Alkali- and Halo-tolerant Catalase from Halomonas sp. SK1 : Overexpression in Escherichia coli, Purification, Characterization, and Genetic Modification
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概要
- 論文の詳細を見る
A catalase gene, ohktA, from an alkali- and halo-tolerant bacterium, Halomonas sp. SK1, on the pKK223-3, was expressed in the catalase-lacking Escherichia coli strain UM2. Highly purified catalase showing a single band on SDS-PAGE was obtained by two liquid chromatography steps on DEAE-Toyopear1 and Chelating-Sepharose Fast Flow. The enzyme, oHktA, shows high catalase activity with a pH optimum at 10, and the activity was stable in 4 M KC1. This enzyme is thermo-sensitive, showing a significant loss of activity within 5 minutes at 37 °C. To modify the stability of the catalase, the addition of domain II of the heat stable Mn catalase from Thermus thermophilus to the C-terminus was made. When coexpressed with a chaperone (PhFKBP29) gene product, peptidyl–prolyl cis–trans isomerase, from a thermophilic bacterium, a chimeric catalase was produced in the soluble fraction. The stability of this catalase in the range of 37°–45 °C was improved and it was stable for more than 1 h at 37 °C.
- 社団法人 日本農芸化学会の論文
- 2004-04-23
著者
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Maruyama Tadashi
Marine Biotechnology Institute Co. Ltd:(present Address) Japan Marine Science & Technology Cente
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Thuy Le
Department Of Biological And Chemical Engineering Faculty Of Engineering Gunma University
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Shinozawa Takao
Department Of Biological And Chemical Engineering Faculty Of Engineering Gunma University
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PHUCHAROEN Krisana
Department of Biological and Chemical Engineering, Faculty of Engineering, Gunma University
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IDENO Akira
Sekisui Chemical Co., Ltd., R&D Division Minase Institute
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Ideno Akira
Sekisui Chemical Co. Ltd. R&d Division Minase Institute
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Phucharoen Krisana
Department Of Biological And Chemical Engineering Faculty Of Engineering Gunma University
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Maruyama Tadashi
Marine Biotechnology Institute
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MARUYAMA Tadashi
Marine Biodiversity Research Program, Japan Agency for Marine-Earth Science and Technology (JAMSTEC)
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