生物技术通报 ›› 2016, Vol. 32 ›› Issue (5): 107-113.doi: 10.13560/j.cnki.biotech.bull.1985.2016.05.014

• 研究报告 • 上一篇    下一篇

红鳍东方鲀(Takifugu rubripes)干扰素调节因子2基因的克隆及原核表达

孙赛红12, 马普2, 孙鹤2, 孔德荣2, 李慧2, 仇雪梅2, 姜志强1, 刘海映3, 刘洋2, 刘圣聪4, 孟雪松4, 王秀利12   

  1. 1. 大连海洋大学 农业部北方海水增养殖重点实验室,大连 116023;
    2. 大连海洋大学水产与生命学院,大连 116023;
    3. 大连海洋大学海洋科技与环境学院,大连 116023;
    4. 大连天正实业有限公司,大连 116011
  • 收稿日期:2015-05-25 出版日期:2016-05-25 发布日期:2016-05-27
  • 作者简介:孙赛红,女,硕士,E-mail:sun.saihong@163.com
  • 基金资助:
    国家海洋公益性行业科研专项经费项目(201405003-2),大连市科技计划项目(2014B11NC091)

Cloning and Prokaryotic Expression of Interferon Regulatory Factor 2 from Takifugu rubripes

SUN Sai-hong12,MA Pu2,SUN He2,KONG De-rong2,Li Hui2,QIU Xue-mei2,JIANG Zhi-qiang1,LIU Hai-ying3,LIU Yang2   

  1. 1. Key Laboratory of Mariculture &Stock Enhancement in North China’s Sea,Ministry of Agriculture,Dalian Ocean University,Dalian 116023;
    2. College of Fisheries and Life Science,Dalian Ocean University,Dalian 116023;
    3.College of Marine Science and Environment,Dalian Ocean University,Dalian 116023;
    4. Dalian Tianzheng Industrial Co. Ltd.,Dalian 116011
  • Received:2015-05-25 Published:2016-05-25 Online:2016-05-27

摘要: 干扰素调节因子(Interferon regulatory factor,IRF)是一种多功能的转录因子。采用反转录聚合酶链式反应(RT-PCR)和cDNA末端快速扩增(RACE)技术克隆了红鳍东方鲀干扰素调节因子2(Interferon regulatory factor 2,IRF2)基因的全长cDNA。该基因全长为1 552 bp,其中5'非编码区(5'-UTR)187 bp,3'非编码区(3'-UTR)429 bp,编码区(CDS)为936 bp,共编码311个氨基酸。将IRF2的编码区序列连接到原核表达载体pET32a(+),成功构建了重组体pET32a(+)-IRF2。将重组体pET32a(+)-IRF2转入大肠杆菌感受态细胞BL21(DE3)中,获得了重组表达IRF2的基因工程菌。经IPTG诱导,pET32a(+)-IRF2在BL21中得到了融合表达。通过对表达产物的纯化和Western blotting检测,结果显示红鳍东方鲀IRF2基因在大肠杆菌中的表达效果较高,目的蛋白准确。

关键词: 红鳍东方鲀, 干扰素调节因子2, cDNA末端快速扩增, 原核表达

Abstract: Interferon Regulatory Factor(IRF)is a transcription factor with multifunctions. The full length cDNA of Takifugu rubripes interferon regulatory factor 2(IRF2)was cloned by RT-PCR and rapid amplification of cDNA ends(RACE). The full-length cDNA of the gene was 1 552 bp,including a 187 bp 5' non-coding region,a 429 bp 3' non-coding region,and 936 bp coding region,and it encoded 311 amino acids. The recombinant pET32a(+)-IRF2 was constructed by ligating code sequence of IRF2 with prokaryotic expression vector pET32a(+). Then,the recombinant genetic engineering bacteria with expressed IRF2 were obtained by transforming pET32a(+)-IRF2 into competent cell Escherichia coli BL21(DE3). pET32a(+)-IRF2 was expressed in BL21 under the induction of IPTG. The results from the detection of the purified products by Western blotting showed that the expression of the IRF2 gene in E. coli was high,and the target protein was accurate.

Key words: Takifugu rubripes, interferon regulatory factor 2, rapid amplification of cDNA end, prokaryotic expression