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在南非东开普省由B.1.351变体引发的疫情中对PanBio快速SARS-CoV-2抗原检测法进行现场性能评估。

Field performance evaluation of the PanBio rapid SARS-CoV-2 antigen assay in an epidemic driven by the B.1.351 variant in the Eastern Cape, South Africa.

作者信息

Akingba Oluwakemi Laguda, Sprong Kaitlin, Marais Gert, Hardie Diana Ruth

机构信息

National Health Laboratory Service, South Africa.

Department of Laboratory Medicine and Pathology, Faculty of Health Sciences, Walter Sisulu University, Mthatha, South Africa.

出版信息

J Clin Virol Plus. 2021 Jun;1(1):100013. doi: 10.1016/j.jcvp.2021.100013. Epub 2021 Apr 7.

Abstract

BACKGROUND

South Africa was the African country with the most recorded cases of SARS-CoV-2 during 2020, experiencing 2 waves of infection. During the first wave, diagnostics were largely based on reverse transcription-linked PCR (RT-PCR). The Abbott PanBio antigen test was deployed during the 2nd wave which may have been driven by emergence of the B.1.351 variant. At the time of evaluation in mid-November 2020, B.1.351 was the dominant circulating virus in Nelson Mandela Bay, in the Eastern Cape Province.

METHODS

Used PanBio antigen swabs (collected from patients with genetically characterised virus) were first validated as suitable for PCR. A prospective study was then undertaken to evaluate assay performance in the field. Testing was conducted at mobile community testing centres on 677 ambulant patients. Used swabs were kept and tested by RT-PCR.

RESULTS

During initial validation, used swabs in proprietary lysis buffer were found to be suitable for PCR and secondly, the PB assay reliably detected patients infected with B.1.351. In the field study, of 146 RT-PCR positive individuals, 101 were RTD positive in the clinic. The RTD had a sensitivity of 69.2% (95%CI 61.4, 75.8) and specificity of 99.0% (95%CI 98.8, 99.3). Sensitivity was dependent on the amount of viral RNA in clinical samples, as reflected by the PCR cycle threshold (CT) value.

CONCLUSIONS

The assay reliably detected B.1.351 infections in ambulatory ill patients during initial validation and in field testing. In the field, assay sensitivity was >90% in patients with high viral loads who are expected to be most infectious. Negative and positive predictive values were also >90%.

摘要

背景

南非是2020年有记录的严重急性呼吸综合征冠状病毒2(SARS-CoV-2)病例最多的非洲国家,经历了两波感染。在第一波疫情期间,诊断主要基于逆转录聚合酶链反应(RT-PCR)。在第二波疫情期间部署了雅培PanBio抗原检测,这可能是由B.1.351变体的出现所驱动。在2020年11月中旬进行评估时,B.1.351是东开普省纳尔逊·曼德拉湾主要的流行病毒。

方法

首先验证了使用过的PanBio抗原拭子(从病毒基因特征已明确的患者中采集)适用于PCR。然后进行了一项前瞻性研究以评估该检测方法在实际应用中的性能。在流动社区检测中心对677名门诊患者进行了检测。保留使用过的拭子并通过RT-PCR进行检测。

结果

在初始验证期间,发现保存在专用裂解缓冲液中的使用过的拭子适用于PCR,其次,PB检测能够可靠地检测出感染B.1.351的患者。在现场研究中,146名RT-PCR检测呈阳性的个体中,有101名在诊所的快速检测(RTD)中呈阳性。RTD的灵敏度为69.2%(95%置信区间61.4, 75.8),特异性为99.0%(95%置信区间98.8, 99.3)。灵敏度取决于临床样本中病毒RNA的量,这由PCR循环阈值(CT)值反映。

结论

在初始验证和现场检测中,该检测方法能够可靠地检测出门诊患病患者中的B.1.351感染。在现场,对于预计传染性最强的高病毒载量患者,检测灵敏度>90%。阴性和阳性预测值也>90%。

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