重组人β-catenin原核表达条件的优化及生物学活性鉴定

牛夏忆; 韩茂椿; 李淼; 陈云雨; 刘晓平

文章摘要

重组人β-catenin原核表达条件的优化及生物学活性鉴定

Optimization of Prokaryotic Expression Conditions and Biological Activity Identification of Recombinant Human β-Catenin

DOI：doi:10.3969/j.issn.1005-7021.2020.01.008

中文关键词: β-catenin 表达优化亲和层析荧光偏振酶联免疫吸附测定实验

英文关键词: β-catenin expression optimization affinity chromatography fluorescence polarization ELISA

基金项目:国家自然科学基金项目（81703546）；安徽省自然科学基金项目（1808085QH265)；安徽省高校自然科学研究重大项目（KJ2019ZD30）;吉林省科技发展计划项目（20160520045JH）；皖南医学院博士科研启动基金项目（RCQD201617）；皖南医学院大学生科研资助金项目（WK2018S54）

作者	单位
牛夏忆	皖南医学院药物筛选与评价研究所，安徽芜湖 241002
韩茂椿	皖南医学院药物筛选与评价研究所，安徽芜湖 241002
李淼	皖南医学院药物筛选与评价研究所，安徽芜湖 241002
陈云雨	皖南医学院药物筛选与评价研究所，安徽芜湖 241002
刘晓平	皖南医学院药物筛选与评价研究所，安徽芜湖 241002

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中文摘要:

优化重组人β-catenin（138-686 aa）在大肠埃希菌中的原核表达条件，经分离纯化后进行生物学活性鉴定。利用基因工程技术，将构建的重组质粒β-catenin-pET-30a(+)转化到Escherichia coli Rosetta(DE3)中，经IPTG诱导后进行β-catenin原核表达。为了提高β-catenin表达量，从诱导时间、诱导温度与IPTG诱导浓度3个单因素方面进行原核表达条件优化。β-catenin经HisTrap层析柱分离纯化后，以荧光偏振实验和酶联免疫吸附测定实验（enzyme-linked immunosorbent assay, ELISA）进行生物学活性鉴定。构建的工程菌经原核表达条件优化后，确定诱导温度25 ℃、诱导时间10 h、0.2 mmol/L IPTG作为β-catenin最佳原核表达条件。荧光偏振实验和ELISA实验说明，纯化的β-catenin具有良好的生物学活性。本研究成功进行了重组人β-catenin原核表达条件的优化与生物学活性鉴定，为深入研究β-catenin在肿瘤免疫抵抗中的生物学功能奠定了实验基础。

英文摘要:

Prokaryotic expression condition of recombinant human β-catenin (138 686 aa) in E.coli was optimized, and carried out biological characterization after isolation and purification. The constructed recombinant β-catenin pET-30a(+) plasmid was transformed into E. coli Rosetta (DE3) adopting genetic engineering technology and carried out prokaryotic expression of β-catenin after adopting IPTG induction. In order to enhance the expression amount of β-catenin, three single factors, induction time length, induction temperature, and IPTG induction concentration were carried out conditions optimization for prokaryotic expression. β-catenin was carried out characterization for biological activity after purification adopting HisTrap chromatographic column and ELISA determination. After the expression conditions optimization of the constructed prokaryotic engineered strain, the induction temperature was confirmed at 25 ℃, induction time at 10 h, and IPTG concentration at 0.2 mmol/L as the optimal conditions for prokaryotic expression. The experiment results of fluorescence polarization (FP) and ELISA showed that the purified catenin had fine bioactivity. This study successfully carried out the prokaryotic expression conditions optimization of the recombinant human β-catenin and characterized its bioactivity, and had laid the experimental foundation for further research on β-catenin in biological function for tumor immunity resistance.

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