Activation of a TGF-β-Specific Multistep Gene Expression Program in Mature Macrophages Requires Glucocorticoid-Mediated Surface Expression of TGF-β Receptor II | Zendy

Alexei Gratchev | Zendy; Julia Kzhyshkowska | Zendy; Sheila Kannookadan | Zendy; Miriam Ochsenreiter | Zendy; А. Н. Попова | Zendy; Xiaolei Yu | Zendy; Srinivas Mamidi | Zendy; Eugenia Stonehouse-Usselmann | Zendy; Isabelle MullerMolinet | Zendy; LiMing Gooi | Zendy; Sergij Goerdt | Zendy

Open Access

Activation of a TGF-β-Specific Multistep Gene Expression Program in Mature Macrophages Requires Glucocorticoid-Mediated Surface Expression of TGF-β Receptor II

Author(s) -

Alexei Gratchev,

Julia Kzhyshkowska,

Sheila Kannookadan,

Miriam Ochsenreiter,

А. Н. Попова,

Xiaolei Yu,

Srinivas Mamidi,

Eugenia Stonehouse-Usselmann,

Isabelle MullerMolinet,

LiMing Gooi,

Sergij Goerdt

Publication year - 2008

Publication title -

the journal of immunology

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 2.737

H-Index - 372

eISSN - 1550-6606

pISSN - 0022-1767

DOI - 10.4049/jimmunol.180.10.6553

Subject(s) - transforming growth factor , receptor , inflammation , tgf beta signaling pathway , cytokine , biology , transforming growth factor beta , signal transduction , microbiology and biotechnology , glucocorticoid , chemistry , cancer research , endocrinology , immunology , biochemistry

Alternatively activated (M2) macrophages regulate steady state-, cancer-, and inflammation-related tissue remodeling. They are induced by Th2-cytokines and glucocorticoids (GC). The responsiveness of mature macrophages to TGF-beta, a cytokine involved in inflammation, cancer, and atherosclerosis, is currently controversial. Recently, we demonstrated that IL-17 receptor B is up-regulated in human monocyte-derived macrophages differentiated in the presence of Th2 cytokines IL-4 and TGF-beta1. In this study, we show that mature human macrophages differentiated in the presence of IL-4, and dexamethasone (M2(IL-4/GC)) but not M2(IL-4) responds to TGF-beta1 which induced a gene expression program comprising 111 genes including transcriptional/signaling regulators (ID3 and RGS1), immune modulators (ALOX5AP and IL-17 receptor B) and atherosclerosis-related genes (ALOX5AP, ORL1, APOC1, APOC2, and APOE). Analysis of molecular mechanism underlying GC/TGF-beta cooperation revealed that surface expression of TGF-betaRII was high in M2(GC) and M2(IL-4/GC), but absent from M2(IL-4), whereas the expression of TGF-betaRI/II mRNA, TGF-betaRII total protein, and surface expression of TGF-betaRIII were unchanged. GC dexamethasone was essential for increased surface expression of functional TGF-betaRII because its effect was observed also in combination with IL-13, M-CSF, and GM-CSF. Prolonged Smad2-mediated signaling observed in TGF-beta1-treated M2(IL-4/GC) was due to insufficient activity of negative feedback mechanism what can be explained by up-regulation of SIRT1, a negative regulator of Smad7, and the retention of TGF-betaRII complex on the cell surface. In summary, mature human M2 macrophages made permissive to TGF-beta by GC-induced surface expression of TGF-betaRII activate in response to TGF-beta1, a multistep gene expression program featuring traits of macrophages found within an atherosclerotic lesion.

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