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Simultaneous Quantification and Genotyping of Hepatitis B Virus for Genotypes A to G by Real-Time PCR and Two-Step Melting Curve Analysis▿

机译:实时PCR和两步解链曲线分析同时对A型至G型乙型肝炎病毒进行定量和基因分型▿

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摘要

Both the viral titer and the genotype significantly determine clinical outcomes and responses to antiviral treatment in chronic hepatitis B virus (HBV) infection. A method was developed for large-scale A-to-G genotyping with simultaneous viral quantification. The assay was run on a LightCycler instrument using hybridization probes. The genotype was determined from the melting points of the probes in a two-step manner. Set 1 amplicons differentiated genotypes B, E, and F from A, C, D, and G and simultaneously quantified viremia by real-time PCR. Melting curve analysis using the set 2-1 amplicon or the set 2-2 amplicon reaction mixture was then used to differentiate these genotype groups into single genotypes. HBV DNA quantification was consistent with that of the Amplicor assay and linear in a range from 102 to 1013 copies/ml. By comparison with the restriction fragment length polymorphism method, 92.3% of 441 samples were accurately genotyped by the current assay. The method should be useful for genotyping and quantification of HBV DNA in areas where all genotypes exist.
机译:病毒滴度和基因型均显着决定了慢性乙型肝炎病毒(HBV)感染的临床结局和对抗病毒治疗的反应。开发了一种用于大规模A-G基因分型并同时进行病毒定量的方法。使用杂交探针在LightCycler仪器上进行测定。从探针的熔点以两步方式确定基因型。组1扩增子将基因型B,E和F与A,C,D和G区分开,并同时通过实时PCR定量病毒血症。然后使用设置2-1的扩增子或设置2-2的扩增子反应混合物进行熔解曲线分析,以将这些基因型组区分为单个基因型。 HBV DNA定量与Amplicor测定一致,线性范围为102至1013拷贝/ ml。通过与限制性酶切片段长度多态性方法比较,当前的测定法对441个样品中的92.3%进行了准确的基因分型。该方法对于所有基因型均存在的地区的HBV DNA的基因分型和定量分析应该是有用的。

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