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序列分析、INNO-LiPA线性探针检测法及AFFIGENE检测法在检测乙型肝炎病毒聚合酶及前核心/核心启动子突变中的性能。

Performance of sequence analysis, INNO-LiPA line probe assays and AFFIGENE assays in the detection of hepatitis B virus polymerase and precore/core promoter mutations.

作者信息

Olivero A, Ciancio A, Abate M L, Gaia S, Smedile A, Rizzetto M

机构信息

Department of Gastroenterology and Hepatology, Molinette Hospital, Turin, Italy.

出版信息

J Viral Hepat. 2006 Jun;13(6):355-62. doi: 10.1111/j.1365-2893.2005.00693.x.

DOI:10.1111/j.1365-2893.2005.00693.x
PMID:16842437
Abstract

In this study, we compare results obtained by sequences analysis and commercial kits in the detection of hepatitis B virus (HBV) polymerase and precore (PC) and core promoter mutations. A total of 23 serum samples from lamivudine treated patients were tested for polymerase mutations by direct sequencing, INNO-LiPA HBV DR and AFFIGENE HBV DE/3TC. Full concordance among the three assays was observed in 63% of the total analysed codons. Concordant results were obtained between sequencing and LiPA in 80%, between sequencing and AFFIGENE in 73% and between LiPA and AFFIGENE in 74% of all tested codons. All discrepancies were observed in mixed population samples in which AFFIGENE and LiPA detected additional viral variants not revealed by sequence. In two patients, with serial samples, LiPA detected earlier than sequence and AFFIGENE an emerging mutate strain. PC and core promoter viral variants were detected in 28 serum samples collected from 14 HBV inactive carriers and from 14 hepatitis B patients with chronic liver disease. Direct sequencing, INNO-LiPA HBV PreCore and AFFIGENE HBV MUTANT VL 19 showed fully coincident results in 88% of tested positions. These findings showed that all assays evaluated were sensitive and accurate tools to analyse HBV genomic variability. Sequence analysis is essential to study new emerging mutations as LiPA and AFFIGENE assays are more easily useful in clinical laboratories to detect the appearance of well-characterized HBV variants.

摘要

在本研究中,我们比较了通过序列分析和商业试剂盒检测乙型肝炎病毒(HBV)聚合酶、前核心(PC)及核心启动子突变所获得的结果。对23份来自接受拉米夫定治疗患者的血清样本,采用直接测序法、INNO-LiPA HBV DR和AFFIGENE HBV DE/3TC检测聚合酶突变。在所有分析的密码子中,63%的密码子在这三种检测方法间完全一致。在所有检测的密码子中,测序法与LiPA法结果一致的占80%,测序法与AFFIGENE法结果一致的占73%,LiPA法与AFFIGENE法结果一致的占74%。所有差异均出现在混合群体样本中,其中AFFIGENE和LiPA检测到序列未揭示的额外病毒变异体。在两名患者的系列样本中,LiPA比测序法和AFFIGENE更早检测到新出现的突变株。从14名HBV非活动携带者和14名慢性肝病乙型肝炎患者采集的28份血清样本中检测到PC和核心启动子病毒变异体。直接测序法、INNO-LiPA HBV PreCore和AFFIGENE HBV MUTANT VL 19在88%的检测位点显示出完全一致的结果。这些发现表明,所评估的所有检测方法都是分析HBV基因组变异性的灵敏且准确的工具。序列分析对于研究新出现的突变至关重要,因为LiPA和AFFIGENE检测方法在临床实验室中更便于检测特征明确的HBV变异体的出现。

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