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首页> 外文期刊>Journal of Clinical Microbiology >Evaluation of a Multiplexed PCR Assay for Detection of Respiratory Viral Pathogens in a Public Health Laboratory Setting
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Evaluation of a Multiplexed PCR Assay for Detection of Respiratory Viral Pathogens in a Public Health Laboratory Setting

机译:在公共卫生实验室环境中检测呼吸道病毒病原的多重PCR检测的评估

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There are numerous viral and bacterial causes of respiratory disease. To enable rapid and sensitive detection of even the most prevalent causes, there is a need for more-simplified testing systems that enable researchers and clinicians to perform multiplexed molecular diagnostics quickly and easily. To this end, a new multiplexed molecular test called the MultiCode-PLx respiratory virus panel (PLx-RVP) was developed and then implemented in a public health laboratory setting. A total of 687 respiratory samples were analyzed for the presence of 17 viruses that commonly cause respiratory disease. As a comparator, the samples were also tested using a standard testing algorithm that included the use of a real-time influenza virus A and B reverse transcription-PCR test and routine viral culture identification. The standard testing algorithm identified 503 (73%) samples as positive and 184 as negative. Analyzing the same 687 samples, the PLx-RVP assay detected one or more targets in 528 (77%) samples and found 159 samples negative for all targets. There were 25 discordant results between the two systems; 14 samples were positive for viruses not routinely tested for by the Wisconsin State Laboratory of Hygiene, and 13 of these were confirmed by real-time PCR. When the results of the standard testing algorithm were considered “true positives,” the PLx-RVP assay showed an overall sensitivity of 99% and an overall specificity of 87%. In total, the PLx-RVP assay detected an additional 40 viral infections, of which 11 were mixed infections.
机译:有许多病毒和细菌引起的呼吸道疾病。为了能够快速,灵敏地检测甚至最普遍的原因,需要更加简化的测试系统,使研究人员和临床医生能够快速,轻松地执行多重分子诊断。为此,开发了一种称为MultiCode-PLx呼吸道病毒小组(PLx-RVP)的新的多重分子测试,然后在公共卫生实验室中进行了测试。分析了总共687个呼吸道样本中是否存在17种通常引起呼吸道疾病的病毒。作为比较者,还使用标准测试算法对样品进行了测试,包括使用实时流感病毒A和B的逆转录PCR检测以及常规病毒培养鉴定。标准测试算法将503个(73%)样本识别为阳性,184个为阴性。分析了相同的687个样本,PLx-RVP分析检测到528个样本中有一个或多个目标(77%),发现所有目标均为159个阴性。两个系统之间有25个不一致的结果。威斯康星州卫生实验室没有常规检测的14份病毒呈阳性,其中13份通过实时PCR确认。当标准测试算法的结果被认为是“真实阳性”时,PLx-RVP分析显示出99%的整体灵敏度和87%的整体特异性。总共,PLx-RVP分析检测到另外40种病毒感染,其中11种是混合感染。

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