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Characterization of membrane-bound dehydrogenases of Gluconobacter oxydans 621H using a new system for their functional expression

机译:用新系统对其功能表达使用新系统表征葡聚糖氧化物621h的膜结合脱氢酶

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摘要

Acetic acid bacteria are used in biotechnology due to their ability to incompletely oxidize a great variety of carbohydrates, alcohols, and related compounds in a regio- and stereo-selective manner. These reactions are catalyzed by membrane-bound dehydrogenases (mDHs), often with a broad substrate spectrum. In this study, the promoters of six mDHs of Gluconobacter oxydans 621H were characterized. The constitutive promoter of the alcohol dehydrogenase and the glucose-repressed promoter of the inositol dehydrogenase were used to construct a shuttle vector system for the fully functional expression of mDHs in the multi-deletion strain G. oxydans BP.9 that lacks its mDHs. This system was used to express each mDH of G. oxydans 621H, in order to individually characterize the substrates, they oxidize. From 55 tested compounds, the alcohol dehydrogenase oxidized 30 substrates and the polyol dehydrogenase 25. The substrate spectrum of alcohol dehydrogenase overlapped largely with the aldehyde dehydrogenase and partially with polyol dehydrogenase. Thus, we were able to resolve the overlapping substrate spectra of the main mDHs of G. oxydans 621H. The described approach could also be used for the expression and detailed characterization of substrates used by mDHs from other acetic acid bacteria or a metagenome.
机译:乙酸细菌在生物技术中使用,因为它们的能力不完全氧化各种各样的碳水化合物,醇和相关化合物,并且立体选择性方式。这些反应通过膜结合的脱氢酶(MDH)催化,通常具有宽的基质光谱。在这项研究中,表征了621h的六MDHs的葡萄糖杆菌的启动子。醇脱氢酶的组成型启动子和肌醇脱氢酶的葡萄糖 - 抑制促进剂用于构建用于在缺乏其MDH的多缺失菌株G.0中的MDHS的全功能表达的梭载体系统。该系统用于表达G. oxydans 621h的每个MDH,以单独表征基材,它们氧化。从55个测试的化合物中,醇脱氢酶氧化30个底物和多元醇脱氢酶25.醇脱氢酶的基材光谱很大程度上与醛脱氢酶相似,部分用多元醇脱氢酶。因此,我们能够解析621h的G. oxydans主MDH的重叠基材光谱。所描述的方法还可用于来自其他乙酸细菌或梅塔蛋白的MDHS使用的底物的表达和详细表征。

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