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TGF-β1刺激对人腹膜间皮细胞内Smad信号转导通路的影响
引用本文:张浩,刘伏友,刘映红,龙志高,吴鼎文,敖翔,陈仙花. TGF-β1刺激对人腹膜间皮细胞内Smad信号转导通路的影响[J]. 中南大学学报(医学版), 2004, 29(2): 142-147
作者姓名:张浩  刘伏友  刘映红  龙志高  吴鼎文  敖翔  陈仙花
作者单位:中南大学1.湘雅三医院肾内科,长沙410013;2.湘雅二医院肾内科,长沙410011;3.遗传学国家重点实验室,长沙410078
基金项目:卫生部临床重点项目 (2 1 99771 9)
摘    要:目的:探讨人腹膜间皮细胞内Smad信号转导通路在TGF-β1致腹膜纤维化过程中是否发挥作用。方法:取健康成年人大网膜进行人腹膜间皮细胞原代培养,经鉴定95%以上为人腹膜间皮细胞。用5 ng/ml TGF-β1刺激第三代培养细胞,采用免疫组织化学染色、Western blotting,ELISA以及RT-PCR等方法,分别观察人腹膜间皮细胞内磷酸化Smad2/3(p-Smad2/3)的蛋白表达以及在细胞内的迁移;细胞内Smad7的蛋白和mRNA表达;细胞外纤维连接蛋白(FN)的蛋白、细胞内FN的mRNA以及细胞内I型胶原(COL1)的蛋白和mRNA表达。结果:人腹膜间皮细胞内p-Smad2/3的蛋白表达在TGF-β1刺激后15 min即开始显著增加,此时p-Smad2/3的阳性细胞率为29%,细胞着色主要分散在细胞质中,30 min阳性细胞率81%至1 h阳性细胞率84%增加最明显,细胞着色加深且集中在细胞核及周边,2 h蛋白表达明显回落,此时阳性细胞率为37%,细胞着色转淡并又分散至细胞质中;细胞内Smad7的蛋白表达在TGF-β1刺激后24 h明显增加,48 h时达高峰,mRNA表达呈时间依从性增强;细胞外FN的蛋白、细胞内FN的mRNA以及细胞内COL1的蛋白和mRNA表达从TGF-β1刺激后24 h起均明显增加,且均显示一定的时间依从性。结论:人腹膜间皮细胞内Smad信号转导通路能被TGF-β1特异性激活,并在TGF-β1致腹膜纤维化过程中发挥效应;经TGF-β1刺激后,在该通路中主要起抑制作用的Smad7蛋白和mRNA表达均反馈性增加。

关 键 词:间皮细胞  TGF-&beta  1  Smad2/3  Smad7  细胞外基质  
文章编号:1672-7347(2004)02-0142-06
收稿时间:2003-08-14
修稿时间:2003-08-14

Effect of TGF-β1 stimulation on the Smad signal transduction pathwayof human peritoneal mesothelial cells
ZHANG Hao ,LIU Fu you ,,LIU Ying hong ,et al.. Effect of TGF-β1 stimulation on the Smad signal transduction pathwayof human peritoneal mesothelial cells[J]. Journal of Central South University. Medical sciences, 2004, 29(2): 142-147
Authors:ZHANG Hao   LIU Fu you     LIU Ying hong   et al.
Affiliation:1.Department of Nephrology, Third Xiangya Hospital, Central South University, Changsha 410013, China;
2.Department of Nephrology, Second Xiangya Hospital, Central South University, Changsha 410011, China
Abstract:OBJECTIVE: To explore whether the Smad signal transduction pathway in human peritoneal mesothelial cells (HPMCs) influences the process of human peritoneal fibrosis stimulated by TGF-beta1. METHODS: HPMCs were isolated from normal human omentum and 95% of the primary cultured cells was confirmed to be HPMCs. The third generation of cultured cells was stimulated by 5 ng/ml TGF-beta1. Immunohistochemistry, Western blotting, ELISA, and RT-PCR were employed to investigate the follows: the protein expression of p-Smad2/3 and its migration in HPMCs; the protein and mRNA expressions of SMAD 7 in cells; and the expressions of extracellular fibronectin (FN) protein, intracellular FN mRNA, as well as intracellular collenge-I (COL1) protein and mRNA. RESULTS: The protein expression of p-Smad2/3 in HPMCs obviously increased 15 min (29% p-Smad2/3-positive cells) after TGF-beta1 stimulation, peaking from 30 min (81% ) to 1 h (84%) and dropping after 2 h (37%); Meanwhile, p-Smad2/3 mainly distributed in cytoplasm at 15 min, concentrated in cell nucleus and peri-nucleus from 30 min to 1 h, and distributed in cytoplasm again at 2 h. The protein expression of SMAD7 in cells obviously increased 24 h after TGF-beta1 stimulation, peaking at 48 h. The mRNA expression of SMAD7 time-dependently increased. The expressions of extracellular FN protein, intracellular FN mRNA, as well as intracellular COL1 protein and mRNA significantly increased and all of them displayed time dependency. CONCLUSION: The SMAD signal transduction pathway of HPMCs can be specifically activated by TGF-beta1 and influence the process of human peritoneal fibrosis. With the stimulation of TGF-beta1, the protein and mRNA expressions of SMAD 7 (an inhibitor of SMAD pathway) significantly increase as a result of feedback.
Keywords:mesothelial cells;TGF-β1 ;Smad2/3;Smad7;extracellular matrix
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