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首页> 外文OA文献 >Switching Gears for an Influenza Pandemic: Validation of a Duplex Reverse Transcriptase PCR Assay for Simultaneous Detection and Confirmatory Identification of Pandemic (H1N1) 2009 Influenza Virus ▿
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Switching Gears for an Influenza Pandemic: Validation of a Duplex Reverse Transcriptase PCR Assay for Simultaneous Detection and Confirmatory Identification of Pandemic (H1N1) 2009 Influenza Virus ▿

机译:流感大流行的开关设备:用于同时检测和确认鉴定大流行性(H1N1)2009流感病毒的双重逆转录酶PCR检测方法的验证▿

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Rapid methods for the detection and confirmatory identification of pandemic influenza A virus (also known as pandemic [H1N1] 2009) are of utmost importance. In this study, a conventional reverse transcriptase PCR (RT-PCR) assay for the detection of influenza A virus and the hemagglutinin of swine lineage H1 (swH1) was designed, optimized, and validated. Nucleic acids were extracted from 198 consecutive nasopharyngeal, nasal, or throat swab specimens collected early in the outbreak (127 negative specimens, 66 specimens with pandemic [H1N1] 2009 influenza virus, 3 specimens with seasonal [H1N1] influenza A virus, and 2 specimens with seasonal [H3N2] influenza A virus). The performance characteristics of the duplex RT-PCR assay were assessed and compared to those of various detection methods: a monoplex RT-PCR assay at the National Microbiology Laboratory, a real-time RT-PCR assay using a Centers for Disease Control and Prevention protocol, an in-house multiplex RT-PCR assay (targeting influenza A virus, influenza B virus, and respiratory syncytial virus), and a rapid antigen test (the Binax Now Influenza A & B assay). The sensitivity of the duplex RT-PCR assay for influenza A virus detection was 97.2%, whereas the sensitivities were 74.6%, 71.8%, 47.8%, and 12.7% for the other four assays, respectively. The duplex RT-PCR assay was also able to identify swH1 in 94% of the cases, thereby reducing the number of specimens forwarded to reference laboratories for confirmatory identification. Only a limited number of specimens that contained influenza A virus had amounts of virus that fell below the limit of detection of the assay with the swH1 primers. Overall, the duplex RT-PCR assay is a reliable method for the simultaneous detection and confirmatory identification of pandemic (H1N1) 2009 influenza virus and would be particularly attractive to laboratories without real-time RT-PCR capabilities.
机译:快速检测和确认大流行性流感病毒(也称为大流行[H1N1] 2009)的方法至关重要。在本研究中,设计,优化和验证了用于检测甲型流感病毒和猪血统H1(swH1)血凝素的常规逆转录酶PCR(RT-PCR)分析方法。从暴发初期收集的198个连续的鼻咽,鼻或咽拭子样本中提取核酸(127个阴性样本,66个具有2009年大流行[H1N1]流感病毒的标本,3个具有季节性[H1N1]甲型流感病毒的标本和2个标本)季节性[H3N2]甲型流感病毒)。评估了双工RT-PCR分析的性能特征,并将其与各种检测方法的性能特征进行了比较:美国国家微生物学实验室的单重RT-PCR分析,使用疾病预防控制中心的实时RT-PCR分析,内部多重RT-PCR分析(针对甲型流感病毒,乙型流感病毒和呼吸道合胞病毒),以及快速抗原检测(Binax Now流感A和B分析)。双重RT-PCR检测对甲型流感病毒的敏感性为97.2%,而其他四种检测的敏感性分别为74.6%,71.8%,47.8%和12.7%。双重RT-PCR测定法还能够在94%的病例中鉴定swH1,从而减少了转交给参考实验室进行确认性鉴定的标本数量。只有有限数量的包含甲型流感病毒的标本的病毒量低于使用swH1引物检测的检测限。总体而言,双重RT-PCR分析是同时检测和确认大流行(H1N1)2009流感病毒的可靠方法,对没有实时RT-PCR功能的实验室特别有吸引力。

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