异丙酚对H_2O_2刺激下细胞内ASK1蛋白激活的影响  

Effects of propofol on the activation of ASK1 in HEK293 cells

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作  者:王乃田[1] 肖华平[1] 肖金仿[1] 古妙宁[1] 

机构地区:[1]南方医科大学南方医院麻醉科,广东广州510515

出  处:《热带医学杂志》2011年第5期505-508,F0003,共5页Journal of Tropical Medicine

基  金:国家自然科学基金(30872431)

摘  要:目的探讨在H2O2刺激下,异丙酚对细胞中Daxx-ASK1信号通路的影响。方法对体外培养的HEK293细胞分为对照组、H2O2刺激组以及H2O2刺激合并异丙酚处理组。采用免疫荧光、Westernblot及MTT等方法,观察异丙酚预处理对H2O2刺激下的HEK293细胞存活率以及细胞中Fas死亡结构域相关蛋白(Daxx)的亚细胞定位以及凋亡信号调节激酶1(ASK1)激活的影响。结果在200~500μmol/LH2O2刺激下,异丙酚在一定程度上能有效保护细胞,缓解抗氧化应激损伤。进一步实验发现,H2O2刺激细胞后,与H2O2刺激组相比,异丙酚处理组细胞中Daxx蛋白大部分仍然聚集在细胞核中,只有少部分移入到细胞浆中,相应ASK1的激活程度也较低。结论氧化应激刺激下,异丙酚可通过抑制细胞中Daxx蛋白的出核,进而抑制胞浆中ASK1蛋白的激活,从而起到保护细胞、抑制细胞死亡的效能。Objective To study the effect of propofol on Daxx-ASK1 signal transduction pathwy in HEK293 cells treated with H2O2.Methods HEK293 cells were devided into three groups:control group,H2O2 treatment group,and H2O2 plus propofol group.Immunofluorescence,Western blot and MTT assays were used to evaluate the cellular viability,subcellular location of Fas death domain-associated protein(Daxx),and the activation of apoptosis signal-regulating kinase 1(ASK1) in H2O2-treated HEK293 cells.Results At the concentration range of 200-500 mol/L,H2O2 propofol effectively protected cells from H2O2-induced oxidative stress.Furthermore,Daxx was mainly remained in the cytoplasm,and the degree of ASK1 activation was less than the H2O2 treatment group.Conclusion Propofol could protect cells from oxidative stress-induced injury through the inhibition of the translocaton of Daxx and the activation of ASK1.

关 键 词:H2O2 异丙酚 DAXX ASK1 保护 

分 类 号:R971.2[医药卫生—药品]

 

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