McAnulla C, Woodall C A, McDonald I R, Studer A, Vuilleumier S, Leisinger T, Murrell J C
Department of Biological Sciences, University of Warwick, Coventry CV4 7AL, England.
Appl Environ Microbiol. 2001 Jan;67(1):307-16. doi: 10.1128/AEM.67.1.307-316.2001.
Hyphomicrobium chloromethanicum CM2(T), an aerobic methylotrophic member of the alpha 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 C(1) transfer pathway for carbon assimilation and CO(2) 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.
氯甲烷生丝微菌CM2(T)是变形菌纲α亚纲的一种需氧甲基营养菌,能够以氯甲烷作为唯一碳源和能源生长。氯甲烷生丝微菌拥有一个用于利用氯甲烷的可诱导酶系统,该系统中表达了两种多肽(67 kDa的CmuA和35 kDa的CmuB)。此前研究表明,cmuA、cmuB、cmuC和purU这四个基因对于氯甲烷甲基杆菌利用氯甲烷生长至关重要。cmuA和cmuB基因被用作探针来鉴定氯甲烷生丝微菌中的同源物。氯甲烷生丝微菌中的一个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)。氯甲烷生丝微菌的CmuA(67 kDa)与氯甲烷甲基杆菌的CmuA具有高度同源性,并且含有一个N端甲基转移酶结构域和一个C端类咕啉结合结构域。氯甲烷生丝微菌的CmuB与一类甲基转移蛋白以及氯甲烷甲基杆菌的CmuB甲基转移酶相关。氯甲烷生丝微菌的CmuC与氯甲烷甲基杆菌的CmuC具有同源性,是一种推定的甲基转移酶。folD编码亚甲基四氢叶酸环水解酶,其可能参与碳同化和二氧化碳产生的C(1)转移途径,而paaE编码一种推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,氯甲烷生丝微菌中的氯甲烷利用途径与氯甲烷甲基杆菌中依赖类咕啉的甲基转移系统相似。已开发出PCR引物,用于从新分离的氯甲烷利用菌和富集培养物中成功扩增cmuA基因。