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检测和 S1 基因分型传染性支气管炎病毒和临床样本中其他密切相关的γ冠状病毒的 RT-PCR 检测方法的建立和验证。

Development and validation of RT-PCR tests for the detection and S1 genotyping of infectious bronchitis virus and other closely related gammacoronaviruses within clinical samples.

机构信息

Veterinary Laboratories Agency, Weybridge, New Haw, Addlestone, Surrey, UK.

出版信息

Transbound Emerg Dis. 2011 Oct;58(5):411-20. doi: 10.1111/j.1865-1682.2011.01222.x. Epub 2011 Apr 7.

Abstract

Two tests were developed that allow the detection and genotyping of infectious bronchitis virus (IBV) and other closely related gammacoronaviruses. The first test employs a one-step, reverse transcription-polymerase chain reaction (RT-PCR) assay in which the amplification is monitored in real time using a TaqMan(®) probe. This real-time RT-PCR test was used to examine a panel of field samples and its performance compared to virus isolation in embryonated fowls' eggs. A total of 323 field samples were tested; 176 samples were positive using the real-time RT-PCR method, but only three were positive by virus isolation. Sequencing was used to confirm the positive real-time RT-PCR results for a subset of samples. The test is suitable for swabs and post-mortem samples and has been shown to be highly sensitive and specific. The second test, a genotyping method, was developed for identification of the strain of IBV present in field samples based on nucleotide variations within the gene encoding the S1 subunit of the surface spike (S) glycoprotein. This method was developed to provide a tool to inform vaccination decisions and for ongoing surveillance to detect new and emerging strains of IBV within the UK. The performance of the test was evaluated using laboratory isolates of IBV and field samples. Both tests are suitable for use in a high-throughput diagnostic laboratory.

摘要

两种检测方法可用于检测传染性支气管炎病毒(IBV)和其他密切相关的γ冠状病毒,并对其进行基因分型。第一种检测方法采用一步法反转录聚合酶链反应(RT-PCR),使用 TaqMan(®)探针实时监测扩增情况。本实时 RT-PCR 检测方法用于检测一组现场样本,并将其与鸡胚病毒分离检测的性能进行了比较。共检测了 323 个现场样本;实时 RT-PCR 方法检测到 176 个样本为阳性,但只有 3 个样本通过病毒分离法检测到为阳性。对部分样本的实时 RT-PCR 阳性结果进行了测序验证。该检测法适用于拭子和尸检样本,具有高灵敏度和特异性。第二种检测方法是一种基因分型方法,用于根据 S1 糖蛋白表面刺突(S)亚单位编码基因内的核苷酸变异,鉴定现场样本中 IBV 的毒株。该方法的开发是为了提供一种工具,用于通知疫苗接种决策,并进行持续监测,以检测英国境内新出现的 IBV 毒株。该方法使用 IBV 实验室分离株和现场样本进行了性能评估。两种检测方法都适用于高通量诊断实验室。

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