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Smad1表达和转录活性的增加会增强肝星状细胞的转分化。

Increased Smad1 expression and transcriptional activity enhances trans-differentiation of hepatic stellate cells.

作者信息

Shen Hong, Fan Jianghong, Burczynski Frank, Minuk Gerald Y, Cattini Peter, Gong Yuewen

机构信息

Medical Research Center, Xiangya Hospital, Central South University, Changsha, Hunan, China.

出版信息

J Cell Physiol. 2007 Sep;212(3):764-70. doi: 10.1002/jcp.21074.

DOI:10.1002/jcp.21074
PMID:17525996
Abstract

Smad1 is a receptor-activated intracellular signaling protein, which mediates signal transduction of bone morphogenetic proteins. Current study investigated the expression and transcriptional activity of Smad1 during hepatic stellate cell (HSC) activation. Rat HSCs were isolated from rats at 1, 2, 3 and 4 days after gavaged with carbon tetrachloride (CCl(4)) or corn oil. RT-PCR, Western blot, gel-shift assay and luciferase assay were employed to examine Smad1 expression and transcriptional activity, respectively. CCl(4)-cirrhotic liver fat-storing cells-8B (CFSC-8B) cells were infected with recombinant adenoviruses of Smad1 and/or Smad1 shRNA. Both mRNA and protein levels of Smad1 were significantly increased at 48 h after gavage of CCl(4). Gel shift assays demonstrated a significant increase in nuclear Smad1 in day 9 HSCs. Transfection of HSCs with Smad1 responsible luciferase indicated an increase in Smad1 transcriptional activity in day 6 HSCs (1.563 +/- 0.229 in day 6 versus 0.785 +/- 0.192 in day 3). When CFSC-8B cells were infected with adenoviruses with Smad1 or Smad1 short hairpin RNA (shRNA), there was an increase or decrease in Smad1 mRNA and protein, respectively. Smooth muscle alpha-actin expression was increased or decreased according to induction or reduction of Smad1. In conclusion, there were significantly increases in Smad1 expression and transcriptional activity during in vivo activation of hepatic stellate cells.

摘要

Smad1是一种受体激活的细胞内信号蛋白,介导骨形态发生蛋白的信号转导。当前研究调查了Smad1在肝星状细胞(HSC)激活过程中的表达及转录活性。从用四氯化碳(CCl₄)或玉米油灌胃后1、2、3和4天的大鼠中分离出大鼠HSC。分别采用逆转录聚合酶链反应(RT-PCR)、蛋白质免疫印迹法、凝胶迁移率变动分析和荧光素酶分析来检测Smad1的表达及转录活性。用Smad1和/或Smad1短发夹RNA(shRNA)的重组腺病毒感染CCl₄诱导的肝硬化肝贮脂细胞-8B(CFSC-8B)细胞。灌胃CCl₄后48小时,Smad1的mRNA和蛋白质水平均显著升高。凝胶迁移率变动分析表明,第9天的HSC中核Smad1显著增加。用Smad1反应性荧光素酶转染HSC表明,第6天的HSC中Smad1转录活性增加(第6天为1.563±0.229,第3天为0.785±0.192)。当CFSC-8B细胞用含Smad1的腺病毒或Smad1短发夹RNA(shRNA)感染时,Smad1的mRNA和蛋白质分别增加或减少。平滑肌α-肌动蛋白的表达根据Smad1的诱导或减少而增加或减少。总之,在肝星状细胞的体内激活过程中,Smad1的表达和转录活性显著增加。

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