The type III histone deacetylase Sirt1 is essential for maintenance of T cell tolerance in mice
Jinping Zhang, … , Habib Zaghouani, Deyu Fang
Jinping Zhang, … , Habib Zaghouani, Deyu Fang
Published September 1, 2009
Citation Information: J Clin Invest. 2009;119(10):3048-3058. https://doi.org/10.1172/JCI38902.
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Research Article Immunology

The type III histone deacetylase Sirt1 is essential for maintenance of T cell tolerance in mice

Abstract

Although many self-reactive T cells are eliminated by negative selection in the thymus, some of these cells escape into the periphery, where they must be controlled by additional mechanisms. However, the molecular mechanisms underlying peripheral T cell tolerance and its maintenance remain largely undefined. In this study, we report that sirtuin 1 (Sirt1), a type III histone deacetylase, negatively regulates T cell activation and plays a major role in clonal T cell anergy in mice. In vivo, we found that loss of Sirt1 function resulted in abnormally increased T cell activation and a breakdown of CD4+ T cell tolerance. Conversely, upregulation of Sirt1 expression led to T cell anergy, in which the activity of the transcription factor AP-1 was substantially diminished. Furthermore, Sirt1 interacted with and deacetylated c-Jun, yielding an inactive AP-1 factor. In addition, Sirt1-deficient mice were unable to maintain T cell tolerance and developed severe experimental allergic encephalomyelitis as well as spontaneous autoimmunity. These findings provide insight into the molecular mechanisms of T cell activation and anergy, and we suggest that activators of Sirt1 may be useful as therapeutic agents for the treatment and/or prevention of autoimmune diseases.

Authors

Jinping Zhang, Sang-Myeong Lee, Stephen Shannon, Beixue Gao, Weimin Chen, An Chen, Rohit Divekar, Michael W. McBurney, Helen Braley-Mullen, Habib Zaghouani, Deyu Fang

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Figure 2

Analysis of T cell–mediated immune responses.

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Analysis of T cell–mediated immune responses. Sirt1+/– and Sirt1–/– mice...
Sirt1+/– and Sirt1–/– mice were immunized with 200 μg OVA protein in CFA. (AD) Seven days later, mice were euthanized and total splenocytes were cultured with different amounts of OVA. (AD) Proliferation (A) and production of IL-2 (B), IFN-γ (C), and IL-5 (D) were determined. Experiments were repeated 3 times using 6 Sirt1+/– and 6 Sirt1–/– mice. Representative data are shown. (E and F) Sera were obtained 10 days after immunization with OVA/CFA (E) or 7 days after a second immunization with OVA/IFA (F). The concentrations of each isotype of immunoglobulin were determined by ELISA. The arbitrary units of IgG1 shown in the figure were determined after 1:1,000 dilution. Data are from 5 Sirt1+/– and 5 Sirt1–/– mice (mean ± SD).