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乙肝表面抗原(HBsAg)突变体的检测

Detection of HBsAg mutants.

作者信息

Osiowy Carla

机构信息

Bloodborne Pathogens and Hepatitis, National Microbiology Laboratory, Public Health Agency of Canada, Winnipeg, Manitoba, Canada.

出版信息

J Med Virol. 2006;78 Suppl 1:S48-51. doi: 10.1002/jmv.20607.

DOI:10.1002/jmv.20607
PMID:16622877
Abstract

HBsAg screening is carried out routinely to detect hepatitis B virus (HBV) infection. The immunoassays used employ capture antibodies often having specificity for epitopes present on the antigenic (a) determinant of the HBsAg. Loss of detection may occur due to mutations within and/or outside of the a determinant that affect conformational epitope recognition or HBsAg secretion or expression. Most of the mutations associated with immune escape occur within the second loop of the a determinant. In order to detect these HBsAg mutants, antibodies to subdominant regions within the a determinant or outside of the HBsAg may be required, and this has been the focus of many recent studies. Any changes to immunoassay formulations should also address the possible effect of HBV genotypic polymorphisms on assay specificity and sensitivity. HBsAg mutants may also be identified through nucleic acid detection of HBV in serum. Various molecular analysis methods have been developed to provide specific and sensitive detection of HBsAg mutants, including sequencing, limiting dilution cloning PCR (LDC-PCR), gap ligase chain reaction (gLCR), and real time PCR. Sequencing the HBsAg coding region provides specific information on the nucleotide sequence; however, it is relatively insensitive for the detection of minority quasispecies. Other nucleic acid methods offer greater sensitivity for the detection of point mutations. To improve immunoassays, further research will be required to increase detection sensitivity and specificity. Ultimately, a better understanding of the structure of antibody-bound HBsAg will help identify the immunological targets required for the accurate detection of HBsAg in blood.

摘要

常规进行乙肝表面抗原(HBsAg)筛查以检测乙型肝炎病毒(HBV)感染。所使用的免疫测定法采用捕获抗体,这些抗体通常对HBsAg抗原性(a)决定簇上存在的表位具有特异性。由于a决定簇内部和/或外部的突变影响构象表位识别或HBsAg分泌或表达,可能会出现检测失败的情况。大多数与免疫逃逸相关的突变发生在a决定簇的第二个环内。为了检测这些HBsAg突变体,可能需要针对a决定簇内或HBsAg外部的亚显性区域的抗体,这一直是最近许多研究的重点。免疫测定法配方的任何变化也应考虑HBV基因多态性对测定特异性和敏感性的可能影响。HBsAg突变体也可以通过血清中HBV的核酸检测来鉴定。已经开发了各种分子分析方法来提供对HBsAg突变体的特异性和灵敏检测,包括测序、有限稀释克隆PCR(LDC-PCR)、缺口连接酶链反应(gLCR)和实时PCR。对HBsAg编码区进行测序可提供有关核苷酸序列的具体信息;然而,它对少数准种的检测相对不敏感。其他核酸方法对检测点突变具有更高的灵敏度。为了改进免疫测定法,需要进一步研究以提高检测灵敏度和特异性。最终,更好地了解抗体结合的HBsAg的结构将有助于确定准确检测血液中HBsAg所需的免疫靶点。

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