An end-point multiplex RT-PCR for SARS-CoV-2, Influenza A and B detection, including simultaneous RNAse P amplification: a timely tool for more accessible differential diagnosis.

Thaísa Regina Rocha Lopes, José Valter Joaquim Silva Júnior, Priscila de Arruda Trindade, Tatiana Schäffer Gregianini, Rudi Weiblen, Eduardo Furtado Flores
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Abstract

The multiplex molecular diagnostic assays described for severe acute respiratory syndrome-related coronavirus 2 (SARS-CoV-2), influenza A (IAV) and B (IBV) viruses have been mainly based on real-time reaction, which limits their access to many laboratories or diagnostic institutions. To contribute to available strategies and expand access to differential diagnosis, we describe an end-point multiplex RT-PCR targeting SARS-CoV-2, IAV and IBV with simultaneous endogenous control amplification. Initially, we looked for well-established primers sets for SARS-CoV-2, IAV, IBV and RNAse P whose amplicons could be distinguished on agarose gel. The multiplex assay was then standardized by optimizing the reaction mix and cycle conditions. The limit of detection (LoD) was determined using titrated viruses (for SARS-CoV-2 and IAV) and by dilution from a pool of IBV-positive samples. The diagnostic performance of the multiplex was evaluated by testing samples with different RNAse P and viral loads, previously identified as positive or negative for the target viruses. The amplicons of IAV (146 bp), SARS-CoV-2 (113 bp), IBV (103 bp) and RNAse P (65 bp) were adequately distinguished in our multiplex. The LoD for SARS-CoV-2, IAV and IBV was 0.02 TCID50/ml, 0.07 TCID50/ml and 10-3 from a pool of positive samples, respectively. All samples positive for SARS-CoV-2 (n=70, Ct 17.2-36.9), IAV (n=53, Ct 14-34.9) and IBV (n=12, Ct 23.9-31.9) remained positive in our multiplex assay. RNAse P from negative samples (n=40, Ct 25.2-30.2) was also amplified in the multiplex. Overall, our assay is a timely and alternative tool for detecting SARS-CoV-2 and influenza viruses in laboratories with limited access to supplies/equipment.

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用于检测 SARS-CoV-2、甲型流感和乙型流感的端点多重 RT-PCR(包括同时进行 RNAse P 扩增):更便于鉴别诊断的及时工具。
针对严重急性呼吸系统综合征相关冠状病毒 2(SARS-CoV-2)、甲型流感病毒(IAV)和乙型流感病毒(IBV)的多重分子诊断方法主要基于实时反应,这限制了许多实验室或诊断机构的使用。为了丰富现有的策略并扩大鉴别诊断的范围,我们介绍了一种针对 SARS-CoV-2、IAV 和 IBV 的端点多重 RT-PCR,并同时进行内源性对照扩增。最初,我们针对 SARS-CoV-2、IAV、IBV 和 RNAse P 寻找可在琼脂糖凝胶上分辨出扩增子的成熟引物集。然后,通过优化反应混合物和循环条件,对多重检测进行了标准化。检测限(LoD)是通过滴定病毒(SARS-CoV-2 和 IAV)和稀释 IBV 阳性样本池确定的。通过检测不同 RNAse P 和病毒载量的样本,评估了多重检测的诊断性能。我们的多重分析仪能充分区分 IAV(146 bp)、SARS-CoV-2(113 bp)、IBV(103 bp)和 RNAse P(65 bp)的扩增子。SARS-CoV-2、IAV 和 IBV 的 LoD 分别为 0.02 TCID50/ml、0.07 TCID50/ml 和 10-3。所有对 SARS-CoV-2(n=70,Ct 17.2-36.9)、IAV(n=53,Ct 14-34.9)和 IBV(n=12,Ct 23.9-31.9)呈阳性的样本在多重检测中都保持阳性。阴性样本(n=40,Ct 25.2-30.2)中的 RNAse P 也能在多重检测中扩增。总之,我们的检测方法是在供应/设备有限的实验室检测 SARS-CoV-2 和流感病毒的一种及时的替代工具。
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