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首页> 外文期刊>Journal of Clinical Microbiology >Enhanced Reverse Transcription-PCR Assay for Detection of Norovirus Genogroup I
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Enhanced Reverse Transcription-PCR Assay for Detection of Norovirus Genogroup I

机译:用于检测诺如病毒基因组I的增强逆转录PCR方法

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We have developed a one-tube reverse transcription (RT)-PCR method using the real-time TaqMan PCR system for the detection of norovirus genogroup I (NV GGI). By introduction of a novel probe based on locked nucleic acid technology, we enhanced the sensitivity of the assay compared to those of conventional TaqMan probes. The sensitivity of the NV GGI RT-PCR was determined by probit analysis with defined RNA standards and quantified norovirus isolates to 711 copies/ml (95% detection limit). In order to detect PCR inhibition, we included a heterologous internal control (IC) system based on phage MS2. This internally controlled RT-PCR was tested on different real-time PCR platforms, LightCycler, Rotorgene, Mastercycler EP realplex, and ABI Prism. Compared to the assay without an IC, the duplex RT-PCR exhibited no reduction in sensitivity in clinical samples. In combination with an established NV GGII real-time RT-PCR, we used the novel assay in a routine assay for diagnosis of clinical and food-borne norovirus infection. We applied this novel assay to analyze outbreaks of nonbacterial acute gastroenteritis. Norovirus of GGI was detected in these outbreaks. Sequence and similarity plot analysis of open reading frame 1 (ORF1) and ORF2 showed two genotypes, GGI/2 and GGI/4, in semiclosed communities.
机译:我们已经开发了一种使用实时TaqMan PCR系统的单管逆转录(RT)-PCR方法,用于检测诺如病毒基因组I(NV GGI)。通过引入基于锁定核酸技术的新型探针,与常规TaqMan探针相比,我们提高了测定的灵敏度。 NV GGI RT-PCR的敏感性是通过使用规定的RNA标准和定量诺如病毒分离株至711拷贝/ ml(检测限为95%)的概率分析来确定的。为了检测PCR抑制作用,我们包括了基于噬菌体MS2的异源内部对照(IC)系统。在不同的实时PCR平台,LightCycler,Rotorgene,Mastercycler EP realplex和ABI Prism上测试了这种内部控制的RT-PCR。与没有IC的测定相比,双工RT-PCR在临床样品中的敏感性没有降低。结合已建立的NV GGII实时RT-PCR,我们在常规检测中使用了该新型检测方法来诊断临床和食源性诺如病毒感染。我们应用了这种新颖的分析方法来分析非细菌性急性胃肠炎的爆发。在这些暴发中检测到GGI诺如病毒。开放阅读框1(ORF1)和ORF2的序列和相似性图分析显示了半封闭社区中的两种基因型,即GGI / 2和GGI / 4。

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