吉林大学学报(医学版)

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RNAi沉默STAT3基因联合mTOR抑制剂rapamycin诱导BEL-7402肝癌细胞凋亡

张毅1* ,张君薇2,谢淑丽3,王广义4   

  1. (1.辽宁医学院附属第一医院微创肝胆外科,辽宁 锦州 121000;2. 辽宁医学院附属第三医院肿瘤科,辽宁 锦州 121000;3.吉林大学第一医院普通外科实验室,吉林 长春130021;4.吉林大学第一医院肝胆胰外科,吉林 长春130021)
  • 收稿日期:2012-12-20 出版日期:2013-09-28 发布日期:2013-09-28
  • 通讯作者: 王广义 E-mail: (Tel: 0431-85613331,E-mail:pla205@163.com)
  • 作者简介:张 毅 (1969-),男,辽宁省锦州市人,主治医师,医学博士,主要从事肝癌的细胞信号转导与凋亡研究。 
  • 基金资助:

    辽宁省科技厅科学技术计划项目资助课题(201300384)

Apoptosis of hepatocarcinoma cells BEL-7402  induced with STAT3 gene silencing combined with rapamycin

ZHANG Yi 1* ,ZHANG Jun-wei2,XIE Shu-li3,WANG Guang-yi4   

  1. (1. Department of Hepatobiliary and Pancreas Surgery,First Hospital,Liaoning Medical University,Jinzhou 121000,China;2. Department of  Oncology,Third Hospital,Liaoning Medical University,Jinzhou 121000,China;3. Laboratory of General Surgery,First Hospital,Jilin University,Changchun 130021,China;4. Department of Hepatobiliary and Pancreatic Surgery,First Hospital,Jilin University,Changchun 130021,China )
  • Received:2012-12-20 Online:2013-09-28 Published:2013-09-28

摘要:

目的:探讨PI3K/AKT/mTOR和JAK/STAT3 2条信号转导途径共同作用对肝癌细胞凋亡的影响,为肝癌基因治疗提供依据。方法:选取对数生长期BEL-7402细胞,随机分为对照组、mTOR抑制剂rapamycin(Rapa)组、阴性质粒组、阴性质粒+ Rapa组、STAT3-siRNA质粒组和STAT3-siRNA 质粒+Rapa组,应用LipofectamineTM 2000转染试剂将含有目的基因的质粒转染BEL-7402细胞,同时应用rapamycin,分别采用流式细胞术和Hoechst33258荧光染色检测细胞凋亡率和形态学的变化,JC-1 荧光染色观察线粒体膜电位(ΔΨm)变化,Western blotting法检测活性caspase-3蛋白表达水平。结果:STAT3-siRNA+Rapa组细胞凋亡率为60.22%±0.87%,明显高于其他各组(P<0.05),且细胞ΔΨm明显降低(27.28%±1.82%,P<0.05);Hoechst33258荧光染色检测,见STAT3-siRNA有大量细胞出现细胞核聚集、边缘化和核
碎裂等典型细胞凋亡形态;Western blotting检测,STAT3-siRNA+Rapa组活性caspase-3蛋白表达水平明显高于其他各组(P<0.05)。结论:RNAi沉默BEL-7402肝癌细胞STAT3基因联合rapamycin可促进BEL-7402肝癌细胞的凋亡,二者具有明显的协同作用。

关键词: mTOR蛋白, STAT3基因, RNA干扰, rapamycin, 细胞凋亡, 肝细胞癌

Abstract:

Abstract:Objective
To explore the influence of PI3K/AKT/mTOR and JAK/STAT3 signaling pathway in apoptosis of the hepatocarcioma cells(HCC),and to provide basis for gene therapy for liver cancer.Methods BEL-7402 cells at inlogarithm growth phase were selected and randomly divided into control group,scramble-siRNA group,STAT3-siRNA group,scramble-siRNA +rapamycin(Rapa) group,Rapa group and STAT3-siRNA+Rapa group.The plasmids pGCsi.U6/neoRFP-STAT3 designed for expression of STAT3 siRNA was transfected into BEL-7402 cells by LipofectamineTM 2000.The cells with or without transfection siRNA were treated in wells in the absence or presence of rapamycin.The apoptotic rate was detected  by flow cytometry (FCM) and AnnexinV/PI apoptosis detection kit staining.The morphological changes of the cells were assessed by Hoechst33258 immunofluorescence staining.Simultaneously,the mitochondrial membrane potential(ΔΨm) was visualized by the JC-1 fluorescence staining and inverted fluorescence microscope.Further more,the expression level of active caspase-3 protein was analyzed by Western blotting method.Results The apoptotic rate of BEL-7402 cells in STAT3-siRNA+Rapa group (60.22%±0.87 %) was higher than those in other groups (P<0.05);and the ΔΨm was significantly decreased (27.28%±1.82%,P<0.05).The Hoechst33258 fluoresence staining results showed that the characteristic changes of chromatin condensation and nuclear  fragmentation were observed in STAT3-siRNA + Rapa group.The Western blotting results showed that the protein expression level of active caspase-3 in STAT3-siRNA + Rapa group was significantly higher than those in the other groups (P<0.05).Conclusion Combined treatment of rapamycin and STAT3 gene silencing can significantly promote the apoptosis of BEL-7402 cells and they display synergistic effects.

Key words: mTOR protein, STAT3 gene, RNA interference, rapamycin, apoptosis, hepatocelluar carcinoma

中图分类号: 

  • R735.7