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Detection of Organohalide-Respiring Enzyme Biomarkers at a Bioaugmented TCE-Contaminated Field Site

机译:检测生物化TCE污染场地的有机卤代物 - 呼吸酶生物标志物

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摘要

RNA-based biomarkers have been successfully detected at field sites undergoing in situ bioremediation, but the detection of expressed enzymes is a more direct way to prove activity for a particular biocatalytic process of interest since they provide evidence of potential in situ activity rather than simply confirming presence and abundance of genes in a given population by measurement of DNA copies using qPCR. Here we successfully applied shotgun proteomics to field samples from a trichloroethene (TCE)-contaminated industrial site in southern Ontario, Canada that had been bio-augmented with the commercially available KB-1TM microbial culture. The KB-1TM culture contains multiple strains of Dehalococcoides mccartyi (D. mccartyi) as well as an organohalide respiring Geobacter species. The relative abundances of specific enzymatic proteins were subsequently compared to corresponding qPCR-derived levels of DNA and RNA biomarkers in the same samples. Samples were obtained from two wells with high hydraulic connectivity to the KB-1TM-bioaugemented enhanced in situ bioremediation system, and two control wells that showed evidence of low levels of native organohalide respiring bacteria (OHRB), Dehalococcoides and Geobacter. Enzymes involved in organohalide respiration were detected in the metaproteomes of all four field samples, as were chaperonins of D. mccartyi, chemotaxis proteins, and ATPases. The most highly expressed RDase in the bioaugmentation culture (VcrA) was the most highly detected enzyme overall in the bioaugmented groundwater samples. In one background groundwater well, we found high expression of the Geobacter pceA RDase. The DNA and RNA biomarkers detected using qPCR-based assays were a set of orthologs of Dehalococcoides reductive dehalogenases (VcrA, TceA, BvcA, dehalogenase “DET1545”), and the Ni-Fe uptake hydrogenase, HupL. Within a sample, RNA levels for key enzymes correlated with relative protein abundance. These results indicate that laboratory observations of TCE-bioremediation biomarker protein expression are recapitulated in field environmental systems and that both RNA and protein biomarker monitoring hold promise for activity monitoring of in situ populations of OHRB.
机译:已经在发生原位生物修复的现场网站上成功地检测到基于RNA的生物标志物,但是表达酶的检测是一种更直接的方法,以证明特定的生物催化过程的活动,因为它们提供了原位活动的潜力证据而不是简单地确认通过使用QPCR测量DNA拷贝的给定群体中的基因存在和丰度。在这里,我们将霰弹枪蛋白质组学应用于加拿大南安大略省南部的三氯乙烯(TCE)的田间样本,该工业遗址已与市售的KB-1TM微生物培养有生物增强。 KB-1TM培养物含有多种脱卤素菌株McCartyi(D. mccartyi)以及有机卤化物呼吸的地形杆菌物种。随后将特异性酶促蛋白的相对丰度与相同样品中的DNA和RNA生物标志物的相应QPCR衍生水平进行比较。从两种孔中获得样品,其具有高液压连通性的液体连接,其kB-1Tm-BioSumperated in原位生物化系统,以及两种对照孔,显示出低水平的天然有机卤化物呼吸细菌(OHRB),脱卤素和地杆菌的证据。在所有四个田间样品的标准胶质体中检测到有机卤化物呼吸中参与有机卤化物呼吸的酶,如D.McCartyi,趋化性蛋白质和ATP酶的伴侣蛋白。生物沉积培养物(VCRA)中最高表达的RDase是生物化地下水样品中总体检测到的酶。在一个背景下的地下水中,我们发现高表达PPEA RDase的高表达。使用基于QPCR的测定检测到的DNA和RNA生物标志物是一组脱卤素还原脱氢酶(VCRA,TCEA,BVCA,脱卤素“DET1545”)和Ni-Fe摄取氢酶,Hupl。在样品中,与相对蛋白质丰度相关的关键酶的RNA水平。这些结果表明,TCE-生物标病生物标志物蛋白表达的实验室观察在现场环境系统中综合地综合,并且RNA和蛋白质生物标志物监测持有人类群体的活动监测的承诺。

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