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利用等温重组酶辅助扩增快速检测埃博拉病毒。

Rapid detection of Ebolavirus using isothermal recombinase-aided amplification.

机构信息

Institute of Animal Hygiene and Veterinary Public Health, Leipzig University, Leipzig, Germany.

Virology Department, Institut Pasteur de Dakar, Dakar, Senegal.

出版信息

J Med Virol. 2024 Jun;96(6):e29744. doi: 10.1002/jmv.29744.

Abstract

Ebolavirus disease (EVD) is an often-lethal disease caused by the genus Ebolavirus (EBOV). Although vaccines are being developed and recently used, outbreak control still relies on a combination of various factors, including rapid identification of EVD cases. This allows rapid patient isolation and control measure implementation. Ebolavirus diagnosis is performed in treatment centers or reference laboratories, which usually takes a few hours to days to confirm the outbreak or deliver a clear result. A fast and field-deployable molecular detection method, such as the isothermal amplification recombinase-aided amplification (RAA), could significantly reduce sample-to-result time. In this study, a RT-RAA assay was evaluated for EBOV detection. Various primer and probe combinations were screened; analytical sensitivity and cross-specificity were tested. A total of 40 archived samples from the 2014 to 2016 Ebola outbreak in West Africa were tested with both the reference method real-time RT-PCR and the established RT-RAA assay. The assay could detect down to 22.6 molecular copies per microliter. No other pathogens were detected with the Ebolavirus RT-RAA assay. Testing 40 samples yield clinical sensitivity and specificity of 100% each. This rapid isothermal RT-RAA assay can replace the previous RT-RPA and continue to offer rapid EBOV diagnostics.

摘要

埃博拉病毒病(EVD)是一种由埃博拉病毒属(EBOV)引起的常致命疾病。虽然正在开发和最近使用疫苗,但疫情控制仍然依赖于多种因素的结合,包括快速识别 EVD 病例。这可以实现快速的患者隔离和控制措施的实施。埃博拉病毒的诊断是在治疗中心或参考实验室进行的,通常需要几个小时到几天的时间才能确认疫情爆发或得出明确的结果。一种快速且可在现场部署的分子检测方法,如等温扩增重组酶辅助扩增(RAA),可以显著缩短样本到结果的时间。在这项研究中,评估了 RT-RAA 检测方法对 EBOV 的检测。筛选了各种引物和探针组合,测试了分析灵敏度和交叉特异性。总共检测了来自 2014 年至 2016 年西非埃博拉疫情的 40 个存档样本,分别用参考方法实时 RT-PCR 和建立的 RT-RAA 检测方法进行检测。该检测方法可以检测到 22.6 个分子拷贝/微升。Ebolavirus RT-RAA 检测方法未检测到其他病原体。检测 40 个样本的临床灵敏度和特异性均为 100%。这种快速的等温 RT-RAA 检测方法可以替代之前的 RT-RPA,并继续提供快速的 EBOV 诊断。

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