Cloning Expression and Purification of Shiga Toxin B Subunit Gene in E.coli

Yu Huaying1 Gao Feng2 Jia Guizheng1 Wu Donglin2 (1 Taremu Agricultural University of Xingjiang, Alar 843300) (2 Department of Animal Sciences, Quartermaster University of PLA,Changchun 130062)

Shiga toxin B;Cloning expression;purification

Objective To express the ShT-B gene fragment in E.coli. Methods pGEM-ShTB 3 cloning vector and prokaryotic pQE-30 expression vector were respectively digested with the endonucleases KpnⅠand Hind Ⅲ, and then the small fragment of ShT-B and the large fragment of linearized pQE-30 were ligated under T4 DNA ligase, resulted in recombinant vector, named as pQE30-ShTB 2,The resulting expression vector pQE30-ShTB 2 was selected and identified by the colony-PCR and endonucleases digestion, finally expressed in E.coli M15 cell. Results The transgenetic strain E.coli M15 with pQE30-ShTB 2can expressed an ShT-B recombinant protein induced by IPTG. SDS-PAGE showed the size of expressed recombinant protein was similar with ShT-B molecular weight in 10KD, and the target fusion protein occupied 16% of total cell protein and the cell supernatant is occupied 9.2%