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基因枪介导真核表达质粒转染体外培养的COS-7细胞系的实验研究
引用本文:张亮,阎瑾琦,马继尧,王浩,刘宁,贾锐,韩刚,董金凯,田仁礼,于继云.基因枪介导真核表达质粒转染体外培养的COS-7细胞系的实验研究[J].生物技术通讯,2008,19(5):681-684.
作者姓名:张亮  阎瑾琦  马继尧  王浩  刘宁  贾锐  韩刚  董金凯  田仁礼  于继云
作者单位:1. 军事医学科学院,基础医学研究所,北京,100850
2. 解放军总医院,泌尿外科,北京,100853
基金项目:国家自然科学基金,国家高技术研究发展计划(863计划) 
摘    要:目的:建立基因枪子弹制备及转染体外培养COS-7细胞系的方法。方法:以亚精氨、氯化钙沉淀法制备子弹(DNA+金颗粒),利用原子力显微镜观察子弹制备情况;采用基因枪方法分别将真核表达质粒pVax-Dsred-IRES-EGFP转染对照组和实验组COS-7细胞,转染后24h,利用激光扫描共聚焦显微镜观察细胞中红、绿荧光蛋白的表达。结果:制备了基因枪子弹,DNA紧密包裹在金颗粒周围;基因枪介导的pVax-Dsred-IRES-EGFP被转染入体外培养的COS-7细胞,转染后24h可检测到红、绿荧光,而对照组则没有荧光蛋白的表达。结论:国产新芝SJ-500型基因枪能够有效介导外源基因转移,基因枪转染的COS-7细胞能够有效表达报告基因。

关 键 词:基因枪  细胞转染  真核表达载体  荧光蛋白  COS-7细胞系

Empirical Study of Gene Gum-Mediated Eukaryotic Expression Vector Transfection of COS-7 Cell Lines/n Vitro
ZHANG Liang,YAN Jin-Qi,MA Ji-Yao,WANG Hao,LIU Ning,JIA Rui,HAN Gang,DONG Jin-Kai,TIAN Ren-Li,YU Ji-Yun.Empirical Study of Gene Gum-Mediated Eukaryotic Expression Vector Transfection of COS-7 Cell Lines/n Vitro[J].Letters in Biotechnology,2008,19(5):681-684.
Authors:ZHANG Liang  YAN Jin-Qi  MA Ji-Yao  WANG Hao  LIU Ning  JIA Rui  HAN Gang  DONG Jin-Kai  TIAN Ren-Li  YU Ji-Yun
Institution:ZHANG Lian, YAN Jin-Qi, MA Ji-Yao, WANG Hao, LIU Ning, JIA Rui, HAN Gang, DONG Jin-Kai, TIAN Ren-Li, YU Ji-Yun (1.Institute of Basic Medical Sciences, Academy of Military Medical Sciences, Beijing 100850; 2. Department of Urology, PLA General Hospital, Beijing 100853; China)
Abstract:Objective: To establish a preparation method of cartridge for gene gun and to observe the gene gun-mediated gene transfectiono to COS-7 cell lines in vitro. Methods: The cartridge(microcarrier+DNA) was prepared by precipitation method of spermidine and calcium chloride. Using atomic force microscope to observe the detail of the cartridge. The recombinant eukaryotie expression vector pVax-Dsred-IRES-EGFP was tansfected into COS-7 cell lines by gene gun. The. expression of report gene was observed through laser scan confocal microscopy. Results: The cartridge of gene gun was successfully prepared, DNA-coated gold mierocarriers was achieved. Red and green fluorescent protein could be detected in the transfected COS-7 cell lines after 24 hours, when no fluorescent protein was detected in control group. Conclusion: SJ-500 gene gun-mediated gene transfer is effective and practicable. The report gene can be expressed through gene gun mediated transfection to cell lines in vitro.
Keywords:gene gun  cell transfection  eukaryotic expression vector  fluorescent protein  COS-7 cell lines
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