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在以四氯乙烯、三氯乙烯或2,3-二氯苯酚为底物生长的脱卤球菌属菌株195中还原脱卤酶基因的表达。

Expression of reductive dehalogenase genes in Dehalococcoides ethenogenes strain 195 growing on tetrachloroethene, trichloroethene, or 2,3-dichlorophenol.

作者信息

Fung Jennifer M, Morris Robert M, Adrian Lorenz, Zinder Stephen H

机构信息

Department of Microbiology, Cornell University, Ithaca, NY 14840, USA.

出版信息

Appl Environ Microbiol. 2007 Jul;73(14):4439-45. doi: 10.1128/AEM.00215-07. Epub 2007 May 18.

DOI:10.1128/AEM.00215-07
PMID:17513589
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1932842/
Abstract

Reductive dehalogenase (RD) gene transcript levels in Dehalococcoides ethenogenes strain 195 were investigated using reverse transcriptase quantitative PCR during growth and reductive dechlorination of tetrachloroethene (PCE), trichloroethene (TCE), or 2,3-dichlorophenol (2,3-DCP). Cells grown with PCE or TCE had high transcript levels (greater than that for rpoB) for tceA, which encodes the TCE RD, pceA, which encodes the PCE RD, and DET0162, which contains a predicted stop codon and is considered nonfunctional. In cells grown with 2,3-DCP, tceA mRNA was less than 1% of that for rpoB, indicating that its transcription was regulated. pceA and DET0162 were the only RD genes with high transcript levels in cells grown with 2,3-DCP. Proteomic analysis of PCE-grown cells detected both PceA and TceA with high peptide coverage but not DET0162, and analysis of 2,3-DCP-grown cells detected PceA with high coverage but not TceA, DET0162, or any other potential RD. Cells grown with PCE or 2,3-DCP were tested for the ability to dechlorinate PCE, TCE, or 2,3-DCP with H2 as the electron donor. 2,3-DCP-grown cells were unable to dechlorinate TCE but dechlorinated PCE to TCE without a lag, and PCE-grown cells dechlorinated 2,3-DCP without a lag. These results show that 2,3-DCP-grown cells do not produce TceA and that DET0162 is transcribed but its translation product is not detectable in cells and are consistent with PceA's being bifunctional, also serving as the 2,3-DCP RD. Chlorophenols naturally occur in soils and are good candidates for the original substrates for PceA.

摘要

利用逆转录定量PCR技术,研究了嗜氯乙烯脱卤球菌195菌株在四氯乙烯(PCE)、三氯乙烯(TCE)或2,3 -二氯苯酚(2,3 - DCP)生长及还原脱氯过程中还原脱卤酶(RD)基因的转录水平。以PCE或TCE生长的细胞中,编码TCE RD的tceA、编码PCE RD的pceA以及含有预测终止密码子且被认为无功能的DET0162的转录水平较高(高于rpoB)。在以2,3 - DCP生长的细胞中,tceA mRNA不到rpoB的1%,表明其转录受到调控。pceA和DET0162是在以2,3 - DCP生长的细胞中仅有的转录水平较高的RD基因。对以PCE生长的细胞进行蛋白质组分析,检测到PceA和TceA的肽段覆盖率较高,但未检测到DET0162;对以2,3 - DCP生长的细胞进行分析,检测到PceA的覆盖率较高,但未检测到TceA、DET0162或任何其他潜在的RD。测试了以PCE或2,3 - DCP生长的细胞以H2作为电子供体对PCE、TCE或2,3 - DCP进行脱氯的能力。以2,3 - DCP生长的细胞无法使TCE脱氯,但能将PCE无延迟地脱氯为TCE,而以PCE生长的细胞能无延迟地使2,3 - DCP脱氯。这些结果表明,以2,3 - DCP生长的细胞不产生TceA,且DET0162被转录但其翻译产物在细胞中无法检测到,这与PceA具有双功能、也作为2,3 - DCP RD的情况一致。氯酚天然存在于土壤中,是PceA原始底物的良好候选物。

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