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Fas基因转导大肠癌细胞株的表达
引用本文:李恕军,肖冰,等.Fas基因转导大肠癌细胞株的表达[J].第一军医大学学报,2002,22(8):700-703.
作者姓名:李恕军  肖冰
作者单位:[1]北京军区总医院消化内科,北京100700 [2]第一军医大学南方医院消化内科,广州510515
摘    要:目的:建立表达外源性Fas基因的大肠癌细胞株,观察Fas基因在转导前后的表达,方法:采用分子克隆技术将Fas基因插入真核表达载体pBK-CMV的多克隆位点之间,以脂质体介导法将Fas基因导入受体细胞LoVo ,用G418筛选克隆细胞,以dot blotting,Westting blotting检测转导细胞Fas基因的表达,结果:成功建立了Fas基因表达株,转导株在RNA及其蛋白水平表达均明显高于非转导株,转导细胞增殖速度,倍增时间,对数生长期等均比非转导株更为缓慢,但无显著性差异,在Fas抗体作用下,转导株细胞生长明显受到抑制,有非常显著性差异,结论:Fas基因在大肠癌细胞中处于低表达状态,通过真核表达载体介导,Fas基因在RNA及其蛋白水平能有效表达,Fas表达株在Fas抗体作用下可明显抑制体外培养的大肠癌细胞的生长增殖。

关 键 词:表达  Fas基因  基因转导  大肠癌  细胞凋亡

Expression of Fas genes transduced into colorectal cancer cells]
Shu-Jun Li,Bing Xiao,Bo Jiang,Ying Han.Expression of Fas genes transduced into colorectal cancer cells][J].Journal of First Military Medical University,2002,22(8):700-703.
Authors:Shu-Jun Li  Bing Xiao  Bo Jiang  Ying Han
Institution:Department of Digestive Diseases, General Hospital of Beijing Command, Beijing 100700, China.
Abstract:OBJECTIVE: To construct colorectal cancer cells expressing exogenous Fas gene and observe the expression level of its mRNA and protein before and after transduction. METHODS: Fas cDNA was inserted into the multiple cloning site of the expression vector pBK-CMV with molecular cloning technique, and the resultant recombinant plasmid was transduced into colorectal cancer LoVo cells via lipofectamine. G418 was utilized to screen the positive clones containing the recombinant plasmid, where Fas mRNA and protein expression was determined with Western blotting and dot blotting. RESULTS: pBK-CMV Fas cDNA plasmid was successfully constructed. The transduced colorectal cancer cells were screened by G418 and a resistant cell line (LoVo Fas cells) was obtained. Fas expression was detected in both transduced and non-transducted cell lines, but the expression level of both Fas mRNA and protein was much higher in the former, which showed lowered proliferation rate and lengthened doubling time and logarithm growth period than the non-transducted cells, but the difference was not significant. Treatment of the transduced cells with Fas antibody produced significant difference (P<0.05), manifested by apparently inhibited cell growth. CONCLUSIONS: LoVo cells normally has only very low expression level of Fas gene, while transduction with pBK-Fas cDNA can enhance the efficiency of Fas mRNA and protein expressions. Fas antibody significantly inhibits the growth and proliferation of in vitro cultured Fas-expressing LoVo cells.
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