The E3 ligase Hrd1 stabilizes Tregs by antagonizing inflammatory cytokine–induced ER stress response
Yuanming Xu, Johanna Melo-Cardenas, Yana Zhang, Isabella Gau, Juncheng Wei, Elena Montauti, Yusi Zhang, Beixue Gao, Hongjian Jin, Zhaolin Sun, Sang-Myeong Lee, Deyu Fang
Yuanming Xu, Johanna Melo-Cardenas, Yana Zhang, Isabella Gau, Juncheng Wei, Elena Montauti, Yusi Zhang, Beixue Gao, Hongjian Jin, Zhaolin Sun, Sang-Myeong Lee, Deyu Fang
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Research Article Immunology

The E3 ligase Hrd1 stabilizes Tregs by antagonizing inflammatory cytokine–induced ER stress response

Abstract

Treg differentiation, maintenance, and function are controlled by the transcription factor FoxP3, which can be destabilized under inflammatory or other pathological conditions. Tregs can be destabilized under inflammatory or other pathological conditions, but the underlying mechanisms are not fully defined. Herein, we show that inflammatory cytokines induce ER stress response, which destabilizes Tregs by suppressing FoxP3 expression, suggesting a critical role of the ER stress response in maintaining Treg stability. Indeed, genetic deletion of Hrd1, an E3 ligase critical in suppressing the ER stress response, leads to elevated expression of ER stress–responsive genes in Treg and largely diminishes Treg suppressive functions under inflammatory condition. Mice with Treg-specific ablation of Hrd1 displayed massive multiorgan lymphocyte infiltration, body weight loss, and the development of severe small intestine inflammation with aging. At the molecular level, the deletion of Hrd1 led to the activation of both the ER stress sensor IRE1α and its downstream MAPK p38. Pharmacological suppression of IRE1α kinase, but not its endoribonuclease activity, diminished the elevated p38 activation and fully rescued the stability of Hrd1-null Tregs. Taken together, our studies reveal ER stress response as a previously unappreciated mechanism underlying Treg instability and that Hrd1 is crucial for maintaining Treg stability and functions through suppressing the IRE1α-mediated ER stress response.

Authors

Yuanming Xu, Johanna Melo-Cardenas, Yana Zhang, Isabella Gau, Juncheng Wei, Elena Montauti, Yusi Zhang, Beixue Gao, Hongjian Jin, Zhaolin Sun, Sang-Myeong Lee, Deyu Fang

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Figure 3

Decreased FoxP3+ Treg frequencies and reduced FoxP3 stability in Hrd1fl/fl-FoxP3cre mice.

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Decreased FoxP3+ Treg frequencies and reduced FoxP3 stability in Hrd1fl/...
(A) Flow cytometry analysis and frequency of FoxP3+ Tregs in WT and Hrd1fl/fl-FoxP3cre young mice (n = 3–14 per group). Thy, thyroid; pLN, popliteal lymph node; mLN, mesenteric lymph node; SPL, spleen; LPL, lamina propria lymphocytes; SI-IEL, small intestinal intraepithelial lymphocytes; PP, Peyer’s patches. (B–D) Representative images and statistical analysis of Helios expression in the CD4+ cells from the pLN and SPL in WT and Hrd1fl/fl-FoxP3cre mice (n = 8–9 per group). (E and F) BrdU staining 24 hours after injection of BrdU (n = 4–6 per group) and Ki67 staining (n = 2–3 per group) in Tregs (CD4+FoxP3+) from the SPL and pLN of WT and Hrd1fl/fl-FoxP3cre mice. (G–I) CD4+CD25+YFP+ Tregs from CD45.2+ WT and Hrd1-cKO mice were sorted, mixed with CD4+ CD45.1 naive T cells, and adoptively transferred into RAG1-null mice. Eight weeks later, CD45.2+CD4+ Tregs were gated, and the expression of FoxP3 were analyzed (G and H). SSC, side scatter The survival of CD45.2 cells were analyzed by Annexin V staining (I) (n = 4 per group). Data are shown as mean ± SD. *P < 0.05 and **P < 0.01 by 2-tailed Student’s t test.