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作 者:王艳茹[1] 任宏伟[1] 纪建国[1] 李令媛[1] 茹炳根[1]
机构地区:[1]北京大学
出 处:《化学学报》2001年第10期1813-1817,共5页Acta Chimica Sinica
摘 要:利用基因工程方法在大肠杆菌-酵母穿梭质粒pPIC9K上构建了人三叶因子3(Human Trefoil Factor 3,hTFF3)双结构域突变体基因,采用毕氏酵母表达系统对目的基因进行了分泌表达.经S-Sepharose,Q-Sepharose,SephacrylS-100纯化后得到突变体蛋白,主要以单体形式存在.SDS-PAGE表明重组蛋白分子量约为12 000,并在Westernblotting印迹实验中证明能被抗hTFF3抗体所识别,N-端氨基酸测序与天然hTFF3一致,质谱检测纯化的蛋白出现单体和双本两种形式.用重组蛋白对乙醇诱导的大鼠胃溃疡进行实验治疗表明hTFF3双体突变体与天然形成的双本蛋同具有相同的活力,并且活力高于单体形式的hTFF3.Double - trefoil domain mutant of human trefoil factor 3 (hTFF3) was constructed through gene engineering and inserted into the pPIC9K plasmid, then expressed in the methylotrophic yeast Pichia pastoris. The recombinant protein was purified through S - Sepharose, Q - Sepharose and Sephacryl S - 100. Molecular weight of the expressed protein was about 12 000 identified by SDS - PAGE and Western - blotting. N - terminal amino acid analyses proved that the expressed hTFF3 dimeric form mutant was identical to the native N - terminus. Two protein peaks corresponding to the monomeric and dimeric form of Di - hTFF3 mutant were identified by the mass spectrometry. The boiactivity of the mutant was the same as the native dimeric form of hTFF3, and higher than that of the monomeric mutant.
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