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首页> 外文期刊>Diseases of Aquatic Organisms >Detection and surveillance of viral hemorrhagic septicemia virus using real-time RT-PCR. I. Initial comparison of four protocols
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Detection and surveillance of viral hemorrhagic septicemia virus using real-time RT-PCR. I. Initial comparison of four protocols

机译:使用实时RT-PCR检测和监测病毒性出血性败血病病毒。一,四种协议的初步比较

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摘要

Eight laboratories worked collectively to evaluate 4 real-time RT-PCR (rRT-PCR) protocols targeting viral hemorrhagic septicemia virus (VHSV) being considered for deployment to a USA laboratory testing network. The protocols utilized previously published primers and probe sets developed for detection and surveillance of VHSV. All participating laboratories received and followed a standard operating protocol for extraction and for each of the rRT-PCR assays. Performance measures specifically evaluated included limit of detection (defined as the smallest amount of analyte in which 95% of the samples are classified as positive), analytical specificity, assay efficiency across genotype representatives, within- and between-plate variation within a laboratory, and variation between laboratories using the same platform, between platforms, and between software versions. This evaluation clearly demonstrated that the TaqMan (R)-based assay developed by Jonstrup et al. (2013; J Fish Dis 36: 9-23) produced the most consistent analytical performance characteristics for detecting all genotypes of VHSV across the 8 participating laboratories
机译:八个实验室共同努力,评估了针对病毒性败血性败血病病毒(VHSV)的4种实时RT-PCR(rRT-PCR)方案,这些方案正在考虑部署到美国实验室测试网络。该协议利用了先前发布的用于检测和监视VHSV的引物和探针组。所有参与的实验室均接受并遵循标准操作规程以进行提取和每种rRT-PCR测定。专门评估的性能指标包括检测限(定义为将95%的样品分类为阳性的最小分析物量),分析特异性,跨基因型代表的测定效率,实验室内板内和板间变异以及使用同一平台的实验室之间,平台之间以及软件版本之间的差异。该评估清楚地证明了Jonstrup等人开发的基于TaqMan(R)的检测方法。 (2013; J Fish Dis 36:9-23)产生了最一致的分析性能特征,可检测8个参与实验室的所有VHSV基因型

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