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由 HBV 基因型 A-H 的克隆患者 HBV 逆转录酶基因介导的 HBV DNA 复制及其在抗病毒表型测定中的应用。

HBV DNA replication mediated by cloned patient HBV reverse transcriptase genes from HBV genotypes A-H and its use in antiviral phenotyping assays.

机构信息

Gilead Sciences, Inc., 333 Lakeside Drive, Foster City, CA 94404, United States.

出版信息

J Virol Methods. 2011 May;173(2):340-6. doi: 10.1016/j.jviromet.2011.03.006. Epub 2011 Mar 17.

DOI:10.1016/j.jviromet.2011.03.006
PMID:21396961
Abstract

The aim of this study is to establish a phenotyping assay to analyze patient HBV polymerase/reverse transcriptase (RT) sequences for potential drug resistance against RT inhibitors. HBV RT (pol aa 304-715, including the entire RT) from clinical isolates were amplified and ligated into a plasmid vector (pRTAN) expressing a genotype A HBV genome lacking the RT region. HBV DNA replication of the recombinants and their drug susceptibilities were assessed by transient transfection into HepG2 cells and intracellular core DNA was analyzed either by Southern blot or using a 96-well format and quantification by qPCR. Cloning of the HBV RT gene from clinical isolates representing genotypes A-H was successful and led to virus DNA replication. Recombinants expressing patient derived RT genes containing the rtL180M+M204V lamivudine resistance (LAM-R) mutations demonstrated a LAM-R phenotype. Similarly, patient derived RT genes containing the adefovir resistance (ADV-R) mutations rtA181V or rtN236T demonstrated an ADV-R phenotype. Recombinants containing HBV RT from paired patient samples without genotypic changes had similar EC(50) values. In conclusion, a phenotyping assay for HBV RT gene was developed, allowing evaluation of patient-derived HBV RT from genotypes A-H, and confirmed the drug resistance phenotype in samples containing LAM-R or ADV-R mutations.

摘要

本研究旨在建立一种表型分析方法,以分析患者乙型肝炎病毒聚合酶/逆转录酶(RT)序列中对 RT 抑制剂的潜在耐药性。从临床分离株中扩增 HBV RT(pol aa 304-715,包括整个 RT),并将其连接到表达缺乏 RT 区的基因型 A HBV 基因组的质粒载体(pRTAN)中。通过瞬时转染 HepG2 细胞评估重组体的 HBV DNA 复制及其药物敏感性,并通过 Southern blot 或 96 孔格式进行细胞内核心 DNA 分析,并通过 qPCR 进行定量。成功克隆了代表基因型 A-H 的临床分离株的 HBV RT 基因,并导致病毒 DNA 复制。表达含有 rtL180M+M204V 拉米夫定耐药(LAM-R)突变的患者衍生 RT 基因的重组体表现出 LAM-R 表型。同样,含有阿德福韦耐药(ADV-R)突变 rtA181V 或 rtN236T 的患者衍生 RT 基因也表现出 ADV-R 表型。含有基因型无变化的患者样本的 HBV RT 的重组体具有相似的 EC(50)值。总之,已经开发出一种用于 HBV RT 基因的表型分析方法,允许评估来自基因型 A-H 的患者衍生 HBV RT,并确认含有 LAM-R 或 ADV-R 突变的样本中的耐药表型。

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