DADS诱导人胃癌细胞分化作用中ERK/AP-1通路的改变

目的 探讨ERK/AP 1通路在二烯丙基二硫 (DADS)诱导人胃癌细胞分化中的作用 ,阐明DADS诱导人胃癌细胞分化的分子机制。方法 采用免疫细胞化学、图像分析及WesternBlot等方法 ,观察DADS作用于体外培养的人胃癌MGC80 3细胞前后AP 1成员c fos与c jun表达的改变以及ERKMAPK激酶的变化。结果 免疫细胞化学及图像分析结果显示 ,对照组c fos、c jun表达呈强阳性 ,而处理组呈阴性或弱阳性 ,阳性率明显降低 ,处理组光密度值较对照组明显低 (P <0 0 5 )。WesternBlot结果显示 :从 2 0、2 5、30到 35mg·L-1DADS处理癌细胞 ,DADS呈浓度依赖性抑制人胃癌细胞中ERK的活化 (P <0 0 5 ) ;并且DADS +MEK抑制剂PD980 5 9能完全阻断ERK活化 (P <0 0 5 ) ;时间效应上 ,在DADS刺激后 15～ 30min抑制作用最强 ,2h左右恢复至接近正常 (P <0 0 5 )。结论 ERK/AP

烫伤小鼠巨噬细胞内细胞因子变化与ERK信号的关系

目的 :观察烫伤后腹腔巨噬细胞内肿瘤坏死因子 (TNF αmRNA)、活化蛋白 1(AP 1)变化及给予MEK1 2特异性阻断药PD980 5 9后TNF αmRNA、AP 1的改变 ,阐明丝裂原活化蛋白激酶 (MAPK)信号途径中的细胞外信息调节蛋白激酶 (ERK)信号通路是否调控烫伤后TNF αmRNA的生成。方法 :以 15 %体表面积Ⅲ度烫伤小鼠为模型 ,收集腹腔巨噬细胞 ,采用逆转录 多聚酶链式反应 (RT PCR)测TNF αmRNA的表达 ,电泳迁移率改变分析法 (EMSA)测AP 1的活性。结果 :烫伤后巨噬细胞内TNF αmRNA于烫伤后 2 ,12h表达较强 ,以后呈降低趋势。AP 1于烫伤后被激活。与单纯烫伤相比 ,PD980 5 9组的AP 1活性明显被抑制 ,而TNF αmRNA表达量无明显变化。结论 :严重烫伤后巨噬细胞内TNF αmRNA的过量表达反映了烫伤后巨噬细胞的功能紊乱 ,而MAPK信号途径于烫伤后被激活 ,其中TNF αmRNA的表达可能不受ERK信号途径调控。

大鼠胃黏膜细胞EGFR通过ERK-1/2信号传导通路激活AP-1

目的 探讨大鼠胃黏膜细胞EGFR活化AP -1的信号传导通路。方法 用EGFR配体TGF -α刺激分离的大鼠胃黏膜细胞 ,Westernblot和EMSA方法检测ERK -1/ 2信号传导通路的活化程度。结果 1nmol/LTGF -α刺激胃黏膜细胞 3 0min不仅显著诱导AP -1的活性 ,而且明显激活MEK和ERK -1/ 2 ;EGFR特异性抑制剂PD15 3 0 3 5或MEK特异性抑制剂PD980 5 9能完全阻断TGF -α诱导的胃黏膜细胞AP -1活化。结论 大鼠胃黏膜细胞EGFR通过ERK -1/ 2信号传导通路激活AP -1。

Relationship between transmembrane signal transduction pathway and DNA repair and the mechanism after global cerebral ischemia-reperfusion in rats

Objective To !nvestigate the protein levels of phospho-ERK and phospho-APE/Ref-1 in hippocampal neurons after global cerebral ischemia reperfusion in rats, and observe the relationship between transmembrane signal transduction and repair of DNA damage. The role of ERK signal transduction pathway following global cerebral ischemia reperfusion in rats is further discussed. Methods Ninety healthy male SD rats were divided into 3 groups randomly： Sham group （S group）, Ischemia reperfusion group （IR group） and Pd98059 pretreatment/ischemia reperfusion group （PD group）. Global cerebral ischemia reperfusion model was established by four-vessel occlusion （4-VO） method, and reperfusion was performed 5 minutes following ischemia. Protein levels of phospho-ERK and phospho-APE/Ref-1 were detected using immunohistochemical method at 2 h, 6 h, 12 h, 24 h, 48 h and 72 h after reperfusion, and neuron apoptosis was observed by HE and TUNEL staining. Results In CA1 region of IR group, TUNEL positive cells began to appear at 6 h after IR, and reached the apex during 24 h to 48 h. However, TUNEL positive was most strongly exhibited in PD group. In IR group, phospho-ERK was obviously detected in CA3 region at 2 h after IR, and its level was phospho-ERK expression in PD group was weaker than gradually decreased from 6 h until totally absent at 48 h. Besides, that in IR group. For phospho-APE/Ref-1, its expression began to appear in CA1 region in IR group at 2 h after IR, with no obvious changes during 2 h to 12 h. Phospho-APE/Ref-1 expression began to decrease at 24 h and this decrease continued thereafter. Expression level of phospho-APE/Ref-1 in PD group was lower than that in IR group. Results showed the concurrence of decreased phospho-ERK expression level and increased neuron apoptosis after cerebral ischemia reperfusion, the former of which was consistent with the decrease of phospho-APE/ Ref- 1 expression. Also, the greater the inhibition of ERK phosphorylation was, the greater decrease of APE/Ref- 1 expression occurred. Conclusion Activation of ERK signal transduction pathway increased the expression of phospho-APE/Ref-1, and thus faciliated the repair of DNA damage. So, activation of ERK signal transduction pathway may protect neurons from apoptosis after cerebral ischemia reperfusion.