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16S rRNA 基因焦磷酸测序揭示生物固体中细菌病原体的多样性。

Pyrosequencing of the 16S rRNA gene to reveal bacterial pathogen diversity in biosolids.

机构信息

Department of Chemical Engineering, Environmental Engineering Program, Yale University, New Haven, CT 06520, USA.

出版信息

Water Res. 2010 Jul;44(14):4252-60. doi: 10.1016/j.watres.2010.05.039. Epub 2010 Jun 9.

DOI:10.1016/j.watres.2010.05.039
PMID:20566210
Abstract

Given the potential for a variety of bacterial pathogens to occur in variably stabilized sewage sludge (biosolids), an understanding of pathogen diversity and abundance is necessary for accurate assessment of infective risk when these products are land applied. 16S rDNA was PCR amplified from genomic DNA extracted from municipal wastewater residuals (mesophilic- and thermophilic-phased anaerobic digestion (MAD and TPAD), composting (COM)), and agricultural soil (SOIL), and these amplicons were sequenced using massively parallel pyrosequencing technology. Resulting libraries contained an average of 30,893 16S rDNA sequences per sample with an average length of 392 bases. FASTUNIFRAC-based comparisons of population phylogenetic distance demonstrated similarities between the populations of different treatment plants performing the same stabilization method (e.g. different MAD samples), and population differences among samples from different biosolids stabilization methods (COM, MAD, and TPAD). Based on a 0.03 Jukes-Cantor distance to 80 potential bacterial pathogens, all samples contained pathogens and enrichment ranged from 0.02% to 0.1% of sequences. Most (61%) species identified were opportunistic pathogens of the genera Clostridium and Mycobacterium. As risk sciences continue to evolve to address scenarios that include multiple pathogen exposure, the analysis described here can be used to determine the diversity of pathogens in an environmental sample. This work provides guidance for prioritizing subsequent culturable and quantitative analysis, and for the first time, ensuring that potentially significant pathogens are not left out of risk estimations.

摘要

鉴于各种细菌病原体在不同稳定化的污水污泥(生物固体)中可能存在,因此在这些产品施用于土地时,为了准确评估感染风险,有必要了解病原体的多样性和丰度。从城市废水残留物(中温-和高温相厌氧消化(MAD 和 TPAD)、堆肥(COM))和农业土壤(SOIL)中提取的基因组 DNA 中通过 PCR 扩增 16S rDNA,并使用大规模平行焦磷酸测序技术对这些扩增子进行测序。所得文库平均每个样品包含 30,893 个 16S rDNA 序列,平均长度为 392 个碱基。基于 FASTUNIFRAC 的种群系统发育距离比较表明,采用相同稳定化方法的不同处理厂的种群之间存在相似性(例如,不同的 MAD 样品),并且来自不同生物固体稳定化方法的样品之间的种群存在差异(COM、MAD 和 TPAD)。基于 0.03 Jukes-Cantor 距离到 80 种潜在细菌病原体,所有样品均包含病原体,富集度范围为序列的 0.02%至 0.1%。鉴定出的大多数(61%)物种是梭菌属和分枝杆菌属的机会性病原体。随着风险科学的不断发展,以应对包括多种病原体暴露的情况,这里描述的分析可用于确定环境样品中病原体的多样性。这项工作为后续可培养和定量分析提供了指导,并首次确保潜在重要的病原体不会被排除在风险估计之外。

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