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评估 16S rRNA 基因 V2 区的遗传标记,用于通过 qPCR 定量检测选定的拟杆菌目物种和人粪便废物。

Evaluation of genetic markers from the 16S rRNA gene V2 region for use in quantitative detection of selected Bacteroidales species and human fecal waste by qPCR.

机构信息

US Environmental Protection Agency, Office of Research and Development, National Exposure Research Laboratory, Cincinnati, OH 45268, USA.

出版信息

Syst Appl Microbiol. 2010 Oct;33(6):348-57. doi: 10.1016/j.syapm.2010.06.001. Epub 2010 Jul 24.

DOI:10.1016/j.syapm.2010.06.001
PMID:20655680
Abstract

Molecular methods for quantifying defined Bacteroidales species from the human gastrointestinal tract may have important clinical and environmental applications, ranging from diagnosis of infections to fecal source tracking in surface waters. In this study, sequences from the V2 region of the small subunit ribosomal RNA gene were targeted in the development of qPCR assays to quantify DNA from six Bacteroides and one Prevotella species. In silico and experimental analyses suggested that each of the assays was highly discriminatory in detecting DNA from the intended species. Analytical sensitivity, precision and ranges of quantification were demonstrated for each assay by coefficients of variation of less than 2% for cycle threshold measurements over a range from 10 to 4×10(4) target sequence copies. The assays were applied to assess the occurrence and relative abundance of their target sequences in feces from humans and five animal groups as well as in 14 sewage samples from 13 different treatment facilities. Sequences from each of the species were detected at high levels (>10(3)copies/ng total extracted DNA) in human wastes. Sequences were also detected by each assay in all sewage samples and, with exception of the Prevotella sequences, showed highly correlated (R(2)≥0.7) variations in concentrations between samples. In contrast, the occurrence and relative abundance profiles of these sequences differed substantially in the fecal samples from each of the animal groups. These results suggest that analyses for multiple individual Bacteroidales species may be useful in identifying human fecal pollution in environmental waters.

摘要

从人类胃肠道中定量鉴定特定拟杆菌种类的分子方法可能具有重要的临床和环境应用价值,从感染的诊断到地表水的粪便溯源都有涉及。在这项研究中,我们针对小亚基核糖体 RNA 基因 V2 区的序列,开发了用于定量检测六种拟杆菌和一种普雷沃氏菌属的 qPCR 检测方法。计算机和实验分析表明,每种检测方法都能高度特异性地检测到预期物种的 DNA。通过对 10 至 4×10(4)目标序列拷贝范围内的循环阈值测量进行了小于 2%的变异系数,证明了每种检测方法的分析灵敏度、精密度和定量范围。应用这些检测方法评估了这些目标序列在人类和五个动物群体粪便中的存在情况和相对丰度,以及 13 个不同处理设施的 14 个污水样本中的情况。在人类粪便中,所有物种的序列都以高水平(>10(3)拷贝/ng 总提取 DNA)检测到。每个检测方法也都在所有污水样本中检测到了这些序列,除了普雷沃氏菌序列外,在样本之间的浓度变化高度相关(R(2)≥0.7)。相比之下,这些序列在每个动物群体的粪便样本中的存在情况和相对丰度谱存在显著差异。这些结果表明,对多个特定拟杆菌种类的分析可能有助于识别环境水中的人类粪便污染。

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