首页> 外文期刊>The Journal of molecular diagnostics: JMD >Influenza A subtyping: seasonal H1N1, H3N2, and the appearance of novel H1N1.
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Influenza A subtyping: seasonal H1N1, H3N2, and the appearance of novel H1N1.

机译:甲型流感分型:季节性H1N1,H3N2和新颖H1N1的出现。

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摘要

Influenza virus subtyping has emerged as a critical tool in the diagnosis of influenza. Antiviral resistance is present in the majority of seasonal H1N1 influenza A infections, with association of viral strain type and antiviral resistance. Influenza A virus subtypes can be reliably distinguished by examining conserved sequences in the matrix protein gene. We describe our experience with an assay for influenza A subtyping based on matrix gene sequences. Viral RNA was prepared from nasopharyngeal swab samples, and real-time RT-PCR detection of influenza A and B was performed using a laboratory developed analyte-specific reagent-based assay that targets a conserved region of the influenza A matrix protein gene. FluA-positive samples were analyzed using a second RT-PCR assay targeting the matrix protein gene to distinguish seasonal influenza subtypes based on differential melting of fluorescence resonance energy transfer probes. The novel H1N1 influenza strain responsible for the 2009 pandemic showed a melting profile distinct from that of seasonal H1N1 or H3N2 and compatible with the predicted melting temperature based on the published novel H1N1 matrix gene sequence. Validation by comparison with the Centers for Disease Control and Prevention real-time RT-PCR for swine influenza A (novel H1N1) test showed this assay to be both rapid and reliable (>99% sensitive and specific) in the identification of the novel H1N1 influenza A virus strain.
机译:流感病毒亚型已成为诊断流感的关键工具。大多数季节性H1N1甲型流感感染都存在抗病毒耐药性,并且与病毒株类型和抗病毒耐药性相关。通过检查基质蛋白基因中的保守序列,可以可靠地区分出甲型流感病毒亚型。我们描述了基于矩阵基因序列进行A型流感亚型分析的经验。从鼻咽拭子样品中制备病毒RNA,并使用实验室开发的基于分析物特异性试剂的检测方法对A型和B型流感病毒进行实时RT-PCR检测,该检测方法针对A型流感病毒基质蛋白基因的保守区域。使用针对基质蛋白基因的第二次RT-PCR分析法对FluA阳性样品进行分析,以基于荧光共振能量转移探针的差异融合来区分季节性流感亚型。导致2009年大流行的新型H1N1流感病毒株的熔解谱不同于季节性H1N1或H3N2,并且与基于已发表的新型H1N1基质基因序列的预测熔解温度兼容。通过与疾病控制和预防中心的实时RT-PCR进行猪甲型流感(新型H1N1)检测的比较验证,结果表明,该方法在鉴定新型H1N1病毒时既快速又可靠(灵敏度和特异性均> 99%)甲型流感病毒株。

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