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针对 Dehalococcoides mccartyi 微生物蛋白生物标志物的检测,作为受污染地下水中还原脱氯活性的指示物。

Targeted detection of Dehalococcoides mccartyi microbial protein biomarkers as indicators of reductive dechlorination activity in contaminated groundwater.

机构信息

Chemical Sciences Division, Oak Ridge National Laboratory, Oak Ridge, Tennessee, 37831, United States.

Department of Genome Science and Technology, University of Tennessee, Knoxville, Tennessee, 37996, United States.

出版信息

Sci Rep. 2019 Jul 22;9(1):10604. doi: 10.1038/s41598-019-46901-6.

Abstract

Dehalococcoides mccartyi (Dhc) bacterial strains expressing active reductive dehalogenase (RDase) enzymes play key roles in the transformation and detoxification of chlorinated pollutants, including chlorinated ethenes. Site monitoring regimes traditionally rely on qPCR to assess the presence of Dhc biomarker genes; however, this technique alone cannot directly inform about dechlorination activity. To supplement gene-centric approaches and provide a more reliable proxy for dechlorination activity, we sought to demonstrate a targeted proteomics approach that can characterize Dhc mediated dechlorination in groundwater contaminated with chlorinated ethenes. Targeted peptide selection was conducted in axenic cultures of Dhc strains 195, FL2, and BAV1. These experiments yielded 37 peptides from housekeeping and structural proteins (i.e., GroEL, EF-TU, rpL7/L2 and the S-layer), as well as proteins involved in the reductive dechlorination activity (i.e., FdhA, TceA, and BvcA). The application of targeted proteomics to a defined bacterial consortium and contaminated groundwater samples resulted in the detection of FdhA peptides, which revealed active dechlorination with Dhc strain-level resolution, and the detection of RDases peptides indicating specific reductive dechlorination steps. The results presented here show that targeted proteomics can be applied to groundwater samples and provide protein level information about Dhc dechlorination activity.

摘要

表达活性还原脱卤酶 (RDase) 酶的 Dehalococcoides mccartyi (Dhc) 细菌菌株在转化和解毒氯化污染物方面发挥着关键作用,包括氯化烯烃。传统的现场监测方案依赖于 qPCR 来评估 Dhc 生物标志物基因的存在;然而,仅靠这项技术无法直接了解脱卤活性。为了补充基于基因的方法,并提供更可靠的脱卤活性替代物,我们试图展示一种靶向蛋白质组学方法,该方法可以表征受污染地下水的氯化烯烃污染的 Dhc 介导的脱卤作用。在 Dhc 菌株 195、FL2 和 BAV1 的无菌培养物中进行了靶向肽选择。这些实验从管家和结构蛋白(即 GroEL、EF-TU、rpL7/L2 和 S-层)以及参与还原脱卤活性的蛋白质(即 FdhA、TceA 和 BvcA)中产生了 37 个肽。靶向蛋白质组学在定义明确的细菌联合体和受污染地下水样本中的应用导致了 FdhA 肽的检测,这揭示了 Dhc 菌株水平分辨率下的活性脱卤作用,以及 RDases 肽的检测表明了特定的还原脱卤步骤。这里呈现的结果表明,靶向蛋白质组学可以应用于地下水样本,并提供 Dhc 脱卤活性的蛋白质水平信息。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f382/6646388/85ffad5c0977/41598_2019_46901_Fig1_HTML.jpg

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