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机构地区:[1]南方医科大学生物技术学院输血医学系,广州510515 [2]南方医科大学南方医院消化科,广州510515
出 处:《第三军医大学学报》2009年第7期589-591,共3页Journal of Third Military Medical University
基 金:国家重点基础研究发展计划(973计划)(2007CB512901);广东省自然科学基金(06105111);广东省科技攻关计划(0700016)~~
摘 要:目的以磷酸酰肌醇蛋白聚糖-3蛋白(glypican-3,GPC3)的CTL表位EYILSLEEL替换HBsAg中内源性CTL表位LLD,构建用于预防和治疗乙肝的DNA疫苗。方法以重组表面抗原基因pcHBsAg质粒为模板,应用重叠延伸PCR扩增出含EYILSLEEL表位的HBsAg基因HBsAg/GPC3,将其插入pBSSK+载体中,构建出pBSSK/GPC3载体。利用DNA重组技术将其定向插入真核表达载体pcDNA3.1+中,将真核表达载体经PCR、酶切和测序鉴定,构建表达CTL表位EYILSLEEL的DNA疫苗。结果酶切和测序的结果显示序列无错配,获得了完整表达EYILSLEEL表位的真核质粒pcDNA3-HBsAg/GPC3。结论成功将EYILSLEEL表位替换HBsAg的内源性CTL表位,构建了pcDNA3-HBsAg/GPC3真核表达质粒。Objective To replace the endogenous CTL epitope LLD in HBsAg with EYILSLEEL of glypican (GPC3) in order to prepare a GPC3-HBsAg multiple peptides vaccine for HBV infection. Methods The HBsAg/GPC3 DNA was amplified by gene splicing by overlap extension (SOEing) PCR from peHBsAg plasmid and then inserted into pBSSK + vector to construct a pBSSK/GPC3 vector. The vector was then identified by PCR, double digesting and sequencing. The fragment encoding GPC3 CTL epitope EYILSLEEL was obtained by double digesting the plasmid pBSSK/GPC3 and then inserted into pcDNA3. 1 + vector. Results Sequencing and restrict endonulease digestion indicated that eukaryotic expression vector pcDNA- HBsAg/GPC3 was constructed successfully. Conclusion The endogenous CTL epitope LLD of HBsAg is replaced by the EYILSLEEL, and an eukaryotic expression vector pcDNA-HBsAg/GPC3 is constructed.
关 键 词:表位替换 磷酸酰肌醇蛋白聚糖-3蛋白 细胞毒T淋巴细胞表位 重叠延伸PCR
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