人跨膜蛋白39A原核表达载体构建、条件优化及可溶性表达

基础医学与临床 ›› 2019, Vol. 39 ›› Issue (7): 932-936.

人跨膜蛋白39A原核表达载体构建、条件优化及可溶性表达

李向茸¹,马瑞仙²,李倩¹,王兴陇²,李生军³,张海霞¹,冯若飞¹

1. 西北民族大学
2. 西北民族大学生命科学与工程学院
3. 甘肃省兰州市城关区西北新村1号西北民族大学生物医学研究中心

收稿日期:2018-08-15 修回日期:2018-12-03 出版日期:2019-07-05 发布日期:2019-07-02
通讯作者: 冯若飞 E-mail:fengruofei@xbmu.edu.cn
基金资助:
国家自然基金项目;2018年中央高校基本科研业务费资金项目;教育部“创新团队发展计划”项目;西北民族大学“双一流”引导专项生物工程特色学科

Construction of prokaryotic expression vector, optimization of expression conditions and soluble expression of human TMEM39A

Received:2018-08-15 Revised:2018-12-03 Online:2019-07-05 Published:2019-07-02
Contact: ruofei ruofeiFeng E-mail:fengruofei@xbmu.edu.cn

摘要/Abstract

摘要： 目的构建人跨膜蛋白39A基因（TMEM39A）的原核表达载体，优化表达条件并获得可溶性表达的TMEM39A。方法以HEK293细胞的总RNA为模板，反转录PCR扩增TMEM39A，构建其原核表达载体pGEX-6P-1-TMEM39A，并在不同温度、IPTG浓度、A600nm值及时间条件进行诱导表达，然后利用上述获得的最佳诱导条件进行大量表达，分析其可溶性和抗原性。结果重组表达载体pGEX-6P-1-TMEM39A与GenBank中的TMEM39A（登录号：BC021277.2）的核苷酸序列同源性为99.9 %，氨基酸序列同源性为100 %。重组蛋白GST-TMEM39A在69 ku和60 ku处出现两条特异性条带，采用单因素方法对不同温度、IPTG浓度、A600nm值及时间进行分析得出GST-TMEM39A的最佳诱导条件为25 ℃、A600nm值为0.6、IPTG浓度为0.05 mmol/L诱导6 h；在此基础上进行大量表达，并以可溶性形式获得了TMEM39A与GST蛋白的融合表达。结论成功构建了TMEM39A的原核表达载体，确定了GST-TMEM39A的最佳表达条件并实现其的可溶性表达，为后续纯化TMEM39A、制备抗体开展功能研究奠定物质基础，并为深入探讨TMEM39A与许多疾病或病毒的关系提供科学依据。

关键词: 跨膜蛋白39A, 生物信息学分析, 融合蛋白, 条件优化, 可溶性表达

Abstract: Objective To construct prokaryotic expression vector of human TMEM39A, optimize expression conditions and obtain soluble TMEM39A. Methods TMEM39A gene was amplified from HEK293 cells total RNA by RT-PCR to construct its prokaryotic expression vector pGEX-6P-1-TMEM39A, and induced expression was conducted at different temperatures, IPTG concentrations, A600nm values and time conditions. Finally, expression of the recombinant protein GST-TMEM39A abundantly were carried out to analyze its solubility and antigenicity by using the best induction conditions. Results The nucleotide sequence homology of the recombinant expression vector pGEX-6P-1-TMEM39A and TMEM39A in GenBank (BC021277.2) was 99.9 % and the amino acid sequence homology was 100 %. The recombinant protein GST-TMEM39A showed two specific bands at 69 ku and 60 ku by Western blot analysis. The optimal induction conditions for GST-TMEM39A was 25 ℃, A600nm value of 0.6, 0.05 mmol/L IPTG induced 6 h. On this basis, the fusion expression of TMEM39A and GST protein was obtained in a soluble form. Conclusions The prokaryotic expression vector of TMEM39A is successfully constructed, the optimal expression condition of GST-TMEM39A is determined and its soluble expression is realized, which lay a material foundation for the subsequent purification of TMEM39A and the preparation of antibodies for functional studies, and provide scientific basis for further study about the relationship between TMEM39A and many diseases or viruses.

Key words: Transmembrane protein 39A (TMEM39A), Bioinformatics analysis, Fusion protein, Optimization of expression conditions, Soluble expression

李向茸马瑞仙李倩王兴陇李生军张海霞冯若飞. 人跨膜蛋白39A原核表达载体构建、条件优化及可溶性表达[J]. 基础医学与临床, 2019, 39(7): 932-936.

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