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首页> 外文期刊>Journal of Medical Virology >Development and application of a one-step real-time RT-PCR using a minor-groove-binding probe for the detection of a novel bunyavirus in clinical specimens
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Development and application of a one-step real-time RT-PCR using a minor-groove-binding probe for the detection of a novel bunyavirus in clinical specimens

机译:使用次要槽结合探针的一步式实时RT-PCR的开发和应用,用于检测临床标本中的新型布尼亚病毒

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摘要

A highly sensitive one-step real-time RT-PCR method using a minor-groove-binding (MGB) probe was developed for detection and quantitation of severe febrile with thrombocytopenia syndrome virus (SFTSV). The assay could discriminate SFTSV infection from other related viral diseases in human with a minimum detection limit of 10 viral RNA copies/μl and was 1,000 times more sensitive than the conventional PCR. Strong linear correlations (r20.99) between the Ct values and viral RNA standards over a linear range were obtained. The coefficients of variation of intra- and inter-assay reproducibility were both less than 2%. The RT-PCR was also shown to be highly specific, as no positive signals were detected for other related viruses. Evaluation of this assay with serum samples from laboratory confirmed cases and healthy donors showed 100% clinical diagnostic sensitivity and over 99% specificity. Clinical application with samples from 287 patients admitted to the hospital with suspected SFTSV infection showed that 15% were infected by SFTSV. This assay was rapid, requiring just over 2hr, including the nucleic acid extraction step. J. Med. Virol. 85:370-377, 2013.
机译:开发了一种使用次要槽结合(MGB)探针的高灵敏度一步实时RT-PCR方法,用于检测和定量血小板减少症候群病毒(SFTSV)的严重发热。该检测方法可以将SFTSV感染与人类其他相关病毒疾病区分开,最低检测限为10个病毒RNA拷贝/μl,其灵敏度是常规PCR的1000倍。在线性范围内,Ct值与病毒RNA标准品之间具有很强的线性相关性(r2> 0.99)。批内和批间重复性的变异系数均小于2%。 RT-PCR还显示出高度特异性,因为未检测到其他相关病毒的阳性信号。用实验室确诊病例和健康捐献者的血清样品对该方法进行评估,结果显示100%的临床诊断敏感性和超过99%的特异性。临床应用的287​​例疑似SFTSV感染患者入院,表明15%的患者被SFTSV感染。该测定是快速的,仅需2小时以上,包括核酸提取步骤。 J. Med。病毒。 85:370-377,2013年。

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