生物技术通报 ›› 2014, Vol. 0 ›› Issue (9): 178-184.

• 研究报告 • 上一篇    下一篇

人源CD137L基因在不同表达系统中表达效率的比较

何东洋,马超,高振月,王淑珍,陈依军   

  1. 中国药科大学生命科学与技术学院,南京 210009
  • 收稿日期:2014-03-18 出版日期:2014-09-15 发布日期:2014-09-07
  • 作者简介:何东洋,男,博士研究生,研究方向:肿瘤免疫;E-mail:hedongyang1983@163.com
  • 基金资助:
    天然药物活性组分与药效国家重点实验室(中国药科大学)资助项目(JKGQ201105)

The Comparison of Expression Efficiency of Human CD137L in Different Expression System

He Dongyang,Ma Chao,Gao Zhenyue,Wang Shuzhen,Chen Yijun   

  1. College of Life Science and Technology,China Pharmaceutical University,Nanjing 210009
  • Received:2014-03-18 Published:2014-09-15 Online:2014-09-07

摘要: 比较分析人源CD137L在毕赤酵母、枯草杆菌及大肠杆菌中的表达差异,建立适合CD137L的表达系统并检测CD137L的生物学活性。设计PCR引物,以酵母表达质粒pPIC9K-CD137L为模板,扩增CD137L片段,分别构建枯草杆菌表达质粒及大肠杆菌表达质粒,再转化至相应的宿主菌并筛选阳性转化子;SDSPAGE电泳分析CD137L的表达情况并比较差异;稀释复性法复性CD137L包涵体,用离子交换层析纯化CD137L;T细胞激活试验检测CD137L的活性。CD137L在3个表达系统中均可以表达并且得到质谱鉴定,但是在毕赤酵母、枯草杆菌中的表达量微弱,而在大肠杆菌中CD137L以包涵体形式高效表达,平均1L培养液能得到0.8g包涵体沉淀,200mg变性蛋白。经复性纯化后得到的CD137L能有效激活T细胞增殖并且其刺激活性呈现浓度依赖效应。与毕赤酵母、枯草杆菌相比,大肠杆菌表达系统能高效表达CD137L蛋白,并且经稀释复性后CD137L保持了刺激小鼠T细胞增殖的活性。

关键词: 毕赤酵母, 枯草杆菌, 大肠杆菌, CD137L, T细胞增殖

Abstract: It was to construct a suitable expression system for CD137L by comparison of expression level of CD137L in Pichia yeast, Bacillus subtilis, and Escherichia coli and determine the effect of CD137L on T cell proliferation. CD137L was amplified by PCR with designed primers from yeast expression plasmid pPIC9K-CD137L and subcloned into vector pP43 or pET11a. Then recombinant plasmid pPIC9K-CD137L, pP43-CD137L and pET11a-CD137L were transformed into GS115, WB800 and BL21, respectively. Positive clones were screened and expression of CD137L was detected by SDS-PAGE. Then inclusion body of CD137L from Escherichia coli was refolded by dilute refolding and CD137L was purified by ion exchange chromatography. After that, bioactivity of CD137L was determined by T cell proliferation assay. CD137L was expressed by all the three expression system and further confirmed by Western blot assay. But expression level of CD137L in GS115 and WB800 was too weak for further study. In contrast, CD137L was efficiently expressed in BL21 as inclusion body. It was about 0.8 g inclusion body per 1 L cultured BL21 and 200 mg denatured protein was obtained. Then inclusion body was dissolved in 8 mol/L urea at 50℃or 60℃, and active protein CD137L was obtained after dilute refolding. Then refolded CD137L was purified by ion exchange chromatography, and purified CD137L demonstrated significantly costimulatory effect on T cell proliferation in dose-dependent manner. It was demonstrated that CD137L was efficiently expressed in Escherichia coli expression system compared with Pichia yeast and Bacillus subtilis, and purified CD137L kept costimulatory activity on T cell proliferation.

Key words: Pichia pastoris, Bacillus subtilis , Escherichia coli, CD137L , T cell proliferation