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作 者:高云鹏[1] 赵雨[1] 王新宇 白雪媛[1] 王佳雯[1] GAO Yun-peng;ZHAO Yu;WANG Xin-yu;BAI Xue-yuan;WANG Jia-wen(Traditional Chinese Medicine and Biotechnology Research and Development Center,Changchun University of Chinese Medicine,Changchun 130117,China)
机构地区:[1]长春中医药大学中医药与生物工程研究开发中心,长春130117
出 处:《科学技术与工程》2018年第17期141-144,共4页Science Technology and Engineering
基 金:吉林省科技发展计划(20140622003JC)资助
摘 要:在毕赤酵母X33中表达人表皮生长因子并纯化,对表皮生长因子(EGF)进行密码子优化,构建pPICZa A-EGF真核表达质粒,转化X33感受态细胞;利用抗性筛选以及PCR鉴定阳性菌株。经过甲醇诱导和镍柱纯化,聚丙烯酰胺凝胶电泳检测蛋白分泌表达情况。成功构建了表达pPICZa A-EGF真核表达质粒,转入X33中获得阳性菌株,成功诱导蛋白分泌表达并纯化。在毕赤酵母X33中成功表达人表皮生长因子,纯化后纯度为80%,收率为5.8 mg/L。Objective expression and purification of human epidermal growth factor in Pichia pastoris X33,methods egf was codon-optimized to construct pPICZa A-EGF eukaryotic expression plasmid and transformed into competent cells of X33. Positive strains were identified by resistance screening and PCR. After methanol induction and nickel column purification,SDS-PAGE was used to detection of protein secretion. The eukaryotic expression plasmid pPICZa A-EGF was successfully constructed and transformed into X33 to obtain a positive strain,which was successfully induced to express and purify protein. Human epidermal growth factor was successfully expressed in Pichia pastoris X33. The purity of purified protein was 80% with a yield of 5. 8 mg/L.
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