使用单管、反转录、半嵌套多酶等温快速扩增和侧流浸量测定法快速灵敏地检测基孔肯雅病毒。

IF 6.1 2区医学 Q1 MICROBIOLOGY

Journal of Clinical Microbiology Pub Date : 2024-09-11 Epub Date: 2024-08-14 DOI:10.1128/jcm.00383-24

Xinlin Wu, Gaowen Liu, Yingchao Chang, Mengyuan Zheng, Li Liu, Xueshan Xia, Yue Feng

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引用次数: 0

摘要

基孔肯雅热是由伊蚊传播的基孔肯雅病毒（CHIKV）引起的一种急性传染病。简单、快速、灵敏地检测 CHIKV 对预防和传播该疾病至关重要。为了解决这个问题，我们结合了单管反转录半嵌套、多酶等温快速扩增和侧向流沾条检测法来检测 CHIKV RNA。该研究使用 CHIKV NSP4 的 318-bp 基因片段作为检测目标。这种扩增方法在 39°C 下进行两步扩增，需要 30 分钟。将扩增产物的稀释液加入 LFD 条带，10 分钟后肉眼即可看到结果。该方法检测 CHIKV RNA 的灵敏度为 1 拷贝/μL，比传统的反转录多酶等温快速扩增法高出 100 倍，比反转录定量 PCR（RT-qPCR）法高出 10 倍。此外，在临床确诊的患者血浆样本中，该方法表现出良好的特异性，检出率（85.7%，21 例中的 18 例）高于 RT-qPCR（80.9%，21 例中的 17 例）。因此，本研究开发的 CHIKV RNA 快速检测方法将成为快速准确筛查基孔肯雅热患者的重要工具：本研究提出了一种新的单管、反转录半嵌套、多酶等温快速扩增检测法，并结合侧流测芯条用于检测 CHIKV。该技术大大提高了灵敏度，在检测 CHIKV 方面优于 RT-qPCR，尤其是在病毒载量较低的样本中。它的检测速度也明显快于传统的 RT-qPCR，而且不需要特殊设备或标准的 PCR 实验室。本研究开发的等温扩增技术与床旁分子检测相结合，为快速、现场、低成本的 CHIKV 分子诊断提供了可能。

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Rapid and sensitive detection of chikungunya virus using one-tube, reverse transcription, semi-nested multi-enzyme isothermal rapid amplification, and lateral flow dipstick assays.

Chikungunya fever is an acute infectious disease caused by chikungunya virus (CHIKV), which is transmitted by Aedes mosquitoes. Simple, rapid, and sensitive detection of CHIKV is critical for its prevention and spread. To address this issue, we combined one-tube, reverse transcription semi-nested, multi-enzyme isothermal rapid amplification, and lateral flow dipstick strips assay to detect CHIKV RNA. The study used a 318-bp gene fragment of CHIKV NSP4 as the target of the assay. This method of amplification takes 30 min for two-step amplification at 39°C. The dilution of amplification products was added to the LFD strip with results visible to the naked eye after 10 min. The method has a sensitivity of 1 copy/μL for the detection of CHIKV RNA, which is 100-fold higher than the conventional reverse transcription-multi-enzyme isothermal rapid amplification and 10-fold higher than the reverse transcription quantitative PCR (RT-qPCR) method. In addition, the method demonstrated good specificity and a better detection rate (85.7%, 18 of 21) than RT-qPCR (80.9%, 17 of 21) in clinically confirmed patient plasma samples. Thus, the rapid CHIKV RNA assay developed in this study will be an important tool for the rapid and accurate screening of patients for chikungunya fever.

Importance: This study presents a new one-tube, reverse transcription semi-nested, multi-enzyme isothermal rapid amplification assay combined with lateral flow dipstick strips for the detection of CHIKV. This technique significantly improves sensitivity and outperforms RT-qPCR for the detection of CHIKV, especially in samples with low viral loads. It is also significantly faster than conventional RT-qPCR and does not require special equipment or a standard PCR laboratory. The combination of the isothermal amplification technology developed in this study with point-of-care molecular testing offers the potential for rapid, on-site, low-cost molecular diagnosis of CHIKV.

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来源期刊

Journal of Clinical Microbiology 医学-微生物学

CiteScore

17.10

自引率

4.30%

发文量

347

审稿时长

3 months

期刊介绍： The Journal of Clinical Microbiology® disseminates the latest research concerning the laboratory diagnosis of human and animal infections, along with the laboratory's role in epidemiology and the management of infectious diseases.