Antigen receptor-mediated depletion of FOXP3 in induced regulatory T-lymphocytes via PTPN2 and FOXO1

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作者
Evita Bothur
Hartmann Raifer
Claudia Haftmann
Anna-Barbara Stittrich
Anne Brüstle
Dirk Brenner
Nadine Bollig
Maria Bieringer
Chol-Ho Kang
Katharina Reinhard
Bärbel Camara
Magdalena Huber
Alexander Visekruna
Ulrich Steinhoff
Antje Repenning
Uta-Maria Bauer
Veronika Sexl
Andreas Radbruch
Tim Sparwasser
Mir-Farzin Mashreghi
Tak Wah Mak
Michael Lohoff
机构
[1] Institute for Medical Microbiology and Hygiene,Department of Dermatology and Allergy Center
[2] University of Marburg,undefined
[3] German Rheumatism Research Center Berlin,undefined
[4] The John Curtin School of Medical Research,undefined
[5] The Australian National University,undefined
[6] Experimental and Molecular Immunology,undefined
[7] Luxembourg Institute of Health,undefined
[8] Odense Research Center for Anaphylaxis (ORCA),undefined
[9] Odense University Hospital,undefined
[10] University of Southern Denmark,undefined
[11] Institute of Molecular Biology and Tumor Research,undefined
[12] University of Marburg,undefined
[13] Institute for Pharmacology and Toxicology,undefined
[14] University of Veterinary Medicine Vienna,undefined
[15] Institute of Infection Immunology,undefined
[16] TWINCORE,undefined
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摘要
Regulatory T-cells induced via IL-2 and TGFβ in vitro (iTreg) suppress immune cells and are potential therapeutics during autoimmunity. However, several reports described their re-differentiation into pathogenic cells in vivo and loss of their key functional transcription factor (TF) FOXP3 after T-cell antigen receptor (TCR)-signalling in vitro. Here, we show that TCR-activation antagonizes two necessary TFs for foxp3 gene transcription, which are themselves regulated by phosphorylation. Although the tyrosine phosphatase PTPN2 is induced to restrain IL-2-mediated phosphorylation of the TF STAT5, expression of the TF FOXO1 is downregulated and miR-182, a suppressor of FOXO1 expression, is upregulated. TGFβ counteracts the FOXP3-depleting TCR-signal by reassuring FOXO1 expression and by re-licensing STAT5 phosphorylation. Overexpressed phosphorylation-independent active versions of FOXO1 and STAT5 or knockdown of PTPN2 restores FOXP3 expression despite TCR-signal and absence of TGFβ. This study suggests novel targets for stabilisation and less dangerous application of iTreg during devastating inflammation.
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