EGFR基因19外显子del18bp突变检测技术平台的构建及优化

基础医学与临床 ›› 2021, Vol. 41 ›› Issue (10): 1491-1496.

EGFR基因19外显子del18bp突变检测技术平台的构建及优化

蒋艳芳, 谭黎, 向花花, 文小莎, 郭紫芬^*

南华大学药物药理研究所湖南省分子靶标新药研究协同创新中心湖南省肿瘤微环境响应药物研究重点实验室, 湖南衡阳 421001

收稿日期:2020-10-15 修回日期:2021-04-09 发布日期:2021-09-29
通讯作者: *guozifen76@163.com
基金资助:
湖南省教育厅重点项目(19A419);教育部大学生创新创业训练计划项目(S202010555069);南华大学大学生创新创业训练计划项目(X2019183)

Construction and optimization of detection technology platform for EGFR gene exon 19 del18bp mutation

JIANG Yan-fang, TAN Li, XIANG Hua-hua, WEN Xiao-sha, GUO Zi-fen^*

Hunan Province Cooperative Innovation Center for Molecular Target New Drug Study, Hunan Provincial Key Laboratory of Tumor Microenvironment Responsive Drug Research, Institute of Pharmacy and Pharmacology, University of South China, Hengyang 421001, China

Received:2020-10-15 Revised:2021-04-09 Published:2021-09-29
Contact: *guozifen76@163.com

摘要/Abstract

摘要： 目的构建高保真酶介导的EGFR基因19外显子del18bp的突变敏感性分子开关检测平台,并对其进行优化。方法以健康人全血基因组DNA为模板,利用普通PCR与重叠PCR技术扩增分别得到包含EGFR基因19外显子del18bp的野生型和突变型DNA片段,并将其插入pMD19-T质粒,转化大肠埃希菌E.coli DH5α,通过菌液PCR及基因组测序进行鉴定。设计EGFR基因19外显子del18bp突变型特异性检测引物,并在3′端进行硫化修饰;用高保真聚合酶进行双向引物延伸。通过正交实验方案对高保真酶介导的PCR体系中的退火温度、引物浓度、模板浓度、循环数等条件进行优化,建立突变敏感性分子开关检测平台。结果成功建立了EGFR基因19外显子del18bp突变检测技术平台。分子开关技术检测EGFR基因19外显子del18bp突变位点的最佳PCR条件为:模板浓度1.48×10^-2 μmol/L,引物浓度0.16 μmol/L,退火温度57 ℃,循环数25;对突变模板的最低检出率为10^-3copies/μL。结论高保真聚合酶偶联硫化修饰构成的突变敏感性分子开关技术可望为肺癌患者实施EGFR基因突变检测,进行个体化靶向用药提供新的技术手段。

关键词: 肺癌, 表皮生长因子受体(EGFR), 高保真聚合酶, 分子开关

Abstract: Objective To construct and optimize a high-fidelity polymerase-mediated mutation sensitive molecular switch technique platform for detecting exon 19 del18bp of EGFR gene. Methods Using genome DNA from a healthy volunteer as PCR template, the wild-type and mutant-type DNA fragment containing mutation site were amplified by common PCR and overlap PCR respectively, which then were connected with the vector pMD19-T. The constructed wild-type and mutant-type recombinant plasmid was transformed into competent cells E.coli DH5α further appraised by bacteria solution PCR and genome sequencing. The mutation-specific upstream detection primer was designed with 3′phosphorothioate modification, and two-directional primers extension was performed using high- fidelity polymerase. The annealing temperature, primer concentration, template concentration, cycle number, and other high-fidelity polymerase-mediated PCR conditions were all optimized through an orthogonal test protocol to establish a molecular switch detection platform for exon 19 del18bp of EGFR gene. Results The molecular switch detection platform for exon 19 del18bp of EGFR gene was successfully established. The optimal PCR condition of detecting EGFR gene exon 19 del18bp using mutation-sensitive molecular switch technique was as follows: 57 ℃ optimal annealing temperature, 0.16 μmol/L primer concentration, 1.48×10^－2 μmol/L template concentration and 25 PCR cycles. And the allele-specific primer for del18bp can detect the perfectly matched template at a sensitivity of about 10^－3 μmol/L. Conclusions Mutation-sensitive molecular switch technology composed of high-fidelity polymerase with 3′ phosphorothioate-modified prime provides a new technology which can implement EGFR mutation test for personalized targeted meditation for treatment of lung cancer.

Key words: lung cancer, epidermal growth factor receptor(EGFR), high-fidelity polymerase, molecular switch

中图分类号:

蒋艳芳, 谭黎, 向花花, 文小莎, 郭紫芬. EGFR基因19外显子del18bp突变检测技术平台的构建及优化[J]. 基础医学与临床, 2021, 41(10): 1491-1496.

JIANG Yan-fang, TAN Li, XIANG Hua-hua, WEN Xiao-sha, GUO Zi-fen. Construction and optimization of detection technology platform for EGFR gene exon 19 del18bp mutation[J]. Basic & Clinical Medicine, 2021, 41(10): 1491-1496.

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