| 摘要: |
| 目的:探讨TGFβ1诱导皮肤成纤维细胞(FB)向肌成纤维细胞转分化的可能途径和调控机制。方法:将野生型和Smad3基因敲除(KO)型小鼠皮肤FB分为9组:野生型FB组、野生型FB+TGFβ1组、野生型FB+SB431542组、野生型FB+SB431542+TGFβ1组、Smad3 KO FB组、Smad3 KO FB+TGFβ1组、野生型FB+SB203580+TGFβ1组、野生型FB+PD98059+TGFβ1组和野生型FB+SP600125+TGFβ1组。各组细胞经同步化处理后,直接以TGFβ1刺激或经上述各激酶抑制剂预处理后再以TGFβ1刺激。收集细胞,一部分以单细胞RTPCR检测αSMA阳性表达百分比,另一部分细胞抽提总RNA后采用实时荧光定量RTPCR检测αSMA的表达水平变化。结果:Smad3 KO组与SB431542组的αSMA表达水平和阳性百分比显著升高(Smad3 KO FB组vs野生型FB组;野生型FB+SB431542+TGFβ1组vs 野生型FB+SB431542组;Smad3 KO FB+TGFβ1组vs Smad3 KO FB组,P<0.01),而SB203580组和SP600125组中αSMA表达水平和阳性百分比升高的作用则被显著抑制(野生型FB+SB203580+TGFβ1组、野生型FB+SP600125+TGFβ1组vs 野生型FB+TGFβ1组,P<0.05)。结论:在TGFβ1诱导成纤维细胞向肌成纤维细胞的转分化过程中,Smad3途径介导抑制作用,而p38/MAPK、JNK/MAPK途径则介导正向调节作用。 |
| 关键词: 转化生长因子β Smad3 成纤维细胞 肌成纤维细胞 转分化 小鼠,基因敲除 |
| DOI:10.3724/SP.J.1008.2007.01175 |
| 投稿时间:2007-06-18修订日期:2007-09-29 |
| 基金项目:科技部“973”项目子课题(2005CB522603). |
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| TGF-β1-induced transdifferentiation of derma fibroblasts into myofibroblasts:a study of mechanism |
| XIONG Jie,XIA Zhao-fan*,,LvKai-yang,WANG Yu,HAN Shu |
| (Department of Burns,Burn Institute of PLA,Changhai Hospital,Second Military Medical University,Shanghai 200433,China) |
| Abstract: |
| Objective:To explore the possible pathways and regulatory mechanism of TGFβ1induced transdifferentiation of derma fibroblasts(FB) into myofibroblasts. Methods: Mice Wildtype and Smad3 knockout(Smad3 KO) derma FB were divided into 9 groups,namely,A:Wildtype FB; B:Wildtype FB+TGFβ1; C:Wildtype FB+SB431542; D:Wildtype FB+SB431542+TGFβ1; E:Smad3 KO FB; F:Smad3 KO FB+TGFβ1; G:Wildtype FB+SB203580+TGFβ1; H:Wildtype FB+PD98059+TGFβ1; and I:Wildtype FB+SP600125+TGFβ1. After synchronization treatment,the cells were treated with TGFβ1 with or without pretreatment with above mentioned kinases inhibitors. Then the cells were collected for RNA extraction and the expression of αSMA was detected by real time quantitative RTPCR; some cells were analyzed by single cell RTPCR to test the positive expression rate of αSMA.Results: The expression and positive rate of αSMA in SB431542 group and Smad3 knockout group were significantly increased(group E vs. group A;group D vs. group C;group F vs. group E,P<0.01) and those in SP600125 group and SB203580 group were significantly inhibited(group G and I vs. group B,P<0.05). Conclusion: In TGFβ1induced derma fibroblasts transdifferentiation into myofibroblasts,Smad3 pathway plays a negative regulatory role and p38/MAPK and JNK/MAPK pathway play a positive regulatory role. |
| Key words: transforming growth factor beta Smad3 fibroblast myofibroblast transdifferentiation mice,knockout |
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