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Evaluation of integrated cell culture-PCR (C-PCR) for virological analysis of environmental samples

机译:评估用于环境样品病毒学分析的整合细胞培养-PCR(C-PCR)

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Aims: The aims of this study were to establish an integrated culture-polymerase chain reaction (C-PCR) method for detection of enteric viruses in environmental samples, and to evaluate it for sensitivity, speed and provision of virus infectivity data. Methods and Results: C-PCR, direct reverse transcription (RT)-PCR, PCR and plaque assay methods were used to detect enteroviruses and adenoviruses in seeded and naturally contaminated environmental samples. Using C-PCR, infectious enterovirus presence was confirmed in 3 d and adenovirus presence in 5 d, compared with up to 10 d required by conventional cell culture methods. Conclusions: C-PCR was the preferred method for detection of enteric viruses in environmental samples containing high viral concentrations. It was less successful for samples with low viral concentrations or containing toxic materials or inhibitors. Significance and Impact of the Study: C-PCR provides sensitive, specific results within 2-5 and is useful as a rapid screen for environmental samples of low toxicity.
机译:目的:本研究的目的是建立一种用于检测环境样品中肠道病毒的整合培养-聚合酶链反应(C-PCR)方法,并对其灵敏度,速度和提供的病毒感染性数据进行评估。方法和结果:使用C-PCR,直接逆转录(RT)-PCR,PCR和噬菌斑测定方法检测播种的和自然污染的环境样品中的肠病毒和腺病毒。与传统的细胞培养方法相比,使用C-PCR可以在3 d内确认到感染性肠病毒的存在,在5 d内确认到了腺病毒的存在。结论:C-PCR是检测高病毒浓度环境样品中肠病毒的首选方法。对于病毒浓度低或含有毒性物质或抑制剂的样品,这种方法不太成功。研究的意义和影响:C-PCR可在2-5内提供灵敏,特异的结果,可用于快速筛选低毒性的环境样品。

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