生物学杂志

生物学杂志 ›› 2024, Vol. 41 ›› Issue (4): 112-.doi: 10.3969/j.issn.2095-1736.2024.04.112

• 技术方法 • 上一篇    下一篇

ERA实时荧光法快速检测乙肝病毒的建立与应用

翁兴墉1, 邹林涛1, 周 璇1, 唐红花2, 何 军3, 邓仲良1   

  1. 1. 南华大学 衡阳医学院 公共卫生学院, 衡阳 421001; 2. 南华大学衡阳医学院附属
    第一医院, 衡阳 421001; 3. 南华大学衡阳医学院附属南华医院 检验科, 衡阳 421001
  • 出版日期:2024-08-18 发布日期:2024-08-14
  • 通讯作者: 何军,博士,主任技师,研究方向为微生物快速检验,E-mail:junhe2008@163.com;邓仲良,博士,副教授,研究方向为病原菌分子诊断,E-mail:dzl021015@163.com;何军和邓仲良为共同通信作者
  • 作者简介:翁兴墉,硕士研究生,研究方向为病原菌分子诊断,E-mail:1442072975@qq.com
  • 基金资助:
    湖南省教育厅重点项目(21A0261); 湖南省自然科学基金项目(2022JJ30501)

Establishment and application of ERA real-time fluorescence method for rapid detection of hepatitis B virus

WENG Xingyong1, ZOU Lintao1, ZHOU Xuan1, TANG HongHua2, HE Jun3, DENG Zhongliang1   

  1. 1. School of Public Health, Hengyang Medical School, University of South China, Hengyang 421001, China;
    2. The First Affiliated Hospital of University of South China, Hengyang Medical School, University of South China,
    Hengyang 421001, China; 3. Department of Clinical Laboratory, the Affiliated Nanhua Hospital, Hengyang Medica
    School, University of South China, Hengyang 421001, China
  • Online:2024-08-18 Published:2024-08-14

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摘要: 基于酶促重组等温扩增(ERA)技术构建一种快速检测乙肝病毒的实时荧光检测方法。根据乙肝病毒聚合酶编码区(P区)保守序列设计引物和探针,对引物、温度、荧光探针浓度等反应条件进行优化,建立ERA实时荧光法最佳反应体系,再对其敏感性、特异性、抗干扰能力、临床样本检出效果进行验证。结果显示:ERA实时荧光法在42 ℃、20 min内可完成对乙肝病毒的检测,最低检出限为102copies/μL;除乙肝病毒外,其他4种病毒(甲肝病毒、丙肝病毒、EB病毒、巨细胞病毒)均未产生荧光扩增曲线,具有良好的特异性和抗干扰能力;以实时荧光PCR法检测结果为标准,ERA实时荧光法检测58份乙肝病毒临床样本的灵敏度为97.37%、特异度为100%、阴性预测值为95.24%、阳性预测值为100%、Kappa值为0.96。成功建立了一种简单、快速、灵敏、特异、低成本的乙肝病毒早期检测方法,满足乙肝病毒快速检测的需要。

关键词: 酶促重组等温扩增技术, 快速检测, 乙肝病毒, ERA实时荧光法, 早期诊断

Abstract: This study is to establish a real-time fluorescence detection method for rapidly detecting the hepatitis B virus using enzyme recombinase amplification (ERA) technology. The primers and probes were designed according to the conserved sequence of the polymerase coding region (P region) of the hepatitis B virus, and the reaction conditions, such as primers, temperature, and fluorescent probe concentration, were optimized to establish the optimal reaction system of the ERA real-time fluorescence assay, which was further validated in terms of sensitivity, specificity, anti-jamming capacity, and clinical samples. The results showed that the ERA real-time fluorescence method could detect the presence of the hepatitis B virus within 20 minutes at 42 ℃, with a limit of detection of 102copies/μL. The other four viruses (hepatitis A virus, hepatitis C virus, Epstein-Barr virus, and Cytomegalovirus) did not show fluorescence amplification curves, indicating reasonable specificity and anti-interference ability. When compared to the real-time fluorescence PCR method, the ERA real-time fluorescence method for 58 hepatitis B virus clinical samples exhibited a sensitivity of 97.37%, a specificity of 100%, a negative predictive value of 95.24%, a positive predictive value of 100%, and Kappa value of 0.96. This study successfully established a simple, rapid, sensitive, specific, and low-cost method for early detection of hepatitis B virus to meet the need for rapid detection.

Key words: enzymatic recombinase amplification (ERA) technology, rapid detection, hepatitis B virus, the ERA real-time fluorescence method, early diagnosis

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