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A flexible format LAMP assay for rapid detection of Ebola virus

机译:一种柔性格式灯测定,用于快速检测埃博拉病毒

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BackgroundThe unprecedented 2013/16 outbreak of Zaire ebolavirus (Ebola virus) in West Africa has highighted the need for rapid, high-throughput and POC diagnostic assays to enable timely detection and appropriate triaging of Ebola Virus Disease (EVD) patients. Ebola virus is highly infectious and prompt diagnosis and triage is crucial in preventing further spread within community and healthcare settings. Moreover, due to the ecology of Ebola virus it is important that newly developed diagnostic assays are suitable for use in both the healthcare environment and low resource rural locations.Methodology/principle findingsA LAMP assay was successfully developed with three detection formats; a real-time intercalating dye-based assay, a real-time probe-based assay to enable multiplexing and an end-point colourimetric assay to simplify interpretation for the field. All assay formats were sensitive and specific, detecting a range of Ebola virus strains isolated in 1976-2014; with Probit analysis predicting limits of detection of 243, 290 and 75 copies/reaction respectively and no cross-detection of related strains or other viral haemorrhagic fevers (VHF's). The assays are rapid, (as fast as 5-7.25 mins for real-time formats) and robust, detecting Ebola virus RNA in presence of minimally diluted bodily fluids. Moreover, when tested on patient samples from the 2013/16 outbreak, there were no false positives and 93-96% of all new case positives were detected, with only a failure to detect very low copy number samples.Conclusion/significanceThese are a set of robust and adaptable diagnostic solutions, which are fast, easy-to-perform-and-interpret and are suitable for use on a range of platforms including portable low-power devices. They can be readily transferred to field-laboratory settings, with no specific equipment needs and are therefore ideally placed for use in locations with limited resources.
机译:背景技术西非的Zaire Ebolavirus(埃博拉病毒)爆发了Zaire Ebolavirus(埃博拉病毒)的爆发已经过分了解快速,高通量和PoC诊断测定,以实现埃博拉病毒疾病(EVD)患者的及时检测和适当的三环。埃博拉病毒是高度传染性的,迅速的诊断和分类对于预防社区和医疗保健环境的进一步蔓延至关重要。此外,由于埃博拉病毒的生态,重要的是新开发的诊断测定适用于医疗保健环境和低资源农村地区。方法/原理发现灯测定用三种检测格式成功开发;基于实时嵌入染料的测定,是基于实时探针的测定,以实现复用和终点Colouremetric测定以简化该领域的解释。所有测定形式均敏感,特异性,检测一系列埃博拉病毒菌株于1976 - 2014年孤立;探测分析分析分别检测的限制,分别检测243,290和75份/反应,并且没有相关菌株或其他病毒出血性FEVERS(VHF)的交叉检测。该测定迅速,(用于实时格式的5-7.25分钟)和稳健,检测埃博拉病毒RNA在最小稀释的体液存在下。此外,当在2013/16爆发的患者样品上测试时,没有误报,并且检测到所有新案例呈阳性的93-96%,只有未能检测到非常低的拷贝数样本。结论/有效是一个集合强大且可适应的诊断解决方案,这是快速,易于执行的和解释的,并且适用于包括便携式低功耗器件的一系列平台。它们可以容易地转移到现场实验室设置,没有特定的设备需求,因此理想地放置在资源有限的位置。

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