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Universal Primers for Detection and Sequencing of Hepatitis B Virus Genomes across Genotypes A to G

机译:通用引物,用于检测基因型A至G的乙型肝炎病毒基因组

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Hepatitis B virus (HBV) has been divided into 10 genotypes, A to J, based on an 8% nucleotide sequence divergence between genotypes. The conventional practice of using a single set of primers to amplify a near-complete HBV genome is hampered by its low analytical sensitivity. The current practice of using overlapping conserved primer sets to amplify a complete HBV genome in a clinical sample is limited by the lack of pan-primers to detect all HBV genotypes. In this study, we designed six highly conserved, overlapping primer sets to cover the complete HBV genome. We based our design on the sequences of 5,154 HBV genomes of genotypes A to I downloaded from the GenBank nucleotide database. These primer sets were tested on 126 plasma samples from Malaysia, containing genotypes A to D and with viral loads ranging from 20 to >79,780,000 IU/ml. The overall success rates for PCR amplification and sequencing were >96% and >94%, respectively. Similarly, there was 100% amplification and sequencing success when the primer sets were tested on an HBV reference panel of genotypes A to G. Thus, we have established primer sets that gave a high analytical sensitivity for PCR-based detection of HBV and a high rate of sequencing success for HBV genomes in most of the viral genotypes, if not all, without prior known sequence data for the particular genotype/genome.
机译:根据基因型之间8%的核苷酸序列差异,乙型肝炎病毒(HBV)已分为10种基因型,从A到J。使用单组引物扩增接近完整的HBV基因组的常规做法因其较低的分析灵敏度而受阻。目前,在临床样品中使用重叠的保守引物组来扩增完整的HBV基因组的做法由于缺乏检测所有HBV基因型的泛引物而受到限制。在这项研究中,我们设计了六个高度保守的重叠引物组,以覆盖完整的HBV基因组。我们基于从GenBank核苷酸数据库下载的基因型A至I的5,154个HBV基因组序列设计。这些引物对来自马来西亚的126个血浆样本进行了测试,这些样本含有A至D基因型,病毒载量范围为20至> 79,780,000 IU / ml。 PCR扩增和测序的总体成功率分别> 96%和> 94%。同样,当在基因型A到G的HBV参考面板上测试引物组时,扩增和测序成功100%。因此,我们建立了引物组,这些引物组对基于PCR的HBV检测具有很高的分析灵敏度,并且对大部分病毒基因型(如果不是全部)中的HBV基因组测序成功率,如果没有特定基因型/基因组的事先已知序列数据。

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