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 >A SYBR green I–based quantitative RT-PCR assay for bovine ephemeral fever virus and its utility for evaluating viral kinetics in cattle
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A SYBR green I–based quantitative RT-PCR assay for bovine ephemeral fever virus and its utility for evaluating viral kinetics in cattle

机译:基于SYBR Green I的定量RT-PCR测定牛短暂发烧病毒及其用于评估牛病毒动力学的实用性

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摘要

We developed a SYBR green I–based reverse-transcription quantitative PCR (RT-qPCR) assay for bovine ephemeral fever virus (BEFV). Analytical sensitivity of the assay was ~ 100 times higher than conventional RT-PCR. The precision of the RT-qPCR established for RNA standards was high, with intra-assay and inter-assay coefficients of variation of 0.23–0.89% and 0.23–1.02%, respectively. The test was highly specific for BEFV strains, with no cross-reactivity with other viruses of veterinary significance. The assay detected BEFV RNA as early as 1 d post-infection (dpi) and up to 7–8 dpi in the blood samples of experimentally infected cattle. The most stable reference gene, peptidylprolyl isomerase A (PPIA), was selected for the quantification of BEFV. Viral RNA loads reached peak level at 3–5 dpi and then decreased rapidly through 7–8 dpi. Our assay provides a reliable approach for the detection of BEFV in the early infection stage and for use in the profiling of BEFV kinetics in vivo.
机译:我们开发了一个SYBR基于我的绿色逆转录定量PCR(RT-qPCR的),牛流行热病毒(BEFV)测定。该测定的分析灵敏度比常规RT-PCR更高〜100倍。所述RT-qPCR的精度建立了RNA的标准是高的,具有分别0.23-0.89%和0.23-1.02%,变异的测定内和测定间的系数。这次试验是为BEFV株高度特异性,与兽医意义的其他病毒无交叉反应。该分析检测到BEFV RNA早1 d感染后(DPI)和高达实验感染的牛血样中7-8 dpi的。最稳定的参考基因,异构酶A,被选择用于BEFV的定量肽基(PPIA)。病毒RNA负荷在3-5 DPI达高峰,然后经过7-8 DPI迅速下降。我们的测定提供了在早期感染阶段和用于体内BEFV动力学的轮廓使用检测BEFV的可靠的方法。

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