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Publication : Use of Hes1-GFP reporter mice to assess activity of the Hes1 promoter in bone cells under chronic inflammation.

First Author  Zhang H Year  2016
Journal  Bone Volume  90
Pages  80-9 PubMed ID  27269414
Mgi Jnum  J:235508 Mgi Id  MGI:5796698
Doi  10.1016/j.bone.2016.06.003 Citation  Zhang H, et al. (2016) Use of Hes1-GFP reporter mice to assess activity of the Hes1 promoter in bone cells under chronic inflammation. Bone 90:80-9
abstractText  Notch signaling plays a critical role in maintaining bone homeostasis partially by controlling the formation of osteoblasts from mesenchymal stem cells (MSCs). We reported that TNF activates Notch signaling in MSCs which inhibits osteoblast differentiation in TNF transgenic (TNF-Tg) mice, a mouse model of chronic inflammatory arthritis. In the current study, we used Hes1-GFP and Hes1-GFP/TNF-Tg mice to study the distribution and dynamic change of Notch active cells in normal and inflammatory bone loss and mechanisms mediating their enhanced proliferation. We found that Hes1-GFP+ cells are composed of cells expressing mesenchymal, hematopoietic and endothelial surface markers. CD45-/Hes1-GFP+ cells express high levels of mesenchymal markers and form CFU-F and CFU-ALP colonies. Expansion of CFU-F colonies is associated with a rapid increase in Hes1-GFP+ cell numbers and their GFP intensity. The GFP signal is lost when a CFU-F colony differentiates into an ALP+ osteoblast colony. TNF increases the numbers of CD45-/Hes1-GFP+ cells, which are stained negatively for osteoblast marker osteocalcin and localized adjacent to endosteal and trabecular bone surfaces. CD45-/Hes1-GFP+ cells in Hes1-GFP/TNF-Tg mice have increased BrdU incorporation and PDGFRbeta levels. TNF increases the number of proliferating Hes1-GFP+ cells, which is prevented by a specific PDGFRbeta inhibitor. Notch inhibition blocks TNF-mediated PDGFRbeta expression and cell proliferation. Thus, TNF-induced MSC proliferation is mediated by PDGFRbeta signal, which works at downstream of Notch. Hes1-GFP mice can be used to assess the activation status of Notch in bone cells.
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