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Development of TaqMan-based qPCR method for detection of caprine arthritis–encephalitis virus (CAEV) infection

机译:基于TaqMan的qPCR方法开发用于检测鼠关节炎-脑炎病毒(CAEV)感染

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摘要

A specific and sensitive two-step TaqMan real-time PCR has been developed for rapid diagnosis of caprine arthritis-encephalitis virus (CAEV) infection by using a set of specific primers and a TaqMan probe targeting a highly conserved region within the gene encoding the viral capsid protein (CA). The assay successfully detected CAEV proviral DNA in total DNA extracts originating from cell culture, whole blood samples and isolated PBMCs, with a lower detection limit of 102 copies and a linear dynamic range of 105 to 1010 copies/ml. There was no cross-reaction with other animal viruses (e.g., goat pox virus, bovine leukemia virus, bovine mucosal disease virus, swine influenza virus and Nipah virus). When applied in parallel with serological AGID and conventional PCR for detection of CAEV in field samples, this assay exhibited a higher sensitivity than these traditional methods, and 7.8 % of the 308 specimens collected in the Shanxi and Tianjin regions of China from 1993 to 2011 were found to be positive. Thus, the TaqMan qPCR assay provides a fast, specific and sensitive means for detecting CAEV proviral DNA in goat specimens and should be useful for large-scale detection in eradication programs and epidemiological studies.
机译:通过使用一组特异性引物和靶向编码病毒基因的高度保守区域的TaqMan探针,开发了一种特异性和灵敏的两步TaqMan实时PCR,用于快速诊断山羊关节炎-脑炎病毒(CAEV)感染衣壳蛋白(CA)。该测定法成功检测了源自细胞培养物,全血样品和分离的PBMC的总DNA提取物中的CAEV前病毒DNA,检出限下限为10 2 拷贝,线性动态范围为10 5 到10 10 个/ ml。与其他动物病毒(例如,山羊痘病毒,牛白血病病毒,牛粘膜疾病病毒,猪流感病毒和尼帕病毒)没有交叉反应。当与血清AGID和常规PCR平行用于田间样品中CAEV的检测时,此测定法显示出比这些传统方法更高的灵敏度,1993年至2011年在中国山西和天津地区采集的308个标本中有7.8%为发现是积极的。因此,TaqMan qPCR测定法提供了一种快速,特异性和灵敏的方法来检测山羊标本中的CAEV前病毒DNA,对于在根除计划和流行病学研究中进行大规模检测应是有用的。

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