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Luminex xTAG呼吸道病毒检测快速v2分析试剂盒与Anyplex II RV16检测试剂盒及AdvanSure RV实时逆转录聚合酶链反应分析试剂盒用于呼吸道病毒检测的比较

Comparison of the Luminex xTAG Respiratory Viral Panel Fast v2 Assay With Anyplex II RV16 Detection Kit and AdvanSure RV Real-Time RT-PCR Assay for the Detection of Respiratory Viruses.

作者信息

Ko Dae Hyun, Kim Hyun Soo, Hyun Jungwon, Kim Han Sung, Kim Jae Seok, Park Kyoung Un, Song Wonkeun

机构信息

Department of Laboratory Medicine, Hallym University College of Medicine, Hwaseong, Korea.

Department of Laboratory Medicine, Seoul National University Bundang Hospital, Seongnam, Korea.

出版信息

Ann Lab Med. 2017 Sep;37(5):408-414. doi: 10.3343/alm.2017.37.5.408.

DOI:10.3343/alm.2017.37.5.408
PMID:28643489
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5500739/
Abstract

BACKGROUND

The accurate and rapid identification of the causative viruses is important for the timely diagnosis and management of respiratory infections. Multiplex molecular diagnostic techniques have been widely adopted to detect respiratory viruses. We compared the results of a newly upgraded, multiplex, molecular bead-based respiratory viral panel (RVP) assay with the results of Anyplex II RV16 detection kit and AdvanSure RV real-time RT-PCR assay.

METHODS

We tested 254 respiratory specimens and cultured viral strains using the Luminex xTAG RVP Fast v2 assay (Luminex Molecular Diagnostics, Canada) and Anyplex II RV16 detection kit and compared the results. Specimens showing discordant results between the two assays were tested with a AdvanSure RV real-time RT-PCR assay.

RESULTS

Of the 254 respiratory specimens, there was total agreement in the results between the xTAG RVP Fast v2 assay and the other real-time PCR assay in 94.1-100% of the specimens. The agreement levels were relatively low (94.1-97.6%) for specimens of adenovirus, coronavirus NL63, and parainfluenza type 3. In comparison to the other assay, the xTAG RVP Fast v2 assay detected a higher number of parainfluenza type 3 (4 cases) and metapneumovirus (9 cases).

CONCLUSIONS

The xTAG RVP Fast v2 assay showed comparable capabilities compared with the other assays; it will be useful for identifying respiratory viral infections in patients with respiratory symptoms. Clinicians should be aware of the characteristics of the assays they use, since different assays show different detectability for each virus.

摘要

背景

准确快速地鉴定致病病毒对于呼吸道感染的及时诊断和管理至关重要。多重分子诊断技术已被广泛用于检测呼吸道病毒。我们将新升级的基于分子珠的多重呼吸道病毒检测板(RVP)检测结果与Anyplex II RV16检测试剂盒及AdvanSure RV实时逆转录聚合酶链反应(RT-PCR)检测结果进行了比较。

方法

我们使用Luminex xTAG RVP Fast v2检测法(加拿大Luminex分子诊断公司)、Anyplex II RV16检测试剂盒对254份呼吸道标本和培养的病毒株进行检测,并比较结果。对两种检测结果不一致的标本采用AdvanSure RV实时RT-PCR检测法进行检测。

结果

在254份呼吸道标本中,xTAG RVP Fast v2检测法与其他实时PCR检测法的结果在94.1%-100%的标本中完全一致。腺病毒、冠状病毒NL63和3型副流感病毒标本的一致性水平相对较低(94.1%-97.6%)。与其他检测法相比,xTAG RVP Fast v2检测法检测出的3型副流感病毒(4例)和偏肺病毒(9例)数量更多。

结论

xTAG RVP Fast v2检测法与其他检测法相比具有相当的能力;它将有助于识别有呼吸道症状患者的呼吸道病毒感染。临床医生应了解他们所使用检测法的特点,因为不同的检测法对每种病毒的检测能力不同。

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