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检测和遗传分析日本河水中的人类杯状病毒。

Detection and genetic analysis of human sapoviruses in river water in Japan.

机构信息

Department of Urban Engineering, Graduate School of Engineering, The University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-8656, Japan.

出版信息

Appl Environ Microbiol. 2010 Apr;76(8):2461-7. doi: 10.1128/AEM.02739-09. Epub 2010 Feb 26.

Abstract

We investigated the prevalence of sapoviruses (SaVs) in the Tamagawa River in Japan from April 2003 to March 2004 and performed genetic analysis of the SaV genes identified in river water. A total of 60 river water samples were collected from five sites along the river, and 500 ml was concentrated using the cation-coated filter method. By use of a real-time reverse transcription (RT)-PCR assay, 12 (20%) of the 60 samples were positive for SaV. SaV sequences were obtained from 15 (25%) samples, and a total of 30 SaV strains were identified using six RT-PCR assays followed by cloning and sequence analysis. A newly developed nested RT-PCR assay utilizing a broadly reactive forward primer showed the highest detection efficiency and amplified more diverse SaV genomes in the samples. SaV sequences were frequently detected from November to March, whereas none were obtained in April, July, September, or October. No SaV sequences were detected in the upstream portion of the river, whereas the midstream portion showed high positive rates. Based on phylogenetic analysis, SaV strains identified in the river water samples were classified into nine genotypes, namely, GI/1, GI/2, GI/3, GI/5, GI/untyped, GII/1, GII/2, GII/3, and GV/1. To our knowledge, this is the first study describing seasonal and spatial distributions and genetic diversity of SaVs in river water. A combination of real-time RT-PCR assay and newly developed nested RT-PCR assay is useful for identifying and characterizing SaV strains in a water environment.

摘要

我们调查了日本玉川河从 2003 年 4 月到 2004 年 3 月的萨波病毒(SaV)流行情况,并对在河水中鉴定出的 SaV 基因进行了遗传分析。总共从河流的五个地点采集了 60 个河水样本,使用阳离子涂层滤器法浓缩 500ml。通过使用实时 RT-PCR 检测法,60 个样本中的 12 个(20%)为 SaV 阳性。从 15 个(25%)样本中获得了 SaV 序列,并通过六个 RT-PCR 检测法进行克隆和序列分析,共鉴定出 30 株 SaV 株。使用新开发的巢式 RT-PCR 检测法,利用广谱反应性的正向引物,显示出最高的检测效率,并在样本中扩增了更多不同的 SaV 基因组。SaV 序列经常从 11 月到 3 月被检测到,而 4 月、7 月、9 月或 10 月则没有。在河流的上游部分没有检测到 SaV 序列,而在中游部分则显示出较高的阳性率。基于系统进化分析,从河水样本中鉴定出的 SaV 株被分为九个基因型,即 GI/1、GI/2、GI/3、GI/5、GI/未分型、GII/1、GII/2、GII/3 和 GV/1。据我们所知,这是第一份描述河水中 SaV 的季节性和空间分布及遗传多样性的研究。实时 RT-PCR 检测法和新开发的巢式 RT-PCR 检测法的组合,对于鉴定和描述水环境中的 SaV 株是有用的。

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