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比较病毒运输介质热失活对患者样本中 SARS-CoV-2 后续检测的影响。

Comparative effects of viral-transport-medium heat inactivation upon downstream SARS-CoV-2 detection in patient samples.

机构信息

Division of Cancer and Stem Cells, Biodiscovery Institute, School of Medicine, University of Nottingham, Nottingham, NG7 2RD, UK.

School of Pharmacy, University of Nottingham, Nottingham, NG7 2RD, UK.

出版信息

J Med Microbiol. 2021 Mar;70(3). doi: 10.1099/jmm.0.001301. Epub 2021 Mar 18.

Abstract

The COVID-19 pandemic, which began in 2020 is testing economic resilience and surge capacity of healthcare providers worldwide. At the time of writing, positive detection of the SARS-CoV-2 virus remains the only method for diagnosing COVID-19 infection. Rapid upscaling of national SARS-CoV-2 genome testing presented challenges: (1) Unpredictable supply chains of reagents and kits for virus inactivation, RNA extraction and PCR-detection of viral genomes. (2) Rapid time to result of <24 h is required in order to facilitate timely infection control measures. Extraction-free sample processing would impact commercially available SARS-CoV-2 genome detection methods. We evaluated whether alternative commercially available kits provided sensitivity and accuracy of SARS-CoV-2 genome detection comparable to those used by regional National Healthcare Services (NHS). We tested several detection methods and tested whether detection was altered by heat inactivation, an approach for rapid one-step viral inactivation and RNA extraction without chemicals or kits. Using purified RNA, we found the CerTest VIASURE kit to be comparable to the Altona RealStar system currently in use, and further showed that both diagnostic kits performed similarly in the BioRad CFX96 and Roche LightCycler 480 II machines. Additionally, both kits were comparable to a third alternative using a combination of Quantabio qScript one-step Quantitative Reverse Transcription Polymerase Chain Reaction (qRT-PCR) mix and Centre for Disease Control and Prevention (CDC)-accredited N1 and N2 primer/probes when looking specifically at borderline samples. Importantly, when using the kits in an extraction-free protocol, following heat inactivation, we saw differing results, with the combined Quantabio-CDC assay showing superior accuracy and sensitivity. In particular, detection using the CDC N2 probe following the extraction-free protocol was highly correlated to results generated with the same probe following RNA extraction and reported clinically (=127; R=0.9259). Our results demonstrate that sample treatment can greatly affect the downstream performance of SARS-CoV-2 diagnostic kits, with varying impact depending on the kit. We also showed that one-step heat-inactivation methods could reduce time from swab receipt to outcome of test result. Combined, these findings present alternatives to the protocols in use and can serve to alleviate any arising supply-chain issues at different points in the workflow, whilst accelerating testing, and reducing cost and environmental impact.

摘要

自 2020 年开始的 COVID-19 大流行正在考验全球医疗保健提供者的经济弹性和应对能力。在撰写本文时,检测到 SARS-CoV-2 病毒仍然是诊断 COVID-19 感染的唯一方法。快速扩大国家 SARS-CoV-2 基因组检测面临挑战:(1)病毒失活、RNA 提取和 PCR 检测病毒基因组的试剂和试剂盒的不可预测供应链。(2)需要在<24 小时内获得快速结果,以便及时采取感染控制措施。无提取的样本处理会影响现有的 SARS-CoV-2 基因组检测方法。我们评估了替代的商业上可用的试剂盒是否提供了与区域国家医疗保健服务(NHS)使用的试剂盒相当的 SARS-CoV-2 基因组检测的敏感性和准确性。我们测试了几种检测方法,并测试了热失活是否会改变检测,热失活是一种快速一步病毒失活和 RNA 提取的方法,无需使用化学物质或试剂盒。使用纯化的 RNA,我们发现 CerTest VIASURE 试剂盒与目前使用的 Altona RealStar 系统相当,并且进一步表明,这两种诊断试剂盒在 BioRad CFX96 和 Roche LightCycler 480 II 仪器上的性能相似。此外,当专门查看边界样本时,当使用试剂盒进行无提取的方案时,使用结合了 Quantabio qScript 一步定量逆转录聚合酶链反应(qRT-PCR)混合物和疾病控制与预防中心(CDC)认证的 N1 和 N2 引物/探针的第三种替代方法时,两种试剂盒都具有可比性。重要的是,当使用无提取方案中的试剂盒时,我们看到热失活后结果不同,结合使用 Quantabio-CDC 检测试剂盒显示出更高的准确性和敏感性。特别是,无提取方案中使用 CDC N2 探针进行检测与使用相同探针进行 RNA 提取并报告临床检测结果(=127;R=0.9259)高度相关。我们的结果表明,样本处理会极大地影响 SARS-CoV-2 诊断试剂盒的下游性能,不同试剂盒的影响也不同。我们还表明,一步热失活方法可以减少从拭子收到到获得检测结果的时间。综合来看,这些发现为正在使用的方案提供了替代方案,并可以缓解工作流程中不同点出现的任何供应问题,同时加快检测速度,降低成本和环境影响。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/675b/8346722/88a9384cf9ed/jmm-70-301-g001.jpg

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