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

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

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...

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Veröffentlicht in:Journal of clinical microbiology 2015-06, Vol.53 (6), p.1831-1835
Hauptverfasser: Chook, Jack Bee, Teo, Woon Li, Ngeow, Yun Fong, Tee, Kok Keng, Ng, Kee Peng, Mohamed, Rosmawati
Format: Artikel
Sprache:eng
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DNA Primers - genetics
Genome, Viral - genetics
Genotype
Hepatitis B - virology
Hepatitis B virus
Hepatitis B virus - genetics
Humans
Sequence Analysis, DNA - methods
Virology
Virology - methods
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container_end_page 1835
container_issue 6
container_start_page 1831
container_title Journal of clinical microbiology
container_volume 53
creator Chook, Jack Bee
Teo, Woon Li
Ngeow, Yun Fong
Tee, Kok Keng
Ng, Kee Peng
Mohamed, Rosmawati
description 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.
doi_str_mv 10.1128/JCM.03449-14
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subjects DNA Primers - genetics
Genome, Viral - genetics
Genotype
Hepatitis B - virology
Hepatitis B virus
Hepatitis B virus - genetics
Humans
Sequence Analysis, DNA - methods
Virology
Virology - methods
title Universal Primers for Detection and Sequencing of Hepatitis B Virus Genomes across Genotypes A to G
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