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作 者:黄修燕[1] 黄自丽[2] 许永华[2] 郑起[1] 周俭[3] 汤钊猷[3]
机构地区:[1]上海交通大学附属第六人民医院普外科,200233 [2]上海市徐汇区中心医院影像科,200031 [3]复旦大学肝癌研究所,上海200433
出 处:《中华实验外科杂志》2017年第6期963-966,共4页Chinese Journal of Experimental Surgery
基 金:国家自然科学基金面上项目(81272401);中美联合培养学者/留学生转化医学横向课题(UCTMP2015-03C001);上海市卫生局中医药科研基金(2012QJ001A)
摘 要:目的探讨转移消失蛋白B(MIM—B)与微囊蛋白-1(caveolin-1)在肝细胞癌细胞中的相互作用。方法构建携带MIM—B与FLAG融合基因的pcDNA3.1载体,脂质体法转染Hep3B、SMMC7721细胞。通过细胞免疫荧光以及共聚焦显微镜检测MIM—B蛋白与caveolin-1蛋白共定位;应用内、外源免疫共沉淀确认相互作用;以Hep3B、SMMC7721以及MHCC97H细胞为研究模型,分成空载体组、MIM—B与FLAG融合基因组,进行免疫共沉淀实验。结果成功构建携带MIM—B与FLAG融合基因的pcDNA3.1载体,pcDNA3.1-MIM—B—FLAG转染效率为90.0%以上,显著表达MIM-B。共聚焦显微镜结果显示MIM—B能沉淀caveolin-1;MIM-B与caveolin-1共定位;内、外源免疫共沉淀结果显示MIM-B与caveolin-1相互作用。结论MIM-B与caveolin-1在肝癌细胞中共定位并相互作用。Objective To investigate the protein interaction between missing in metastasis B (MIM -B) and caveolin - 1 in hepatocellular carcinoma (HCC). Methods After the construction of pcDNA3. 1 vector carrying the fusion gene of FLAG- MIM -B, we transfected the vectors into Hep3B and SMMC7721 cells respectively. The immunofluorescence and confocal microscopy were applied in detecting distribution of MIM - B and caveolin - 1 in MHCC97H cells. The immunoprecipitation in vitro and in vivo was used to confirm the protein interaction between MIM -B and caveolin - 1 in Hep3B, SMMC7721 and MHCC97H cells. The cells were divided into empty vector group and FLAG - MIM - B fusion protein group. Results The pcDNA3.1 vector with FLAG - MIM - B fusion gene was successfully constructed and the transfection efficiency of pcDNA3. 1 - MIM - B - FLAG was over 90%. The results of Western blotting analysis demonstrated that the expression of MIM - B was significantly increased. The results of mass spec- trometry showed that MIM - B could precipitate caveolin - 1. The confocal microscopy analysis showed that MIM - B was co - localized with caveolin - 1. The immunoprecipitation in endo and in exo illustrated the interaction between MIM- B and caveolin- 1. Conclusion Our research found that MIM - B and caveolin - 1 co - localized and interacted in HCC cell lines, and it is possible to provide a new molecu- lar target therapy for HCC.
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