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机构地区:[1]西安交通大学生物科学与工程研究所,西安 710049
出 处:《西安医科大学学报》2000年第6期512-514,共3页Journal of Xi'an Medical University(Chinese)
摘 要:目的 通过基因克隆技术获得饰胶蛋白基因cDNA克隆并表达。为研究饰胶蛋白的生物学功能及应用打基础。方法 应用PCR技术从T细胞cDNA文库获得饰胶蛋白全长基因cDNA片段 ,并克隆到pUC1 9载体中 ,采用Sanger双脱氧末端终止法测定全部cDNA序列 ,将测序正确的饰胶蛋白cDNA序列插入pGEX 4T 1表达载体中 ,经BamHI和EcoRI双酶切后 1 2 %凝胶电泳鉴定 ,IPTG诱导表达产物经SDS PAGE分析。结果 克隆的饰胶蛋白cDNA序列与GenBank中AF1 3830 0记载的序列完全一致 ,所表达的融合蛋白质分子量与理论计算值(65 6KD)也一致并为可溶性蛋白。结论 本研究成功地克隆了饰胶蛋白基因和表达了GSTObjective To study Decorin biological effects,Decorin gene cDNA was cloned and expressed in E.coli.Methods The Decorin gene obtained by PCR from T cell cDNA library and cloned into plasmid vector pUC19.The encoding sequence of Decorin in the pUC19 was confirmed by DNA sequencing using Sanger Dideoxy method,and then it was subcloned into expression plasmid vector pGEX 4T 1,the recombinant vector was indentified with BamHI and EcoRI in 1.2% agarose gel electrophoresis.The expression of Decorin fusion protein with GST in E.coli JM109 was induced with IPTG and identified by SDS PAGE.Results The PCR amplified DNA fragment shared identical sequence with known Decorin gene reported in GenBank(Accession number:AF138300).The SDS PAGE analysis revealed that the expressed fusion protein MW was approximatelly 65.6KD and in soluble format. Conclusion The cloned Decorin gene is correct and it was expressed in fusion protein with GST.
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