Eukaryotic expression and serodiagnostic potential of HIV-1 p24 antigen

Q4 Immunology and Microbiology

中华微生物学和免疫学杂志 Pub Date : 2019-08-31 DOI:10.3760/CMA.J.ISSN.0254-5101.2019.08.005

Wei-Zheng Song, Xiangyu Chen, Y. Shao, Y. Hao, Ying Wang

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引用次数: 0

Abstract

Objective To express HIV-1 capsid p24 antigen in an eukaryotic expression system and to evaluate its antigenicity and potential in the early diagnosis of HIV. Methods The full-length gene of HIV-1 p24 and the signal peptide DRVI gene were amplified by PCR. The signal peptide DRVI preceding the p24 gene was introduced using fusion PCR, and cloned into vector pDRVI1.0. Two recombinant plasmids pDRVI-p24 and pDRVI-p24s were constructed and transfected into 293F cells. Expression and secretion of p24 protein were detected by SDS-PAGE, Ni-NTA column chromatography and molecular sieve were used to purify p24s protein. The purified protein was identified by Western blot and indirect ELISA using human/mouse HIV-1-positive serum samples. Results The eukaryotic expression system for HIV-1 p24 antigen was successfully established with high efficiency. The target protein of interest with the signal peptide DRVI was obviously detected in the supernatants of cell culture. The recombinant protein had good specificity and sensitivity based on the results of serological tests using serum samples of five HIV-1-positive and five HIV-negative mice, 30 HIV-1-positive patients and 50 HIV-1-negative healthy individuals. Conclusions The eukaryotic expression system for HIV-1 p24 antigen was successfully established. The purified HIV-1 p24s antigen had good antigenicity. An indirect ELISA assay with good specificity and sensitivity for the detection of HIV-1 was preliminarily constructed and showed great potential for application. Key words: HIV-1; p24 core antigen; Eukaryotic expression; Serological diagnosis

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hiv - 1p24抗原的真核表达和血清诊断潜力

目的在真核表达系统中表达HIV-1衣壳p24抗原，评价其抗原性及其在HIV早期诊断中的应用价值。方法采用PCR扩增HIV-1 p24全长基因和信号肽DRVI基因。采用融合PCR法将p24基因前的信号肽DRVI导入到pDRVI1.0载体中。构建重组质粒pDRVI-p24和pDRVI-p24s，并转染293F细胞。采用SDS-PAGE检测p24蛋白的表达和分泌情况，采用Ni-NTA柱层析和分子筛分离纯化p24s蛋白。利用人/小鼠hiv -1阳性血清样品，采用Western blot和间接ELISA方法对纯化蛋白进行鉴定。结果成功建立了HIV-1 p24抗原的真核表达体系。在细胞培养的上清液中明显检测到与信号肽DRVI相关的目标蛋白。利用5只hiv -1阳性和5只hiv -1阴性小鼠、30例hiv -1阳性患者和50例hiv -1阴性健康人的血清样本进行血清学检测，结果表明重组蛋白具有良好的特异性和敏感性。结论成功建立了hiv - 1p24抗原真核表达体系。纯化的HIV-1 p24s抗原具有良好的抗原性。初步构建了一种特异性和敏感性较好的间接ELISA检测HIV-1的方法，具有较大的应用潜力。关键词:HIV-1;P24核心抗原;真核表达;血清学诊断

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来源期刊

中华微生物学和免疫学杂志 Immunology and Microbiology-Virology

CiteScore

0.50

自引率

0.00%

发文量

6906

期刊介绍： Chinese Journal of Microbiology and Immunology established in 1981. It is one of the series of journal sponsored by Chinese Medical Association. The aim of this journal is to spread and exchange the scientific achievements and practical experience in order to promote the development of medical microbiology and immunology. Its main contents comprise academic thesis, brief reports, reviews, summaries, news of meetings, book reviews and trends of home and abroad in this field. The distinguishing feature of the journal is to give the priority to the reports on the research of basic theory, and take account of the reports on clinical and practical skills.