首页> 美国卫生研究院文献>Journal of Bacteriology >Epoxyalkane:Coenzyme M Transferase in the Ethene and Vinyl Chloride Biodegradation Pathways of Mycobacterium Strain JS60
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Epoxyalkane:Coenzyme M Transferase in the Ethene and Vinyl Chloride Biodegradation Pathways of Mycobacterium Strain JS60

机译:分枝杆菌菌株JS60乙烯和氯乙烯生物降解途径中的环氧烷烃:辅酶M转移酶

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摘要

Mycobacterium strains that grow on ethene and vinyl chloride (VC) are widely distributed in the environment and are potentially useful for biocatalysis and bioremediation. The catabolic pathway of alkene assimilation in mycobacteria is not well characterized. It is clear that the initial step is a monooxygenase-mediated epoxidation that produces epoxyethane from ethene and chlorooxirane from VC, but the enzymes involved in subsequent transformation of the epoxides have not been identified. We investigated epoxyethane metabolism in Mycobacterium strain JS60 and discovered a coenzyme M (CoM)-dependent enzyme activity in extracts from VC- and ethene-grown cells. PCR amplifications using primers targeted at epoxyalkane:CoM transferase (EaCoMT) genes yielded part of the JS60 EaCoMT gene, which was used to clone an 8.4-kb genomic DNA fragment. The complete EaCoMT gene (etnE) was recovered, along with genes (etnABCD) encoding a four-component monooxygenase and two genes possibly involved in acyl-CoA ester metabolism. Reverse transcription-PCR indicated that the etnE and etnA genes were cotranscribed and inducible by ethene and VC. Heterologous expression of the etnE gene in Mycobacterium smegmatis mc2155 using the pMV261 vector gave a recombinant strain capable of transforming epoxyethane, epoxypropane, and chlorooxirane. A metabolite identified by mass spectrometry as 2-hydroxyethyl-CoM was produced from epoxyethane. The results indicate that the EaCoMT and monooxygenase enzymes encoded by a single operon (etnEABCD) catalyze the initial reactions in both the VC and ethene assimilation pathways. CoM-mediated reactions appear to be more widespread in bacteria than was previously believed.
机译:在乙烯和氯乙烯(VC)上生长的分枝杆菌菌株广泛分布在环境中,可能对生物催化和生物修复有用。分枝杆菌中烯烃同化的分解代谢途径尚不十分清楚。显然,第一步是单加氧酶介导的环氧化,其由乙烯产生环氧乙烷,由VC产生氯环氧乙烷,但尚未鉴定出与环氧化物后续转化有关的酶。我们调查了分枝杆菌菌株JS60中的环氧乙烷代谢,并发现了VC和乙烯生长的细胞提取物中的辅酶M(CoM)依赖性酶活性。使用针对环氧烷烃:CoM转移酶(EaCoMT)基因的引物进行的PCR扩增产生了JS60 EaCoMT基因的一部分,该基因被用于克隆8.4 KB的基因组DNA片段。恢复了完整的EaCoMT基因(etnE),以及编码四组分单加氧酶的基因(etnABCD)和两个可能参与酰基辅酶A酯代谢的基因。逆转录-PCR表明,etnE和etnA基因被乙烯和VC共转录并诱导。用pMV261载体在耻垢分枝杆菌mc 2 155中异源表达etnE基因,得到了能够转化环氧乙烷,环氧丙烷和氯代环氧乙烷的重组菌株。由环氧乙烷产生的代谢物经质谱鉴定为2-羟乙基-CoM。结果表明,单个操纵子(etnEABCD)编码的EaCoMT和单加氧酶催化VC和乙烯同化途径中的初始反应。 CoM介导的反应似乎比以前认为的更广泛地存在于细菌中。

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