人源性肝细胞生长因子稳定转染细胞株的建立(英文)  被引量:3

Building of stably transfected cell strain on human hepatocyte DNA synthetic stimulating factor

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作  者:唐世刚[1] 覃琼华[2] 罗育林[3] 苏先狮[4] 

机构地区:[1]中南大学湘雅三医院感染病科,湖南长沙410013 [2]中南大学职工医院湘雅分院,湖南长沙410008 [3]中南大学卫生部肝胆肠外科研究中心,湖南长沙410008 [4]中南大学湘雅二医院传染科,湖南长沙410008

出  处:《中国现代医学杂志》2004年第12期8-11,共4页China Journal of Modern Medicine

摘  要:目的通过实验获得人源性肝细胞生长因子(hHDSSF)稳定转染细胞株,为重组产品的获得奠定基础。方法通过脂质体包裹重组质粒pcDNA3。1hisB-HDSSF转染Hela细胞,以G418筛选转染细胞;进而通过RT-PCR和NorthernBlot鉴定G418筛选后的单克隆抗性细胞株。结果重组质粒pcDNA3.1hisB-HDSSF转染Hela细胞后,第20天可见G418单克隆抗性细胞株的形成。G418抗性Hela细胞株RT-PCR扩增出600bp左右的目的条带;NorthernBlot获得了明显的阳性杂交影。结论我们的实验证实HDSSF表达重组体被成功转入Hela细胞,并稳定表达;从而获得了HDSSF稳定表达细胞株,为进一步研究HDSSF表达、蛋白纯化和测定其生物学活性奠定了基础。Objective: To obtain human hepatocyte DNA synthetic stimulating factor (hHDSSF) stable transfected cell strain. Methods: Recombinant plasmid pcDNA3.1hisB-HDSSF transfected Hela cell by lipofectin, G418 was used for screening. The monoclonal resisting cell strain screened by G418 was confirmed with RT-PCR and Northern Blot. Result: The monoclonal cell strains with resistance to G418 were formed on 20th day after Hela cell was tansfected with pcDNA3.1hisB-HDSSF. A 600bp special fragment was amplified by RT-PCR in the monoclonal cell strains, and Northern Blot also showed obvious positive hybridization shadow in the cell strain. Conclusions: HDSSF expressive recombinant has been transfected successfully into Hela cells and expressed steadily, which sets up a base for further study of HDSSF expression, purification and its biological activity.

关 键 词:人源性 肝细胞生长因子 细胞转染 细胞株 克隆 

分 类 号:R575[医药卫生—消化系统]

 

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