RUNX3全长和不同结构域原核表达载体的构建及其重组蛋白表达

doi:10.7694/jldxyxb20130606

Abstract

Abstract:

Abstract:Objective
To construct the prokaryotic expression vectors of overall length and different domains of RUNX3 and to identify the expressions of their recombinant proteins.Methods The coding sequence of overall length and different domain truncations of RUNX3 were amplified from the pcDNA3.1-myc-RUNX3 plasmid by PCR method and inserted into glutathione transferase(GST) fusion expression vector pGEX-4T-2 through EcoRⅠand BamHⅠ restriction enzyme sites.Then they were transformed into E.coli BL21 and the fusion proteins were induced and identified by SDS-PAGE electrophoresis.Results The vector fragments FL (1 245 bp),ΔRunt(843 bp),Nter(159 bp),Runt(402 bp), and Cter (684 bp) which were consistent with the expected fragments were obtained after double enzyme digestion of EcoRⅠand BamHⅠ.The SDS-PAGE electrophoresis result showed that the relative molecular mass of GST-RUNX3 truncated fusion proteins of overall length and different domains of RUNX3 (GST-FL,GST-Runt,GST-Nter and GST-Cter)were 72 000,40 000,32 000, and 51 000,respectively.Conclusion GST-tagged prokaryotic expression vectors overall length and different truncated regions of RUNX3 are constructed and their recombinant proteins are expressed successfully.

Key words: RUNX3, vector, inducing of protein, expression of protein

CLC Number:

SONG Yan-yan，WANG Gui-ling. Construction of prokaryotic expression vector of overall length and different domains of RUNX3 and expressions of their recombinant proteins[J].Journal of Jilin University Medicine Edition, 2013, 39(6): 1112-1115.

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Construction of prokaryotic expression vector of overall length and different domains of RUNX3 and expressions of their recombinant proteins

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