大鼠热休克因子结合蛋白1原核表达载体的构建及表达

以重组克隆载体pGEM—T—hsbp1为模板,PCR扩增hsbp1,用限制性内切酶双酶切、T4连接酶连接、转化BL -21的方法构建pGEX-2TK-hsbp1原核表达载体,实现了hsbp1在BL21中的表达,SDS—PAGE检测表达的融合蛋白主要以可溶形式存在,并利用亲和层析得到融合蛋白。

Construction of pGEX-2TK-Hsbp1 Prokaryotic Expression Vector and Expression of HSBP1

Using recombination cloning plasmid pGEM-T-hsbp1 as template,heat shock factor binding protein gene was cloned;By restriction endonuclease,T4 DNA ligase,BL-21,the pGEX-2TK-hsbpl prokaryotic expression vector was constructed.The recombinant expression vector can express fusion proteins of recombinant HSBP1 in BL21.The result of SDS-PAGE manifests that the target protein was expressed in soluble form.We obtained target protein by affinity chromatography.