Sensitive SARS-CoV-2 detection, air travel Covid-19 testing, variant determination and fast direct PCR detection, using ddPCR and RT-qPCR methods.

IF 1.1 4区 医学 Q4 VIROLOGY Acta virologica Pub Date : 2023-01-01 DOI:10.4149/av_2023_101
Tatiana Burjanivova, Eva Lukacova, Vincent Lucansky, Marek Samec, Petar Podlesniy, Zuzana Kolkova, Lenka Reizigova, Marian Grendar, Eva Turyova, Veronika Holubekova, Bibiana Malicherova, Vladimir Nosal, Ivana Kasubova, Robert Dusenka, Denisa Osinova, Jana Hosalova Matisova, Dana Dvorska, Dusan Brany, Zuzana Dankova, Elena Novakova, Andrea Calkovska, Erika Halasova
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引用次数: 2

Abstract

Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) monitoring in air traffic is important in the prevention of the virus spreading from abroad. The gold standard for SARS-CoV-2 detection is RT-qPCR; however, for early and low viral load detection, a much more sensitive method, such as droplet digital PCR (ddPCR), is required. Our first step was to developed both, ddPCR and RT-qPCR methods, for sensitive SARS-CoV-2 detection. Analysis of ten swab/saliva samples of five Covid-19 patients in different stages of disease showed positivity in 6/10 samples with RT-qPCR and 9/10 with ddPCR. We also used our RT-qPCR method for SARS-CoV-2 detection without the need of RNA extraction, obtaining results in 90-120 minutes. We analyzed 116 self-collected saliva samples from passengers and airport staff arriving from abroad. All samples were negative by RT-qPCR, while 1 was positive, using ddPCR. Lastly, we developed ddPCR assays for SARS-CoV-2 variants identification (alpha, beta, gamma, delta/kappa) that are more economically advantageous when compared to NGS. Our findings demonstrated that saliva samples can be stored at ambient temperature, as we did not observe any significant difference between a fresh sample and the same sample after 24 hours (p = 0.23), hence, saliva collection is the optimal route for sampling airplane passengers. Our results also showed that droplet digital PCR is a more suitable method for detecting virus from saliva, compared to RT-qPCR. Keywords: COVID-19; RT-PCR; ddPCR; SARS-CoV-2; nasopharyngeal swab; saliva.

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采用ddPCR和RT-qPCR方法对SARS-CoV-2进行灵敏检测、航空旅行Covid-19检测、变异检测和快速直接PCR检测。
在空中交通中监测严重急性呼吸综合征冠状病毒2 (SARS-CoV-2)对预防该病毒从国外传播具有重要意义。检测SARS-CoV-2的金标准是RT-qPCR;然而,对于早期和低病毒载量检测,需要一种更灵敏的方法,如液滴数字PCR (ddPCR)。我们的第一步是开发ddPCR和RT-qPCR方法,用于灵敏的SARS-CoV-2检测。对5例不同病程患者的10份拭子/唾液样本进行RT-qPCR和ddPCR分析,分别有6/10和9/10样本呈阳性。我们也使用我们的RT-qPCR方法检测SARS-CoV-2,不需要提取RNA,在90-120分钟内得到结果。我们分析了116份来自国外旅客和机场工作人员的唾液样本。RT-qPCR结果均为阴性,ddPCR结果为阳性1例。最后,我们开发了用于SARS-CoV-2变异鉴定(α、β、γ、δ /kappa)的ddPCR检测方法,与NGS相比,这些方法在经济上更具优势。我们的研究结果表明,唾液样本可以在室温下保存,因为我们没有观察到新鲜样本与相同样本在24小时后的显著差异(p = 0.23),因此,唾液采集是对飞机乘客进行采样的最佳途径。结果还表明,与RT-qPCR相比,液滴数字PCR是一种更适合检测唾液病毒的方法。关键词:COVID-19;rt - pcr;ddPCR;SARS-CoV-2;鼻咽拭子;唾液。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Acta virologica
Acta virologica 医学-病毒学
CiteScore
3.10
自引率
11.80%
发文量
43
审稿时长
>12 weeks
期刊介绍: Acta virologica is an international journal of predominantly molecular and cellular virology. Acta virologica aims to publish papers reporting original results of fundamental and applied research mainly on human, animal and plant viruses at cellular and molecular level. As a matter of tradition, also rickettsiae are included. Areas of interest are virus structure and morphology, molecular biology of virus-cell interactions, molecular genetics of viruses, pathogenesis of viral diseases, viral immunology, vaccines, antiviral drugs and viral diagnostics.
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