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首页> 外文期刊>Journal of Clinical Microbiology >Sensitive Assay for Quantification of Hepatitis B Virus Mutants by Use of a Minor Groove Binder Probe and Peptide Nucleic Acids
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Sensitive Assay for Quantification of Hepatitis B Virus Mutants by Use of a Minor Groove Binder Probe and Peptide Nucleic Acids

机译:通过使用小槽活页夹探针和肽核酸定量分析乙型肝炎病毒突变体的灵敏方法

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Lamivudine is the first nucleoside analogue that was shown to have a potent effect on hepatitis B virus (HBV). However, the emergence of mutants resistant or cross-resistant to nucleosideucleotide analogues remains a serious problem. Several assays for the detection and quantification of antiviral-resistant mutants have been reported, but it has been difficult to measure the amounts of mutants accurately, especially when the target strain is a minor component of the mixed population. It has been shown that accurate measurement of a minor strain is difficult as long as a matching reaction with a single probe is included in the assay. We developed a new method for the quantification of lamivudine-resistant strains in a mixed-virus population by real-time PCR using minor groove binder probes and peptide nucleic acids, and we achieved a wide and measurable range, from 3 to 10 log10 copies/ml, and high sensitivity, with a discriminative limit of 0.01% of the predominant strain. The clinical significance of measuring substitutions not only of M204 but also of L180 residues of HBV polymerase was demonstrated by this method. This assay increases the versatility of a sensitive method for the quantification of a single-nucleotide mutation in a heterogeneous population.
机译:拉米夫定是第一个被证明对乙型肝炎病毒(HBV)具有有效作用的核苷类似物。然而,对核苷/核苷酸类似物具有抗性或交叉抗性的突变体的出现仍然是一个严重的问题。已经报道了几种检测和定量抗病毒抗性突变体的方法,但是很难准确地测量突变体的数量,特别是当目标菌株是混合群体的一小部分时。已经表明,只要测定中包括与单个探针的匹配反应,就很难精确测量次要菌株。我们开发了一种新的方法,通过使用小沟结合剂探针和肽核酸的实时PCR定量混合病毒种群中的拉米夫定耐药菌株,我们实现了从3到10 log 10 拷贝/ ml,灵敏度高,判别极限为主要菌株的0.01%。通过该方法证明了不仅测量M204的取代,而且测量HBV聚合酶的L180残基的取代的临床意义。该测定法提高了定量异质群体中单核苷酸突变的灵敏方法的多功能性。

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