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Rapid Semiautomated Subtyping of Influenza Virus Species during the 2009 Swine Origin Influenza A H1N1 Virus Epidemic in Milwaukee, Wisconsin

机译:在威斯康星州密尔沃基市的2009年猪源甲型H1N1病毒流行期间,对流感病毒种进行快速半自动亚型分析

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In the spring of 2009, a novel influenza A (H1N1) virus (swine origin influenza virus [S-OIV]) emerged and began causing a large outbreak of illness in Milwaukee, WI. Our group at the Midwest Respiratory Virus Program laboratory developed a semiautomated real-time multiplex reverse transcription-PCR assay (Seasonal), employing the NucliSENS easyMAG system (bioMérieux, Durham, NC) and a Raider thermocycler (HandyLab Inc., Ann Arbor, MI), that typed influenza A virus, influenza B virus, and respiratory syncytial virus (RSV) and subtyped influenza A virus into the currently circulating H1 and H3 subtypes, as well as a similar assay that identified H1 of S-OIV. The Seasonal and H1 S-OIV assays demonstrated analytical limits of detection of <50 50% tissue culture infective doses/ml and 3 to 30 input copies, respectively. Testing of the analytical specificities revealed no cross-reactivity with 41 and 26 different common organisms and demonstrated outstanding reproducibility of results. Clinical testing showed 95% sensitivity for influenza A virus and influenza B virus and 95 and 97% specificity compared to tissue culture. Comparisons of results from other molecular tests showed levels of positive agreement with the Seasonal and H1 S-OIV assay results of 99 and 100% and levels of negative agreement of 98 and 100%. This study has demonstrated the use of a semiautomated system for sensitive, specific, and rapid detection of influenza A virus, influenza B virus, and RSV and subtyping of influenza A virus into human H1 and H3 and S-OIV strains. This assay/system performed well in clinical testing of regular seasonal influenza virus subtypes and was outstanding during the 2009 Milwaukee S-OIV infection outbreak. This recent outbreak of infection with a novel influenza A (H1N1) virus also demonstrates the importance of quickly distributing information on new agents and of having rapid influenza virus subtyping assays widely available for clinical and public health decisions.
机译:2009年春季,出现了一种新型的甲型H1N1流感病毒(猪源性流感病毒[S-OIV]),并开始在威斯康星州密尔沃基市引发大规模疾病暴发。我们小组在中西部呼吸道病毒计划实验室开发了一种半自动化的实时多重逆转录PCR方法(季节性),采用了NucliSENS easyMAG系统(北卡罗来纳州达勒姆的bioMérieux)和Raider热循环仪(密西根州安娜堡的HandyLab Inc. ),然后将A型流感病毒,B型流感病毒和呼吸道合胞病毒(RSV)以及亚型的A型流感病毒分为当前正在传播的H1和H3亚型,以及类似的检测方法来鉴定S-OIV的H1。季节性和H1 S-OIV分析分别显示了检测限<50 50%组织培养物感染剂量/ ml和3至30个输入拷贝的分析极限。分析特异性的测试表明,它与41种和26种不同的常见生物没有交叉反应,并显示了出色的结果可重复性。临床测试显示,与组织培养相比,甲型流感病毒和乙型流感病毒的敏感性为95%,特异性为95%和97%。其他分子测试结果的比较显示,季节性和H1 S-OIV分析结果的阳性一致性水平为99%和100%,阴性一致性的水平为98%和100%。这项研究证明了使用半自动化系统对甲型流感病毒,乙型流感病毒和RSV进行灵敏,特异和快速的检测,并将甲型流感病毒亚型分为人H1和H3以及S-OIV株。该分析/系统在常规季节性流感病毒亚型的临床测试中表现良好,在2009年密尔沃基S-OIV感染暴发期间表现出色。最近爆​​发的新型甲型H1N1流感病毒感染也证明了快速分发有关新药物的信息以及具有广泛用于临床和公共卫生决策的快速流感病毒亚型分析的重要性。

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