首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Optimization of a Combined Human Parechovirus-Enterovirus Real-Time Reverse Transcription-PCR Assay and Evaluation of a New Parechovirus 3-Specific Assay for Cerebrospinal Fluid Specimen Testing
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Optimization of a Combined Human Parechovirus-Enterovirus Real-Time Reverse Transcription-PCR Assay and Evaluation of a New Parechovirus 3-Specific Assay for Cerebrospinal Fluid Specimen Testing

机译:人肺细小病毒-肠道病毒实时逆转录-PCR联合检测方法的优化和脑脊髓液标本检测的新型细小病毒3-特异性检测方法的评估

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摘要

Human parechoviruses (HPeVs), particularly type 3 (HPeV3), are known central nervous system (CNS) pathogens, causing serious infections in infants similar to those caused by enteroviruses (EVs). The primary aim of this study was to combine and validate HPeV and EV real-time reverse transcription-PCR (RT-PCR) detection assays with the best available RT-PCR reagents and conditions for parallel detection of HPeV and EV on a single platform. The secondary aim was to develop and validate a newly developed HPeV3-specific real-time RT-PCR assay. Five commercially available RT-PCR kits were evaluated with the pan-HPeV and EV assays in one-step and two-step RT-PCRs. Two-step RT-PCR with the AgPath ID RT-PCR (AGP) kit performed best for both pan-HPeV and EV assays. The pan-HPeV-specific assay performed best with the AGP kit in a one-step RT-PCR. Frozen aliquots of 145 (for HPeV, n = 70; for EV, n = 75) previously characterized cerebrospinal fluid (CSF) specimens were tested by EV-, pan-HPeV-, and HPeV3-specific (HPeV specimens only) assays. The pan-HPeV and EV assays demonstrated 100% analytical sensitivity and specificity compared to historic results, while the HPeV3-specific assay demonstrated 97% sensitivity and 100% specificity. We propose a real-time pan-HPeV, EV two-step RT-PCR algorithm for simultaneous detection of HPeV and EV from CSF specimens on a single platform. The HPeV3-specific one-step RT-PCR assay can be used as a rapid and cost-effective assay to detect and identify HPeV3 in pan-HPeV RT-PCR assay-positive CSF specimens.
机译:人副病毒(HPeV),特别是3型(HPeV3),是已知的中枢神经系统(CNS)病原体,在婴儿中引起的严重感染与肠道病毒(EV)引起的感染相似。这项研究的主要目的是将HPeV和EV实时逆转录PCR(RT-PCR)检测分析与最佳可得的RT-PCR试剂和条件相结合并验证,以在单个平台上并行检测HPeV和EV。第二个目的是开发和验证新开发的HPeV3特异性实时R​​T-PCR检测方法。使用pan-HPeV和EV测定法在一步和两步RT-PCR中评估了五种市售RT-PCR试剂盒。带有AgPath ID RT-PCR(AGP)试剂盒的两步RT-PCR在泛HPeV和EV分析中表现最佳。使用AGP试剂盒在一步式RT-PCR中进行pan-HPeV特异性检测的效果最佳。通过EV,pan-HPeV-和HPeV3特异性检测(仅HPeV样本)检测了145份冻存的等分试样(对于HPeV,n = 70;对于EV,n = 75)先前表征的脑脊液(CSF)标本。与历史结果相比,pan-HPeV和EV分析显示出100%的分析灵敏度和特异性,而HPeV3特异性分析显示出97%的灵敏度和100%特异性。我们提出了一种实时的泛HPeV,EV两步RT-PCR算法,用于在单个平台上同时检测CSF标本中的HPeV和EV。 HPeV3特异性的一步式RT-PCR测定法可作为一种快速且经济高效的测定法来检测和鉴定泛HPeV RT-PCR测定呈阳性的CSF标本中的HPeV3。

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