Technical validation of a multiplex real-time PCR for combined detection of Rift Valley fever, chikungunya, Zika and dengue viruses

IF 1.6 4区医学 Q3 BIOCHEMICAL RESEARCH METHODS

Journal of virological methods Pub Date : 2025-05-07 DOI:10.1016/j.jviromet.2025.115174

Anne Hauner , Stijn Rogé , Veerle Vanlerberghe , Luciana Lepore , Fabrice Ndayisenga , Anselme Shyaka , Marjan Van Esbroeck , Silvia Situma , Carolyne Nasimiyu , Steve Ahuka-Mundeke , M. Kariuki Njenga , Robert F. Breiman , Justin Masumu , Daniel Mukadi-Bamuleka , Kevin K. Ariën

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引用次数: 0

Abstract

Several arthropod-borne (arbo)-viruses have overlapping symptoms, insect vectors and geographical occurrence. With little known about the importance of arboviruses as cause of acute undifferentiated fever (AUF) in East and Central Africa (ECA), there is a clear need for a multiplex-PCR allowing for multi-pathogen surveillance. A multiplex real-time RT-PCR (RDCZ-multiplex) was developed and validated for the simultaneous detection of Rift Valley fever virus (RVFV), dengue virus 1–4 (DENV), chikungunya virus (CHIKV) and Zika virus (ZIKV). Phocine distemper virus (PDV) was added to the PCR as sample extraction control. Validation was conducted following the MIQE-guidelines using a panel of retrospective clinical samples and Quality Control for Molecular Diagnostics (QCMD, https://www.qcmd.org/en/) samples with the simplex-PCR as reference. These included samples from RVFV in animals (n = 19), DENV (n = 15), CHIKV (n = 11), ZIKV (n = 2) and YFV (n = 1, QCMD), and 14 negative endemic controls. Extractions and PCRs were done with commercially available kits. Some loss of sensitivity was observed at low target concentrations for RVFV, DENV1 and DENV4, when comparing the standard curves of simplex-PCRs with the multiplex-PCR. The limit of detection of the multiplex-PCR was 2064 copies/ml for CHIKV, 3587 copies/ml for DENV1, 30,249 copies/ml for ZIKV and 73 PFU/ml for RVFV. Specificity of the multiplex-PCRs was 100 %. For 12 out of 48 positive samples with high Cq values, RVFV (n = 7), CHIKV (n = 2), DENV1 (n = 2), YFV (n = 1), the multiplex-PCRs were negative. Although PCR sensitivity of the RDCZ-multiplex is slightly lower with low target concentrations, it offers a useful tool for molecular surveillance and clinical diagnosis for arboviruses for the ECA-region.

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多重实时PCR联合检测裂谷热、基孔肯雅热、寨卡和登革热病毒的技术验证

一些节肢动物传播的病毒具有重叠的症状、昆虫媒介和地理分布。由于对虫媒病毒作为东非和中非（ECA）急性未分化热（AUF）病因的重要性知之甚少，因此显然需要一种多重聚合酶链反应，以便进行多病原体监测。建立了同时检测裂谷热病毒（RVFV）、登革热病毒1-4 （DENV）、基孔肯雅病毒（CHIKV）和寨卡病毒（ZIKV）的多重实时RT-PCR （RDCZ-multiplex）方法并进行了验证。PCR中加入猪瘟热病毒（PDV）作为样品提取对照。采用回顾性临床样本和分子诊断质量控制（QCMD, https://www.qcmd.org/en/）样本，并以simplex-PCR作为参考，按照miq指南进行验证。其中包括样本RVFV动物(n = 19),DENV (n = 15),CHIKV (n = 11),ZIKV (n = 2)和YFV (n = QCMD), 14 -流行控制。提取和pcr用市售试剂盒进行。在低目标浓度下，对RVFV、DENV1和DENV4进行检测时，将单一- pcr标准曲线与多重- pcr标准曲线进行比较，发现灵敏度有所下降。多重pcr检出限分别为：CHIKV为2064 copies/ml， DENV1为3587 copies/ml， ZIKV为30249 copies/ml， RVFV为73 PFU/ml。多重pcr的特异性为100% %。48份高Cq值阳性样本中，RVFV （n = 7）、CHIKV （n = 2）、DENV1 （n = 2）、YFV (n = 1)12份多重pcr均为阴性。虽然在低靶浓度下，RDCZ-multiplex的PCR敏感性略低，但它为eca区虫媒病毒的分子监测和临床诊断提供了一种有用的工具。

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来源期刊

Journal of virological methods 医学-病毒学

CiteScore

5.80

自引率

0.00%

发文量

209

审稿时长

41 days

期刊介绍： The Journal of Virological Methods focuses on original, high quality research papers that describe novel and comprehensively tested methods which enhance human, animal, plant, bacterial or environmental virology and prions research and discovery. The methods may include, but not limited to, the study of: Viral components and morphology- Virus isolation, propagation and development of viral vectors- Viral pathogenesis, oncogenesis, vaccines and antivirals- Virus replication, host-pathogen interactions and responses- Virus transmission, prevention, control and treatment- Viral metagenomics and virome- Virus ecology, adaption and evolution- Applied virology such as nanotechnology- Viral diagnosis with novelty and comprehensive evaluation. We seek articles, systematic reviews, meta-analyses and laboratory protocols that include comprehensive technical details with statistical confirmations that provide validations against current best practice, international standards or quality assurance programs and which advance knowledge in virology leading to improved medical, veterinary or agricultural practices and management.