首页> 美国卫生研究院文献>Journal of Veterinary Diagnostic Investigation : Official Publication of the American Association of Veterinary Laboratory Diagnosticians Inc >Development and validation of direct PCR and quantitative PCR assaysfor the rapid sensitive and economical detection of porcine circovirus3
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Development and validation of direct PCR and quantitative PCR assaysfor the rapid sensitive and economical detection of porcine circovirus3

机译:直接PCR和定量PCR分析的开发和验证用于快速灵敏和经济地检测猪圆环病毒3

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摘要

Since the identification of species Porcine circovirus 2, the relevance of genus Circovirus has increased given its impact on the swine industry. A new species (Porcine circovirus 3, PCV-3) has been detected in association with various clinical conditions. Consequently, there is an urgent need for reliable and widely accessible tests for both routine diagnostic and research purposes. We developed a direct PCR (requiring no DNA extraction) and a quantitative (q)PCR targeting the conserved rep gene to detect the PCV-3 genome. Test performance was assessed by testing 120 field samples within different matrices. Both methods were sensitive (detection of 10 viral genome/µL), specific, and repeatable. The substantially perfect agreement between the 2 assays strongly supports their high sensitivity and specificity. The low cost and short processing time of the direct PCR protocol, together with the reliable quantitative results provided by qPCR, support the establishment of common testing guidelines.
机译:自从鉴定猪圆环病毒2以来,由于圆环病毒对猪产业的影响,圆环病毒属的相关性有所提高。与各种临床状况相关的新物种(猪圆环病毒3,PCV-3)已被发现。因此,迫切需要用于常规诊断和研究目的的可靠且可广泛使用的测试。我们开发了直接PCR(无需提取DNA)和靶向保守的rep基因的定量(q)PCR,以检测PCV-3基因组。通过在不同矩阵中测试120个现场样品来评估测试性能。两种方法均灵敏(检测10个病毒基因组/ µL),特异性且可重复。两种测定之间基本完全一致的协议有力地支持了它们的高灵敏度和特异性。直接PCR方案的低成本和短处理时间,以及qPCR提供的可靠定量结果,均支持建立通用的测试指南。

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