PPP2R2D suppresses IL-2 production and Treg function
Wenliang Pan, Amir Sharabi, Andrew Ferretti, Yinfeng Zhang, Catalina Burbano, Nobuya Yoshida, Maria G. Tsokos, George C. Tsokos
Wenliang Pan, Amir Sharabi, Andrew Ferretti, Yinfeng Zhang, Catalina Burbano, Nobuya Yoshida, Maria G. Tsokos, George C. Tsokos
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Research Article Immunology

PPP2R2D suppresses IL-2 production and Treg function

Abstract

Protein phosphatase 2A is a ubiquitously expressed serine/threonine phosphatase that comprises a scaffold, a catalytic, and multiple regulatory subunits and has been shown to be important in the expression of autoimmunity. We considered that a distinct subunit may account for the decreased production of IL-2 in people and mice with systemic autoimmunity. We show that the regulatory subunit PPP2R2D is increased in T cells from people with systemic lupus erythematosus and regulates IL-2 production. Mice lacking PPP2R2D only in T cells produce more IL-2 because the IL-2 gene and genes coding for IL-2–enhancing transcription factors remain open, while the levels of the enhancer phosphorylated CREB are high. Mice with T cell–specific PPP2R2D deficiency display less systemic autoimmunity when exposed to a TLR7 stimulator. While genes related to Treg function do not change in the absence of PPP2R2D, Tregs exhibit high suppressive function in vitro and in vivo. Because the ubiquitous expression of protein phosphatase 2A cannot permit systemic therapeutic manipulation, the identification of regulatory subunits able to control specific T cell functions opens the way for the development of novel, function-specific drugs.

Authors

Wenliang Pan, Amir Sharabi, Andrew Ferretti, Yinfeng Zhang, Catalina Burbano, Nobuya Yoshida, Maria G. Tsokos, George C. Tsokos

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Figure 4

PPP2R2D deficiency enhances IL-2 production by T cells.

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PPP2R2D deficiency enhances IL-2 production by T cells. Splenic CD4+ or ...
Splenic CD4+ or CD8+ T cells were isolated from R2Dfl/fl and LckCreR2Dfl/fl mice. (AC) Splenic CD4+ or CD8+ T cells were stimulated with phorbol myristate acetate (PMA)/ionomycin and brefeldin A for 4 hours before subjected to FACS analysis of intracellular staining of IL-2 production. Representative flow cytometry plots were shown in A. Cumulative data (n = 6 mice/group) from individual mice depicting the percentages of IL-2–producing cells (B) and the expression of IL-2 (C) were presented. MFI, mean fluorescence intensity. (D) The mRNA expression level of PPP2R2D and IL-2 in R2Dfl/fl and LckCreR2Dfl/fl T cells. Splenic CD4+ T cells were stimulated with plate-bound anti-CD3 and anti-CD28 for 6 hours before extraction of RNA for quantitative PCR analysis. Data are shown as n = 3 mice/group with 2 technical replicates for each mouse. (E) The promoter activity of IL-2 in R2Dfl/fl and LckCreR2Dfl/fl T cells. Splenic CD4+ T cells were nucleofected with IL-2 promoter by using Amaxa Nucleofector electroporation, rested overnight, and stimulated with plate-bound anti-CD3 and anti-CD28 for 24 hours before measurement of luciferase activity. Data are shown as n = 3 mice/group with 2 technical replicates for each mouse. (F and G) Splenic CD4+ T cells were stimulated with plate-bound anti-CD3 and anti-CD28 for 6 hours. (F) Western blot analysis of PPP2R2D, p-CREB, CREB, and β-actin in T cells. Representative immunoblots and cumulative data (n = 3 mice/group, right) are presented. (G) Co-IP analysis of PP2AC and CREB in T cells. The blot is representative of 3 independent experiments. **P < 0.01, ***P < 0.001, ****P < 0.001 using unpaired t test.