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作 者:孙方浩[1,2] 郑骏年[1] 徐为[3] 刘晓昀[1] 张宝福[1] 宋文哲[3] 刘俊杰[3] 章龙珍[3] 顾玉明[3] 高超[3] 李望[1] 裴冬生[1]
机构地区:[1]江苏徐州医学院肿瘤生物治疗实验室,221002 [2]徐州市第一人民医院泌尿外科,221002 [3]徐州医学院附属医院肿瘤中心
出 处:《中华实验外科杂志》2009年第1期87-88,共2页Chinese Journal of Experimental Surgery
基 金:基金项目:国家自然科学基金资助项目(30873021)
摘 要:目的克隆肿瘤特异Ki-67启动子,观察其在人肿瘤细胞中的转录活性。方法提取。肾癌Ketr-3细胞基因组总DNA作为模板,聚合酶链反应(PCR)获取1.6kb的Ki-67启动子DNA片段。克隆到pGL3-Basic载体构建双荧光素酶检测质粒pGLB-Ki-67。将pGLB—Ki-67转染4种人肿瘤细胞及人脐静脉内皮Huvec细胞,使用双荧光素酶检测系统鉴定启动子活性及肿瘤特异性。结果电泳与测序结果显示克隆出的Ki-67启动子片段序列与Genbank中记录一致,pGLB.Ki-67质粒构建成功。其启动子活性在Hela、BIU-87、Ketr-3、A5494种人肿瘤细胞内分别达到SV40 promoter/enhancer活性的21.0%、31.1%、23.9%和7.2%;在Huvec细胞内仅为0.5%。结论克隆出Ki-67基因启动子(-820~+771),并证明其具有良好转录活性。Objective To clone DNA sequence of Ki-67 promoter,and identify its transcriptional activities in different human carcinoma cell lines. Methods The DNA fragment of Ki-67 promoter was cloned from the genomie DNA of Ketr-3 cells and inserted into lueiferase reporter vectors (pGL3-Basic) to reconstruct a recombinant plasmid named pGLB-Ki-67. The dual-lnciferase reporter assay system was used to identify the transcriptional activity and tumor specificity of Ki-67 in normal umbilical vein epithelial cell line Huvec and 4 different carcinoma cell lines ( Hela, BIU-87, Ketr-3 and A549 ). Results Eleetrophoresis and DNA sequencing demonstrated that cloned Ki-67 promoter was 1.6 kb, as registered in Genbank. The recombinant plasmid pGLB-Ki-67 was comfirmed by DNA sequencing. In ela, BIU-87, Kerr-3 and A549 cells,the Ki-67 promoter exhibited different transcriptional activities respectively equivalent to 21. 0% ,31.1% ,23.9% and 7.2% of SV40 promoter/enhancer. In normal Huvec cells,the transcriptional activity of Ki-67 was only 0.5%. Conclusion We first cloned the Ki-67 promoter, which had a strong transcriptional activity and tumor specificity.
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