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作 者:廉沈沂[1] 孟麟[1] 杨永勇[1] 寿成超[1]
机构地区:[1]北京大学肿瘤医院暨北京市肿瘤防治研究所,生物化学与分子生物学实验室,恶性肿瘤发病机制及转化研究教育部重点实验室,北京100142
出 处:《生物技术通讯》2015年第6期790-793,共4页Letters in Biotechnology
基 金:国家自然科学基金青年项目(81301747)
摘 要:目的:构建针对TERF2IP1基因的短发夹RNA(sh RNA)表达载体,在HCT116细胞中鉴定该载体对TERF2IP1基因的干扰效果。方法:设计针对TERF2IP1基因的sh RNA序列,将其克隆至p GPHI/Hygro载体中,瞬时转染HCT116细胞48 h后,用400 mg/m L的潮霉素筛选抗性克隆,获得阳性单克隆细胞株;分别提取细胞总RNA和蛋白,进行RT-PCR和Western印迹,检测TERF2IP1的表达水平。结果:构建了4对针对TERF2IP1基因的sh RNA表达载体,通过潮霉素筛选获得稳定干扰TERF2IP1基因的HCT116细胞系,实时定量PCR和Western印迹实验均证实潮霉素筛选后,HCT116细胞中TERF2IP1的表达水平明显降低。结论:构建了4对人TERF2IP1基因的sh RNA表达载体,获得4株分别针对TERF2IP1基因不同位点的稳定干扰HCT116细胞株。Objective:To construct a recombinant vector of short hairpin RNA(shRNA) targeting TERF2IP1 gene,and to identify its inhibitory effect in HCT116 cells.Methods:the TERF2IP1 shRNA sequences were designed and inserted into pGPHI/Hygro vector.HCT116 cells were transiently transfect with shRNA vector and control vector,selected positive clone by hygromycin for 2~3 days.The total RNA and protein were extracted from the cells and the silence effect of TERF2IP1 was detected.Results:Four pair pGPHI/Hygro vector targeting TERF2IP1 were constructed,and the stably TERF2IP1 knockdown HCT116 cells were obtained.The expression of TERF2IP1 in HCT116 cells were downregulated significantly,confirmed by real-time PCR and Western blot.Conclusion:The constructed shRNA vector targeting human TERF2IP1 gene can stably suppress TERF2IP1 expression in HCT116 cells.
关 键 词:TERF2IPI基因 HCT116细胞 短发夹RNA
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