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检测和定量纤维素降解、发酵、硫酸盐还原细菌和产甲烷古菌的功能基因。

Detection and quantification of functional genes of cellulose- degrading, fermentative, and sulfate-reducing bacteria and methanogenic archaea.

机构信息

Laboratory of Microbiology and Infectious Diseases, Faculty of Veterinary Medicine, Aristotle University of Thessaloniki, 54124 Thessaloniki, Greece.

出版信息

Appl Environ Microbiol. 2010 Apr;76(7):2192-202. doi: 10.1128/AEM.01285-09. Epub 2010 Feb 5.

Abstract

Cellulose degradation, fermentation, sulfate reduction, and methanogenesis are microbial processes that coexist in a variety of natural and engineered anaerobic environments. Compared to the study of 16S rRNA genes, the study of the genes encoding the enzymes responsible for these phylogenetically diverse functions is advantageous because it provides direct functional information. However, no methods are available for the broad quantification of these genes from uncultured microbes characteristic of complex environments. In this study, consensus degenerate hybrid oligonucleotide primers were designed and validated to amplify both sequenced and unsequenced glycoside hydrolase genes of cellulose-degrading bacteria, hydA genes of fermentative bacteria, dsrA genes of sulfate-reducing bacteria, and mcrA genes of methanogenic archaea. Specificity was verified in silico and by cloning and sequencing of PCR products obtained from an environmental sample characterized by the target functions. The primer pairs were further adapted to quantitative PCR (Q-PCR), and the method was demonstrated on samples obtained from two sulfate-reducing bioreactors treating mine drainage, one lignocellulose based and the other ethanol fed. As expected, the Q-PCR analysis revealed that the lignocellulose-based bioreactor contained higher numbers of cellulose degraders, fermenters, and methanogens, while the ethanol-fed bioreactor was enriched in sulfate reducers. The suite of primers developed represents a significant advance over prior work, which, for the most part, has targeted only pure cultures or has suffered from low specificity. Furthermore, ensuring the suitability of the primers for Q-PCR provided broad quantitative access to genes that drive critical anaerobic catalytic processes.

摘要

纤维素降解、发酵、硫酸盐还原和产甲烷作用是微生物在各种自然和工程厌氧环境中共同存在的过程。与 16S rRNA 基因研究相比,研究负责这些具有不同系统发育功能的酶的基因具有优势,因为它提供了直接的功能信息。然而,目前还没有方法可以从复杂环境中具有特征的未培养微生物中广泛定量这些基因。在这项研究中,设计并验证了通用简并杂交寡核苷酸引物,以扩增纤维素降解菌的糖苷水解酶基因、发酵菌的 hydA 基因、硫酸盐还原菌的 dsrA 基因和产甲烷古菌的 mcrA 基因。通过计算机模拟和从具有目标功能的环境样本中获得的 PCR 产物的克隆和测序来验证特异性。进一步将引物对适应定量 PCR(Q-PCR),并在处理矿山排水的两个硫酸盐还原生物反应器的样本中进行了方法验证,一个基于木质纤维素,另一个以乙醇为食。正如预期的那样,Q-PCR 分析表明,基于木质纤维素的生物反应器含有更多的纤维素降解菌、发酵菌和产甲烷菌,而以乙醇为食的生物反应器则富含硫酸盐还原菌。开发的这套引物代表了一个重大进展,超过了之前的工作,之前的工作大部分只针对纯培养物,或者特异性较低。此外,确保引物适合 Q-PCR 为驱动关键厌氧催化过程的基因提供了广泛的定量方法。

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