • 特開2000-23687:熱安定性DNAポリメラ―ゼ  2000年01月25日
    北林 雅夫, 荒川 琢, 井上 浩明, 川上 文清, 川村 良久, 今中 忠行, 高木 昌宏, 森川 正章
  • 特開平11-056349:蔗糖脂肪酸エステル合成酵素を産生する微生物  1999年03月02日
    今中 忠行, 森川 正章, 西畑 隆男, 神野 和人
  • 特開平11-056364:薯糖脂肪酸エステラーゼ  1999年03月02日
    今中忠行, 森川正章, 西畑隆男, 神野和人
  • 特開平11-32773:耐熱性グリセロールキナーゼ及びそれをコードするDNA  1999年02月09日
    金谷茂則, 森川正章
  • 特開平10-306098:環状リポペプチド化合物の化学合成方法および環状リポペプチド化合物  1998年11月17日
    今中 忠行, 平田 善彦, 森川 正章
  • 特許第3120114号:新規微生物  
    森川正章, 金 沙
  • 特開平8-322597:核酸の増幅方法およびその試薬  1996年12月10日
    北林 雅夫, 荒川 琢, 井上 浩明, 川上 文清, 川村 良久, 今中 忠行, 高木 昌宏, 森川 正章
  • 特開平7-298879:超好熱始原菌由来のDNAポリメラーゼ遺伝子およびその用途  1995年11月14日
    今中 忠行, 高木 昌宏, 森川 正章, 柿原 博文
  • 特願平5-352901:シュードモナス属細菌を用いた炭化水素の生産方法及び新規シュードモナス属細菌  1993年12月29日
    今中 忠行, 森川 正章, 桜井 尚二
  • 特開平5-276933:新規微生物  1993年10月26日
    森川 正章
  • 特開平5-211876:バイオサーファクタントの濃縮方法  1993年08月24日
    桜井 尚二, 今中 忠行, 森川 正章
  • 特開平5-211892:バイオサーファクタント産生菌のスクリーニング方法及びバイオサーファクタントの活性測定方法  1993年08月24日
    桜井 尚二, 真鍋 洋平, 今中 忠行, 森川 正章
  • 特開平1-120286:改変ヒト・リゾチーム、それをコードする遺伝子及び改変ヒト・リゾチームの製造方法  1989年05月12日
    村木三智郎, 地神芳文, 田中秀明, 森川正章
  • 特願2015-130895:植物の生長を促進する方法、植物生長促進物質を製造する方法及びこれらに利用されるタンパク質  
    森川 正章
  • 特開昭62-263192:卵黄レシチンの製造方法  
    森川正章, 徳永恵美子, 堺宗雄

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