Differential Signalling Through ALK-1 and ALK-5 Regulates Leptin Expression in Mesenchymal Stem Cells

被引:14
|
作者
Zeddou, Mustapha [2 ]
Relic, Biserka [2 ]
Malaise, Olivier [2 ]
Charlier, Edith [2 ]
Desoroux, Aline [2 ]
Beguin, Yves [2 ,3 ]
de Seny, Dominique [2 ]
Malaise, Michel G. [1 ,2 ]
机构
[1] Univ Liege, Dept Rheumatol, GIGA I3, GIGA Res Ctr,Lab Rheumatol, B-4000 Liege, Belgium
[2] CHU Liege, B-4000 Liege, Belgium
[3] Univ Liege, Haematol Lab, GIGA I3, GIGA Res Ctr, B-4000 Liege, Belgium
关键词
ACTIVATED-RECEPTOR-GAMMA; HUMAN ADIPOSE-TISSUE; UMBILICAL-CORD; IN-VITRO; OSTEOARTHRITIS; SECRETION; DEXAMETHASONE; FIBROBLASTS; ADIPOCYTES; APOPTOSIS;
D O I
10.1089/scd.2011.0321
中图分类号
Q813 [细胞工程];
学科分类号
摘要
Leptin plays a central role in maintaining energy balance, with multiple other systemic effects. Despite leptin importance in peripheral regulation of mesenchymal stem cells (MSC) differentiation, little is known about its expression mechanism. Leptin is often described as adipokine, while it is expressed by other cell types. We have recently shown an in vitro leptin expression, enhanced by glucocorticoids in synovial fibroblasts (SVF). Here, we investigated leptin expression in MSC from bone marrow (BM-MSC) and umbilical cord matrix (UMSC). Results showed that BM-MSC, but not UMSC, expressed leptin that was strongly enhanced by glucocorticoids. Transforming growth factor beta 1 (TGF-beta 1) markedly inhibited the endogenous-and glucocorticoid-induced leptin expression in BM-MSC. Since TGF-beta 1 was shown to signal via ALK-5-Smad2/3 and/or ALK-1-Smad1/5 pathways, we analyzed the expression of proteins from both pathways. In BM-MSC, TGF-beta 1 increased phosphorylated Smad2 (p-Smad2) expression, while ALK-5 inhibitor (SB431542) induced leptin expression and significantly restored TGF-beta 1-induced leptin inhibition. In addition, both prednisolone and SB431542 increased p-Smad1/5 expression. These results suggested the ALK-5-Smad2 pathway as an inhibitor of leptin expression, while ALK-1-Smad1/5 as an activator. Indeed, Smad1 expression silencing induced leptin expression inhibition. Furthermore, prednisolone enhanced the expression of TGF-beta RII while decreasing p-Smad2 in BM-MSC and SVF but not in UMSC. In vitro differentiation revealed differential osteogenic potential in SVF, BM-MSC, and UMSC that was correlated to their leptin expression potential. Our results suggest that ALK-1/ALK-5 balance regulates leptin expression in MSC. It also underlines UMSC as leptin nonproducer MSC for cell therapy protocols where leptin expression is not suitable.
引用
收藏
页码:1948 / 1955
页数:8
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