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应用脱脂乳凝块法和 PCR 技术检测和定量两种地理区域河水中的经典病毒和新兴病毒。

Detection and quantification of classic and emerging viruses by skimmed-milk flocculation and PCR in river water from two geographical areas.

机构信息

Department of Microbiology, Faculty of Biology, University of Barcelona, Av. Diagonal 643, Barcelona 08028, Spain.

出版信息

Water Res. 2013 May 15;47(8):2797-810. doi: 10.1016/j.watres.2013.02.043. Epub 2013 Mar 13.

Abstract

Molecular techniques and virus concentration methods have shown that previously unknown viruses are shed by humans and animals, and may be transmitted by sewage-contaminated water. In the present study, 10-L river-water samples from urban areas in Barcelona, Spain and Rio Janeiro, Brazil, have been analyzed to evaluate the viral dissemination of human viruses, validating also a low-cost concentration method for virus quantification in fresh water. Three viral groups were analyzed: (i) recently reported viruses, klassevirus (KV), asfarvirus-like virus (ASFLV), and the polyomaviruses Merkel cell (MCPyV), KI (KIPyV) and WU (WUPyV); (ii) the gastroenteritis agents noroviruses (NoV) and rotaviruses (RV); and (iii) the human fecal viral indicators in water, human adenoviruses (HAdV) and JC polyomaviruses (JCPyV). Virus detection was based on nested and quantitative PCR assays. For KV and ASFLV, nested PCR assays were developed for the present study. The method applied for virus concentration in fresh water samples is a one-step procedure based on a skimmed-milk flocculation procedure described previously for seawater. Using spiked river water samples, inter- and intra-laboratory assays showed a viral recovery rate of about 50% (20-95%) for HAdV, JCPyV, NoV and RV with a coefficient of variation ≤ 50%. HAdV and JCPyV were detected in 100% (12/12) of the river samples from Barcelona and Rio de Janeiro. Moreover, NoV GGII was detected in 83% (5/6) and MCPyV in 50% (3/6) of the samples from Barcelona, whereas none of the other viruses tested were detected. NoV GGII was detected in 33% (2/6), KV in 33% (2/6), ASFLV in 17% (1/6) and MCPyV in 50% (3/6) of the samples from Rio de Janeiro, whereas KIPyV and WUPyV were not detected. RV were only analyzed in Rio de Janeiro and resulted positive in 67% (4/6) of the samples. The procedure applied here to river water represents a useful, straightforward and cost-effective method that could be applied in routine water quality testing. The results of the assays expand our understanding of the global distribution of the viral pathogens studied here and their persistence in the environment.

摘要

分子技术和病毒浓缩方法表明,人类和动物会排出以前未知的病毒,这些病毒可能通过受污水污染的水传播。本研究分析了来自西班牙巴塞罗那和巴西里约热内卢城区的 10 升河水样本,以评估人类病毒的病毒传播情况,并验证一种用于淡水病毒定量的低成本浓缩方法。分析了三组病毒:(i) 最近报道的病毒,如 klassevirus(KV)、asfarvirus-like virus(ASFLV)和多瘤病毒 Merkel 细胞(MCPyV)、KI(KIPyV)和 WU(WUPyV);(ii) 胃肠炎病原体诺如病毒(NoV)和轮状病毒(RV);以及 (iii) 水中的人粪便病毒指标,如人腺病毒(HAdV)和 JC 多瘤病毒(JCPyV)。病毒检测基于巢式和定量 PCR 检测。对于 KV 和 ASFLV,本研究中开发了巢式 PCR 检测方法。用于淡水样品病毒浓缩的方法是一种基于脱脂奶絮凝程序的一步法,该程序先前已用于海水。使用加标河水样本,实验室间和实验室内部检测表明,HAdV、JCPyV、NoV 和 RV 的病毒回收率约为 50%(20-95%),变异系数≤50%。巴塞罗那和里约热内卢的 100%(12/12)河水样本中均检测到 HAdV 和 JCPyV。此外,在巴塞罗那的 6 个样本中,83%(5/6)检测到 NoV GGII,50%(3/6)检测到 MCPyV,而其他测试的病毒均未检测到。在里约热内卢的 6 个样本中,33%(2/6)检测到 NoV GGII,33%(2/6)检测到 KV,17%(1/6)检测到 ASFLV,50%(3/6)检测到 MCPyV,而 KIPyV 和 WUPyV 未检测到。RV 仅在里约热内卢进行了分析,结果 67%(4/6)的样本为阳性。这里应用于河水的方法是一种有用、直接且具有成本效益的方法,可用于常规水质检测。检测结果扩展了我们对全球分布的病毒病原体的了解,并了解了它们在环境中的持久性。

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