首页> 美国卫生研究院文献>Applied and Environmental Microbiology >A Novel Reductive Dehalogenase, Identified in a Contaminated Groundwater Enrichment Culture and in Desulfitobacterium dichloroeliminans Strain DCA1, Is Linked to Dehalogenation of 1,2-Dichloroethane
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A Novel Reductive Dehalogenase, Identified in a Contaminated Groundwater Enrichment Culture and in Desulfitobacterium dichloroeliminans Strain DCA1, Is Linked to Dehalogenation of 1,2-Dichloroethane

机译:在污染的地下水富集培养中和在脱硫细菌dichloroeliminans菌株DCA1中鉴定出的新型还原性脱卤酶与1,2-二氯乙烷脱卤有关

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摘要

A mixed culture dechlorinating 1,2-dichloroethane (1,2-DCA) to ethene was enriched from groundwater that had been subjected to long-term contamination. In the metagenome of the enrichment, a 7-kb reductive dehalogenase (RD) gene cluster sequence was detected by inverse and direct PCR. The RD gene cluster had four open reading frames (ORF) showing 99% nucleotide identity with pceB, pceC, pceT, and orf1 of Dehalobacter restrictus strain DSMZ 9455T, a bacterium able to dechlorinate chlorinated ethenes. However, dcaA, the ORF encoding the catalytic subunit, showed only 94% nucleotide and 90% amino acid identity with pceA of strain DSMZ 9455T. Fifty-three percent of the amino acid differences were localized in two defined regions of the predicted protein. Exposure of the culture to 1,2-DCA and lactate increased the dcaA gene copy number by 2 log units, and under these conditions the dcaA and dcaB genes were actively transcribed. A very similar RD gene cluster with 98% identity in the dcaA gene sequence was identified in Desulfitobacterium dichloroeliminans strain DCA1, the only known isolate that selectively dechlorinates 1,2-DCA but not chlorinated ethenes. The dcaA gene of strain DCA1 possesses the same amino acid motifs as the new dcaA gene. Southern hybridization using total genomic DNA of strain DCA1 with dcaA gene-specific and dcaB- and pceB-targeting probes indicated the presence of two identical or highly similar dehalogenase gene clusters. In conclusion, these data suggest that the newly described RDs are specifically adapted to 1,2-DCA dechlorination.
机译:从长期受到污染的地下水中浓缩了将1,2-二氯乙烷(1,2-DCA)脱氯为乙烯的混合培养物。在富集的基因组中,通过反向和直接PCR检测到了一个7-kb的还原性脱卤素酶(RD)基因簇序列。 RD基因簇具有四个开放阅读框(ORF),它们与限制性脱盐杆菌DSMZ 9455 T 的pceB,pceC,pceT和orf1具有99%的核苷酸同一性,该细菌能够对氯化乙烯进行脱氯。但是,编码催化亚基的ORF dcaA与DSMZ 9455 T 菌株的pceA仅显示94%的核苷酸和90%的氨基酸同一性。 53%的氨基酸差异位于预测蛋白的两个定义区域中。将培养物暴露于1,2-DCA和乳酸盐会使dcaA基因的拷贝数增加了2个对数单位,在这些条件下,dcaA和dcaB基因被主动转录。在dcaA脱氯杆菌属DCA1菌株中鉴定出与dcaA基因序列具有98%相同性的非常相似的RD基因簇,这是唯一已知的选择性分离1,2-DCA而不是氯化乙烯的分离物。 DCA1菌株的dcaA基因具有与新dcaA基因相同的氨基酸基序。使用菌株DCA1的总基因组DNA与dcaA基因特异性探针以及dcaB和pceB靶向探针进行的Southern杂交表明存在两个相同或高度相似的脱卤酶基因簇。总之,这些数据表明,新描述的RD特别适用于1,2-DCA脱氯。

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