首页> 美国卫生研究院文献>Journal of Clinical Microbiology >Rapid Multiplex Reverse Transcription-PCR Typing of Influenza A and B Virus and Subtyping of Influenza A Virus into H1 2 3 5 7 9 N1 (Human) N1 (Animal) N2 and N7 Including Typing of Novel Swine Origin Influenza A (H1N1) Virus during the 2009 Outbreak in Milwaukee Wisconsin
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Rapid Multiplex Reverse Transcription-PCR Typing of Influenza A and B Virus and Subtyping of Influenza A Virus into H1 2 3 5 7 9 N1 (Human) N1 (Animal) N2 and N7 Including Typing of Novel Swine Origin Influenza A (H1N1) Virus during the 2009 Outbreak in Milwaukee Wisconsin

机译:甲型和乙型流感病毒的快速多重逆转录PCR键入以及将甲型流感病毒亚型分为H1、2、3、5、7、9N1(人类)N1(动物)N2和N7包括键入威斯康星州密尔沃基市2009年爆发的新型猪源性甲型H1N1流感病毒的传播

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摘要

A large outbreak of novel influenza A (H1N1) virus (swine origin influenza virus [S-OIV]) infection in Milwaukee, WI, occurred in late April 2009. We had recently developed a rapid multiplex reverse transcription-PCR enzyme hybridization assay (FluPlex) to determine the type (A or B) and subtype (H1, H2, H3, H5, H7, H9, N1 [human], N1 [animal], N2, or N7) of influenza viruses, and this assay was used to confirm the diagnoses for the first infected patients in the state. The analytical sensitivity was excellent at 1.5 to 116 copies/reaction, or 10−3 to 10−1 50% tissue culture infective doses/ml. The testing of all existing hemagglutinin and neuraminidase subtypes of influenza A virus and influenza B virus (41 influenza virus strains) and 24 common respiratory pathogens showed only one low-level H3 cross-reaction with an H10N7 avian strain and only at 5.2 × 106 copies/reaction, not at lower concentrations. Comparisons of the FluPlex results with results from multiple validated in-house molecular assays, CDC-validated FDA-approved assays, and gene sequencing demonstrated 100% positive agreement for the typing of 179 influenza A viruses and 3 influenza B viruses, the subtyping of 110 H1N1 (S-OIV; N1 [animal]), 62 H1N1 (human), and 6 H3N2 (human) viruses, and the identification of 24 negative clinical samples and 100% negative agreement for all viruses tested except H1N1 (human) (97.7%). The small number of false-positive H1N1 (human) samples most likely represent increased sensitivity over that of other in-house assays, with four of four results confirmed by the CDC's influenza virus subtyping assay. The FluPlex is a rapid, inexpensive, sensitive, and specific method for the typing and subtyping of influenza viruses and demonstrated outstanding utility during the first 2 weeks of an S-OIV infection outbreak. Methods for rapid detection and broad subtyping of influenza viruses, including animal subtypes, are needed to address public concern over the emergence of pandemic strains. Attempts to automate this assay are ongoing.
机译:2009年4月下旬,在威斯康星州密尔沃基爆发了大规模的新型A型流感(H1N1)病毒(猪源流感病毒[S-OIV])感染。我们最近开发了一种快速的多重逆转录PCR PCR杂交试验(FluPlex )以确定流感病毒的类型(A或B)和亚型(H1,H2,H3,H5,H7,H9,N1 [人类],N1 [动物],N2或N7),并且该测定法用于确认该州首批感染患者的诊断。分析灵敏度在1.5至116个拷贝/反应或10 -3 至10 -1 50%组织培养感染剂量/ ml时极佳。对所有现有的A型流感病毒和B型流感病毒血凝素和神经氨酸酶亚型(41种流感病毒株)和24种常见呼吸道病原体的测试显示,仅一种低水平的H3与H10N7禽流感株发生交叉反应,并且只有5.2×10 < sup> 6 复制/反应,而不是较低的浓度。 FluPlex结果与多种经过验证的内部分子分析,CDC验证的FDA批准的分析以及基因测序结果的比较,表明179种甲型流感病毒和3种乙型流感病毒的分型分别为100%阳性,其中110个分型H1N1(S-OIV; N1 [动物]),62种H1N1(人类)和6种H3N2(人类)病毒,对于除H1N1(人类)以外的所有测试病毒,鉴定出24份阴性临床样品和100%阴性一致性(97.7 %)。少量假阳性H1N1(人类)样本最有可能代表了比其他内部检测更高的敏感性,CDC的流感病毒亚型检测证实了四个结果中的四个。 FluPlex是一种快速,廉价,敏感,特异的流感病毒分型和分型方法,在S-OIV感染爆发的前两周内显示出出色的效用。需要快速检测流感病毒和包括动物亚型在内的广泛亚型的方法,以解决公众对大流行毒株出现的关注。自动化该测定的尝试正在进行中。

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