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作 者:朱颖超[1] 杨耀琴[1] 陶惠红[1] 陈海霞[1] 王和勇[2]
机构地区:[1]同济大学医学院肿瘤研究所,上海200092 [2]同济大学附属肺科医院中心实验室,上海200433
出 处:《同济大学学报(医学版)》2013年第4期6-9,共4页Journal of Tongji University(Medical Science)
基 金:国家自然科学青年基金(30800631)
摘 要:目的构建miR-29c真核表达载体并转染95D肺癌细胞,观察miR-29c过表达对95D细胞增殖能力的影响。方法克隆miR-29c片段插入质粒pcDNA3.1,构建miR-29c表达质粒pcDNA3.1-miR-29c;通过脂质体瞬时转染人肺癌细胞株95D,荧光PCR检测细胞miR-29c表达水平,MTT法检测过表达miR-29c对细胞增殖能力的影响。结果重组质粒pcDNA3.1-miR-29c经酶切及测序证明构建成功,荧光PCR证实转染后95D细胞miR-29c表达水平显著升高,是对照组的36倍。MTT检测结果表明,过表达miR-29c的95D细胞增殖受到显著抑制,至72 h抑制率最高,达38.63%。结论成功构建miR-29c真核表达质粒pcDNA3.1-miR-29c,初步观察显示过表达miR-29c显著抑制95D肺癌细胞增殖效应。为进一步深入研究miR-29c对肺癌的作用打下良好基础。Objective To construct eukaryotic expression vector of miR-29c and to investigate its effect on proliferation of human lung cancer 95D ceils. Methods pcDNA3. 1-miR-29c was constructed by inserting cloned gene miR-29c to eukaryotic expression vector pcDNA3.1. Sequencing and restriction endonucleases were used to verify the recombinant vector. Human lung cancer 95D cells were transfected by pcDNA3. 1-miR-29c. The expression level of miR-29c in 95D cells after transfection was identified by Real-Time PCR. The cell proliferative levels were assessed by MTT test. Results The expression vector of recombined pcDNA3.1-miR-29c was successfully constructed. The miR-29c expression levels in 95D cells after transfection significantly increased and were 36 times as that of control group. The proliferative activity was suppressed in pcDNA3. 1-miR-29c cells and the inhibition rate reached the highest 38.63% at 72 hour. Conclusion MiR-29c eukaryotic expression plasmid pcDNA3. 1-miR-29c was successfully constructed. Preliminary study indicated that over- expression of miR-29c can inhibit the proliferation of human lung cancer 95D cells.
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