靶向抑制肝癌耐药细胞多药耐药基因表达的实验研究

INHIBITION OF MDR1 EXPRESSION IN HEPATOCELLULAR CARCINOMA CELL BEL-7402/R BY VECTOR-MEDIATED RNA INTERFERENCE

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摘要目的:构建含多药耐药基因MDR1的短发夹状RNA(shorthairp in RNA,shRNA)表达质粒,并观察其对肝癌耐药细胞Bel-7402/R的MDR1 mRNA的抑制作用。方法:利用分子克隆技术,将含MDR1的双链DNA,与经双酶切后的载体PGE-1连接,构建pshRNA-MDR1重组质粒,在脂质体的介导下转染肝癌耐药细胞株BEL-7402/R,RT-PCR分析MDR1mRNA的表达,流式细胞仪检测细胞P-gp的表达。结果:PCR和DNA测序证实了表达质粒构建成功,并能明显地抑制MDR1mRNA的表达;P-gp的表达阳性率降低了57.3%,P<0.05。结论:构建的pshRNA-MDR1表达质粒能靶向抵制肝癌耐药细胞MDR1mRNA和P-gp的表达。 Objective：To construct a recombinant plasmids generating short hairpin RNA contain of multi-drug resistance gene MDR1 in mammalian cells in order to investigate suppression of MDR1 mRNA in hepatocellular carcinoma cells Bel-7402/R.Methods： Using molecular cloning technique,double-stranded DNA which contained MDR1 cloned into PGE-1 vector digesting by two restricted endoenzymes according to its special orientation.Human hepatocellular carcinoma cells Bel-7402/R was transfected with recombinant plasmid by LyoVecTM,MDR1 mRNA was assessed by RT-PCR,we determined the expression of P-gp by flow cytometry（FCM）.Results： The size of the PCR product was 669bp.DNA sequencing showed the sequence of recombinant vector pshRNA-MDR1 was successfully constructed,and suppressed MDR1 mRNA expression;positive rate of P-gp receded from 77.7% to 20.4%,P0.05.Conclusion： The result showed that the recombinant plasmid constructed by the authors can suppress the expression of MDR1 mRNA and P-gp in hepatocellular carcinoma cells Bel-7402/R.

作者胡礼仪张有顺周业庭臧家兰吴柏华

机构地区沭阳人民医院检验科湖北医药学院附属东风医院肝脏外科研究所

出处《牡丹江医学院学报》 2010年第5期31-34,共4页 Journal of Mudanjiang Medical University

关键词基因多药耐药 RNA干涉肝癌 gene MDR RNA interference hepatocellular carcinoma

分类号 R733.71 [医药卫生—肿瘤]

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靶向抑制肝癌耐药细胞多药耐药基因表达的实验研究

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