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第二轮美国 45 家兽医诊断实验室使用的 SARS-CoV2 分子检测方法的实验室间比较。

Second round of an interlaboratory comparison of SARS-CoV2 molecular detection assays used by 45 veterinary diagnostic laboratories in the United States.

机构信息

Division of Food Processing Science and Technology, U.S. Food and Drug Administration, Bedford Park, IL, USA.

出版信息

J Vet Diagn Invest. 2022 Sep;34(5):825-834. doi: 10.1177/10406387221115702. Epub 2022 Aug 18.

Abstract

The COVID-19 pandemic presents a continued public health challenge. Veterinary diagnostic laboratories in the United States use RT-rtPCR for animal testing, and many laboratories are certified for testing human samples; hence, ensuring that laboratories have sensitive and specific SARS-CoV2 testing methods is a critical component of the pandemic response. In 2020, the FDA Veterinary Laboratory Investigation and Response Network (Vet-LIRN) led an interlaboratory comparison (ILC1) to help laboratories evaluate their existing RT-rtPCR methods for detecting SARS-CoV2. All participating laboratories were able to detect the viral RNA spiked in buffer and PrimeStore molecular transport medium (MTM). With ILC2, Vet-LIRN extended ILC1 by evaluating analytical sensitivity and specificity of the methods used by participating laboratories to detect 3 SARS-CoV2 variants (B.1; B.1.1.7 [Alpha]; B.1.351 [Beta]) at various copy levels. We analyzed 57 sets of results from 45 laboratories qualitatively and quantitatively according to the principles of ISO 16140-2:2016. More than 95% of analysts detected the SARS-CoV2 RNA in MTM at ≥500 copies for all 3 variants. In addition, for nucleocapsid markers N1 and N2, 81% and 92% of the analysts detected ≤20 copies in the assays, respectively. The analytical specificity of the evaluated methods was >99%. Participating laboratories were able to assess their current method performance, identify possible limitations, and recognize method strengths as part of a continuous learning environment to support the critical need for the reliable diagnosis of COVID-19 in potentially infected animals and humans.

摘要

新冠疫情仍然是公共卫生领域的一大挑战。美国的兽医诊断实验室使用 RT-rtPCR 进行动物检测,许多实验室都获得了检测人类样本的认证;因此,确保实验室拥有灵敏且特异的 SARS-CoV2 检测方法是疫情应对的关键组成部分。2020 年,FDA 兽医实验室调查和响应网络(Vet-LIRN)主导了一项实验室间比较(ILC1),以帮助实验室评估其现有的用于检测 SARS-CoV2 的 RT-rtPCR 方法。所有参与实验室均能够检测到缓冲液和 PrimeStore 分子运输介质(MTM)中添加的病毒 RNA。在 ILC2 中,Vet-LIRN 通过评估参与实验室用于检测 3 种 SARS-CoV2 变异株(B.1;B.1.1.7 [Alpha];B.1.351 [Beta])的方法的分析灵敏度和特异性,扩展了 ILC1。我们根据 ISO 16140-2:2016 的原则,对来自 45 个实验室的 57 组结果进行了定性和定量分析。对于所有 3 种变异株,超过 95%的分析人员在 MTM 中检测到≥500 拷贝的 SARS-CoV2 RNA。此外,对于核衣壳标志物 N1 和 N2,81%和 92%的分析人员分别在检测中检测到≤20 拷贝。评估方法的分析特异性>99%。参与实验室能够评估其当前方法的性能,发现可能的局限性,并认识到方法的优势,这是一个持续学习环境的一部分,以支持对可能感染的动物和人类 COVID-19 进行可靠诊断的迫切需求。

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