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Chloromethane-Induced Genes Define a Third C1 Utilization Pathway in Methylobacterium chloromethanicum CM4

机译:氯甲烷诱导的基因在甲基甲基细菌甲基氯甲烷CM4中定义了第三种C1利用途径

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摘要

Methylobacterium chloromethanicum CM4 is an aerobic α-proteobacterium capable of growth with chloromethane as the sole carbon and energy source. Two proteins, CmuA and CmuB, were previously purified and shown to catalyze the dehalogenation of chloromethane and the vitamin B12-mediated transfer of the methyl group of chloromethane to tetrahydrofolate. Three genes located near cmuA and cmuB, designated metF, folD and purU and encoding homologs of methylene tetrahydrofolate (methylene-H4folate) reductase, methylene-H4folate dehydrogenase-methenyl-H4folate cyclohydrolase and formyl-H4folate hydrolase, respectively, suggested the existence of a chloromethane-specific oxidation pathway from methyl-tetrahydrofolate to formate in strain CM4. Hybridization and PCR analysis indicated that these genes were absent in Methylobacterium extorquens AM1, which is unable to grow with chloromethane. Studies with transcriptional xylE fusions demonstrated the chloromethane-dependent expression of these genes. Transcriptional start sites were mapped by primer extension and allowed to define three transcriptional units, each likely comprising several genes, that were specifically expressed during growth of strain CM4 with chloromethane. The DNA sequences of the deduced promoters display a high degree of sequence conservation but differ from the Methylobacterium promoters described thus far. As shown previously for purU, inactivation of the metF gene resulted in a CM4 mutant unable to grow with chloromethane. Methylene-H4folate reductase activity was detected in a cell extract of strain CM4 only in the presence of chloromethane but not in the metF mutant. Taken together, these data provide evidence that M. chloromethanicum CM4 requires a specific set of tetrahydrofolate-dependent enzymes for growth with chloromethane.
机译:甲基甲烷氯甲烷苯丙酸杆菌CM4是一种需氧的α-变形杆菌,能够以氯甲烷为唯一碳和能源生长。预先纯化了两种蛋白质CmuA和CmuB,它们显示出催化氯甲烷的脱卤作用和维生素B12介导的氯甲烷甲基向四氢叶酸转移的能力。位于cmuA和cmuB附近的三个基因分别命名为metF,folD和purU,分别编码四氢叶酸亚甲基(亚甲基-H4叶酸)还原酶,亚甲基-H4叶酸脱氢酶-亚甲基-H4叶酸环化酶和甲酰-H4叶酸水解酶的同源物。菌株CM4中从四氢叶酸甲酯到甲酸的特异性氧化途径。杂交和PCR分析表明,这些基因在甲基芽胞杆菌AM1中不存在,而后者不能与氯甲烷一起生长。转录xylE融合的研究证明了这些基因的氯甲烷依赖性表达。转录起始位点通过引物延伸进行定位,并允许定义三个转录单元,每个转录单元可能包含数个基因,它们在含氯甲烷的CM4菌株生长过程中特异性表达。推导的启动子的DNA序列显示出高度的序列保守性,但是与迄今为止描述的甲基杆菌启动子不同。如先前对于purU所示,灭活metF基因导致CM4突变体无法与氯甲烷一起生长。仅在存在氯甲烷的情况下,才在菌株CM4的细胞提取物中检测到亚甲基H4叶酸还原酶活性,而在metF突变体中未检测到。综上所述,这些数据提供了证据,证明氯甲烷单胞菌CM4需要一组特定的四氢叶酸依赖性酶才能与氯甲烷一起生长。

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