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Chloromethane Utilization Gene Cluster from Hyphomicrobium chloromethanicum Strain CM2T and Development of Functional Gene Probes To Detect Halomethane-Degrading Bacteria

机译:拟南芥次生细菌CM2T的氯甲烷利用基因簇及检测卤甲烷降解细菌的功能基因探针的开发

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摘要

Hyphomicrobium chloromethanicum CM2T, an aerobic methylotrophic member of the α subclass of the class proteobacteria, can grow with chloromethane as the sole carbon and energy source. H. chloromethanicum possesses an inducible enzyme system for utilization of chloromethane, in which two polypeptides (67-kDa CmuA and 35-kDa CmuB) are expressed. Previously, four genes, cmuA, cmuB, cmuC, and purU, were shown to be essential for growth of Methylobacterium chloromethanicum on chloromethane. The cmuA and cmuB genes were used as probes to identify homologs in H. chloromethanicum. A cmu gene cluster (9.5 kb) in H. chloromethanicum contained 10 open reading frames: folD (partial), pduX, orf153, orf207, orf225, cmuB, cmuC, cmuA, fmdB, and paaE (partial). CmuA from H. chloromethanicum (67 kDa) showed high identity to CmuA from M. chloromethanicum and contains an N-terminal methyltransferase domain and a C-terminal corrinoid-binding domain. CmuB from H. chloromethanicum is related to a family of methyl transfer proteins and to the CmuB methyltransferase from M. chloromethanicum. CmuC from H. chloromethanicum shows identity to CmuC from M. chloromethanicum and is a putative methyltransferase. folD codes for a methylene-tetrahydrofolate cyclohydrolase, which may be involved in the C1 transfer pathway for carbon assimilation and CO2 production, and paaE codes for a putative redox active protein. Molecular analyses and some preliminary biochemical data indicated that the chloromethane utilization pathway in H. chloromethanicum is similar to the corrinoid-dependent methyl transfer system in M. chloromethanicum. PCR primers were developed for successful amplification of cmuA genes from newly isolated chloromethane utilizers and enrichment cultures.
机译:变形细菌类α亚类的好氧甲基营养菌chloromethanicum CM2T可以以氯甲烷作为唯一碳和能源来生长。氯甲基苯丙酸杆菌具有利用氯甲烷的诱导酶系统,其中表达了两个多肽(67-kDa CmuA和35-kDa CmuB)。以前,四个基因cmuA,cmuB,cmuC和purU被证明对氯甲烷苯甲基甲烷杆菌在氯甲烷上的生长至关重要。使用cmuA和cmuB基因作为探针来鉴定氯甲基苯丙酸杆菌中的同源物。氯甲基苯丙酸杆菌中的一个cmu基因簇(9.5 kb)包含10个开放阅读框:folD(部分),pduX,orf153,orf207,orf225,cmuB,cmuC,cmuA,fmdB和paaE(部分)。来自H. chloromethanicum(67 kDa)的CmuA与来自M. chloromethanicum的CmuA具有高度同一性,并包含一个N端甲基转移酶结构域和一个C端类固醇结合域。来自氯甲基苯丙酸杆菌的CmuB与甲基转移蛋白家族有关,并且与来自氯甲基苯丙酸杆菌的CmuB甲基转移酶有关。来自氯甲烷苯丙酸杆菌的CmuC与来自氯甲烷苯丙酸甲烷的CmuC显示相同,并且是推定的甲基转移酶。 folD编码亚甲基四氢叶酸环化酶,可能参与碳同化和CO2产生的C1传递途径,而paaE编码假定的氧化还原活性蛋白。分子分析和一些初步的生化数据表明,H。chloromethanicum中氯甲烷的利用途径类似于M. chloromethanicum中依赖于类雌激素的甲基转移系统。开发了PCR引物,可从新分离的氯甲烷利用者和富集培养物中成功扩增cmuA基因。

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