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Highly Sensitive and Quantitative Detection of the H274Y Oseltamivir Resistance Mutation in Seasonal A/H1N1 Influenza Virus ▿

机译:季节性A / H1N1流感病毒中H274Y奥瑟他韦抗性突变的高灵敏定量检测▿

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摘要

A C-to-T transition mutation in the neuraminidase gene from seasonal A/H1N1 causes a His-to-Tyr mutation at amino acid position 275 (H274Y, universal N2 numbering), conferring resistance against oseltamivir (Tamiflu). This mutation was first detected in clinical samples in Europe during the 2007-2008 influenza season. Viruses with this mutation reached a prevalence of ∼11% by the end of the season in North American isolates tested by the CDC. We developed a highly sensitive and specific quantitative real-time reverse transcriptase PCR assay to detect the H274Y mutation. This assay utilizes a 5′-methyl-isocytosine (isoC) residue and fluorescent reporters on genotype-specific primers. During PCR, a quencher coupled to isoguanine (isoG) is site-specifically incorporated complementary to the isoC/dye, resulting in loss of fluorescence. Optimization of primers and assay conditions produced a limit of detection of 100 gene copies per reaction for both wild-type and H274Y genotypes. In samples with mixed populations, it can reliably detect as little as a 1% wild-type or 0.1% H274Y component. This high sensitivity makes the assay usable on samples with viral loads too low for dideoxy or pyrosequencing analysis. Additionally, the assay distinguishes seasonal A/H1N1 from A/H3N2, influenza B, or 2009 pandemic A/H1N1, making it useful for influenza virus subtyping as well as for drug resistance detection. We probed seasonal A/H1N1 samples from the 2005-2006, 2006-2007, and 2007-2008 influenza seasons. Data from the new assay closely matched available drug resistance genotype data previously determined by dideoxy sequencing. The H274Y mutation was only found in samples from the 2007-2008 season.
机译:来自季节性A / H1N1的神经氨酸酶基因中的C到T转换突变导致第275位氨基酸处的His到Tyr突变(H274Y,通用N2编号),赋予了对奥司他韦(Tamiflu)的耐药性。此突变是在2007-2008年流感季节期间在欧洲的临床样本中首次发现的。到本季节结束时,在CDC测试的北美分离物中,具有这种突变的病毒的流行率达到约11%。我们开发了一种高灵敏度和特异性的实时定量逆转录酶PCR检测法,以检测H274Y突变。该测定法利用基因型特异性引物上的5'-甲基-异胞嘧啶(isoC)残基和荧光报告分子。在PCR期间,与异鸟嘌呤(isoG)偶联的淬灭剂与isoC / dye互补互补位点掺入,导致荧光损失。引物和测定条件的优化产生了针对野生型和H274Y基因型每个反应100个基因拷贝的检测极限。在具有混合种群的样品中,它可以可靠地检测出低至1%的野生型或0.1%的H274Y成分。这种高灵敏度使该测定法可用于病毒载量太低而无法进行双脱氧或焦磷酸测序分析的样品。此外,该测定法还可以将季节性A / H1N1与A / H3N2,乙型流感或2009年大流行性A / H1N1区别开来,使其可用于流感病毒分型和耐药性检测。我们调查了2005-2006、2006-2007和2007-2008流感季节的季节性A / H1N1样本。来自新测定的数据与先前通过双脱氧测序确定的可用药物抗性基因型数据紧密匹配。 H274Y突变仅在2007-2008季节的样品中发现。

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