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低氧诱发人肝癌细胞株HepG2中IAP-2表达及相关机制
引用本文:谷华,赵秋,廖家智,杜静,覃华,刘南植. 低氧诱发人肝癌细胞株HepG2中IAP-2表达及相关机制[J]. 华中科技大学学报(医学版), 2006, 35(3): 310-313
作者姓名:谷华  赵秋  廖家智  杜静  覃华  刘南植
作者单位:华中科技大学同济医学院附属同济医院消化内科,武汉,430030
摘    要:目的 研究极度低氧下人肝癌细胞株HepG2中凋亡抑制蛋白2(IAP-2)表达的变化,初步探讨其与缺氧诱导因子1(HIF-1)的相关性。方法 HepG2细胞株分组孵育,用免疫细胞化学定性检测IAP-2蛋白,再用Western blot半定量检测IAP-2蛋白变化,同时对比HIF-1蛋白表达;用RT-PCR检测IAP-2基因水平改变。结果 免疫细胞化学检测IAP-2蛋白在HepG2细胞中呈阳性表达,定位于胞质。Western blot显示,极度低氧1 h IAP-2蛋白表达明显高于常氧组(t=5.723,P〈0.05),3、5 h IAP-2持续高表达,复氧后恢复基线水平;实验还显示HIF-1和IAP-2的蛋白表达具有差异性:常氧组HIF-1未表达,低氧4h可诱发,IAP-2保持基线水平;极度低氧HIF-1无变化,IAP-2表达明显增高;复氧后HIF-1不表达,IAP-2恢复基线表达;加入氯化钴后HIF-1恢复表达,IAP-2保持基线。RT-PCR检测表明,极度低氧1 h IAP-2 mRNA表达明显高于常氧组(t=7.097,P〈0.05),3、5 h IAP-2持续高表达,该结果与上述IAP-2蛋白表达具有一致性。结论 首次表明极度低氧下IAP-2在人肝癌细胞株HepG2表达上调,并具有独立于HIF-1的抗凋亡机制。

关 键 词:低氧  肝癌细胞  凋亡抑制蛋白2
修稿时间:2005-06-30

Expression and Related Mechanism of Apoptosis Inhibitory Protein 2 in Hepatic Cancer Cell HepG2 Induced by Hypoxia
Gu Hua,Zhao Qiu,Liao Jiazhi. Expression and Related Mechanism of Apoptosis Inhibitory Protein 2 in Hepatic Cancer Cell HepG2 Induced by Hypoxia[J]. Journal of Huazhong University of Science and Technology(Health Sciences), 2006, 35(3): 310-313
Authors:Gu Hua  Zhao Qiu  Liao Jiazhi
Affiliation:Gu Hua,Zhao Qiu,Liao Jiazhi~
Abstract:Objective To investigate the changes in the expression of apoptosis inhibitory protein 2(IAP-2) in hepatic cancer cell HepG2 under severe hypoxia and explore its relation with hypoxia inducible factor 1(HIF-1).Methods HepG2 cells were cultured in different groups.Immunocytochemistry was used to qualitatively assay IAP-2 protein.Western blot analysis was applied to semi-quantitatively determine IAP-2 protein and HIF-1 protein.RT-PCR was performed to detect the mRNA expression of IAP-2.Results The immunocytochemical staining showed the positive expression of IAP-2 protein in HepG2 cytoplasma.Western blot analysis revealed the expression of IAP-2 protein could be markedly induced(t=5.723,P<0.05) under severe hypoxia for 1 h and remain high after 3 or 5 h.There was difference in the expression of IAP-2 and HIF-1 proteins.HIF-1 was undetectable in normoxic HepG2 cells,but induced by hypoxia.Under sever hypoxia HIF-1 was modest but IAP-2 was abundantly detected.After re-oxygenation HIF-1 was degraded and IAP-2 returned to basal level.Colalt chloride activated HIF-1 but not IAP-2.RT-PCR analysis found the expression of IAP-2 mRNA after 1 h of sever hypoxia was evidently higher than that in normoxia(t=7.097,P<0.05),and remained high after 3 or 5 h.Conclusion Severe hypoxia induced the up-regulation of IAP-2 in HepG2 through HIF-1-independent pathways.
Keywords:hypoxia  hepatic cancer cell  apoptosis inhibitory protein 2
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