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作 者:马炬明[1] 苏长青[2] 王伟国[1] 施建国[1] 胡慧珍[1] 李林芳[2] 钱其军[2]
机构地区:[1]解放军第117医院内科 [2]上海第二军医大学东方肝胆外科医院病毒基因治疗实验室,200438
出 处:《临床肿瘤学杂志》2007年第3期166-168,共3页Chinese Clinical Oncology
基 金:国家自然科学基金项目(30572149);浙江省科技计划项目(2006C30021)
摘 要:目的:克隆转录因子E2F的启动子,研究其针对pRb/E2F/p16调控环路缺陷肿瘤的特异性。方法:提取HepG-Ⅱ细胞基因组DNA,PCR扩增其转录因子E2F启动子(E2Fp),插入pGL3-Basic多克隆位点,构建成pGL3-E2Fp;采用Luciferase报告基因检测方法,在肿瘤细胞和正常细胞内测定E2Fp介导的Luciferase表达,以推测E2Fp肿瘤的特异性。结果:E2Fp在正常细胞内几乎没有活性,而在肿瘤细胞内具有较高的活性,两组间Luciferase报告基因表达的差异有显著性(P=0.0004)。结论:靶向pRb/E2F/p16环路缺陷肿瘤的E2Fp,具有对基因表达调控的特异性,能够提高Luciferase报告基因在肿瘤细胞中表达的靶向性。E2Fp的克隆为改进肿瘤基因治疗的疗效提供了一种可靠的工具。Objectlve:To clone the promoter of transcriptional factor E2F (E2Fp), and to investigate its specific activity targeting the cancers with a defective pRb/E2F/p16 regulatory pathway. Methods:E2Fp was amplified from the genome DNA of HepG-Ⅱ cells, then inserted into the multiple cloning sites of the plasmid pGL3-Basic to generate the pGL3-E2Fp. Dual-luciferase reporter assay was used to detect the expression of luciferase in cancer and normal cells, by which the E2Fp cancer-specificity was analyzed. Results: E2Fp almost had no activity in normal cells, but had strong activity in cancer cells. There was an obvious difference between the expression of luciferase in cancer and normal cells ( P = 0. 000 4 ). Conclusion: The E2Fp targeting the cancers with a defective pRb/E2F/p16 regulatory pathway has a cancer-specificity for regulating gene expression. It can increase the specificity of luciferase gene expression in cancer cells. The cloning of E2Fp provides us a useful tool for target gene therapy of cancers.
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