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两种用于检测呼吸道病毒的分子方法的真实世界比较。

Real-world comparison of two molecular methods for detection of respiratory viruses.

机构信息

Department of Pediatrics, Vanderbilt University School of Medicine, 1161 21st Avenue South, Nashville, TN 37232, USA.

出版信息

Virol J. 2011 Jun 29;8:332. doi: 10.1186/1743-422X-8-332.

DOI:10.1186/1743-422X-8-332
PMID:21714915
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3154182/
Abstract

BACKGROUND

Molecular polymerase chain reaction (PCR) based assays are increasingly used to diagnose viral respiratory infections and conduct epidemiology studies. Molecular assays have generally been evaluated by comparing them to conventional direct fluorescent antibody (DFA) or viral culture techniques, with few published direct comparisons between molecular methods or between institutions. We sought to perform a real-world comparison of two molecular respiratory viral diagnostic methods between two experienced respiratory virus research laboratories.

METHODS

We tested nasal and throat swab specimens obtained from 225 infants with respiratory illness for 11 common respiratory viruses using both a multiplex assay (Respiratory MultiCode-PLx Assay [RMA]) and individual real-time RT-PCR (RT-rtPCR).

RESULTS

Both assays detected viruses in more than 70% of specimens, but there was discordance. The RMA assay detected significantly more human metapneumovirus (HMPV) and respiratory syncytial virus (RSV), while RT-rtPCR detected significantly more influenza A. We speculated that primer differences accounted for these discrepancies and redesigned the primers and probes for influenza A in the RMA assay, and for HMPV and RSV in the RT-rtPCR assay. The tests were then repeated and again compared. The new primers led to improved detection of HMPV and RSV by RT-rtPCR assay, but the RMA assay remained similar in terms of influenza detection.

CONCLUSIONS

Given the absence of a gold standard, clinical and research laboratories should regularly correlate the results of molecular assays with other PCR based assays, other laboratories, and with standard virologic methods to ensure consistency and accuracy.

摘要

背景

基于分子聚合酶链反应(PCR)的检测方法越来越多地用于诊断病毒性呼吸道感染并进行流行病学研究。分子检测方法通常通过与传统的直接荧光抗体(DFA)或病毒培养技术进行比较来进行评估,但是很少有关于分子方法之间或机构之间的直接比较的文献发表。我们试图在两个经验丰富的呼吸道病毒研究实验室之间对两种分子呼吸道病毒诊断方法进行真实世界的比较。

方法

我们使用多重检测法(Respiratory MultiCode-PLx 检测法[RMA])和单独的实时 RT-PCR(RT-rtPCR)对 225 例呼吸道疾病婴儿的鼻和咽拭子标本进行了 11 种常见呼吸道病毒的检测。

结果

两种检测方法均在超过 70%的标本中检测到了病毒,但存在不一致之处。RMA 检测法检测出人偏肺病毒(HMPV)和呼吸道合胞病毒(RSV)的比例明显更高,而 RT-rtPCR 检测到甲型流感的比例明显更高。我们推测引物差异是造成这些差异的原因,因此重新设计了 RMA 检测法中用于检测甲型流感的引物和探针,以及 RT-rtPCR 检测法中用于检测 HMPV 和 RSV 的引物和探针。然后再次进行了测试和比较。新的引物提高了 RT-rtPCR 检测法检测 HMPV 和 RSV 的能力,但 RMA 检测法在检测流感方面仍然相似。

结论

鉴于缺乏金标准,临床和研究实验室应定期将分子检测方法的结果与其他基于 PCR 的检测方法、其他实验室以及与标准病毒学方法进行比较,以确保一致性和准确性。

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Comparison of the Eragen Multi-Code Respiratory Virus Panel with conventional viral testing and real-time multiplex PCR assays for detection of respiratory viruses.比较 Eragen Multi-Code 呼吸道病毒检测试剂盒与常规病毒检测和实时多重 PCR 检测试剂盒在呼吸道病毒检测中的应用。
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