Reciprocal regulation of Th2 and Th17 cells by PAD2-mediated citrullination
Bo Sun, Hui-Hsin Chang, Ari Salinger, Beverly Tomita, Mandar Bawadekar, Caitlyn L. Holmes, Miriam A. Shelef, Eranthie Weerapana, Paul R. Thompson, I-Cheng Ho
Bo Sun, Hui-Hsin Chang, Ari Salinger, Beverly Tomita, Mandar Bawadekar, Caitlyn L. Holmes, Miriam A. Shelef, Eranthie Weerapana, Paul R. Thompson, I-Cheng Ho
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Research Article Immunology

Reciprocal regulation of Th2 and Th17 cells by PAD2-mediated citrullination

Abstract

Dysregulated citrullination, a unique form of posttranslational modification catalyzed by the peptidylarginine deiminases (PADs), has been observed in several human diseases, including rheumatoid arthritis. However, the physiological roles of PADs in the immune system are still poorly understood. Here, we report that global inhibition of citrullination enhances the differentiation of type 2 helper T (Th2) cells but attenuates the differentiation of Th17 cells, thereby increasing the susceptibility to allergic airway inflammation. This effect on Th cells is due to inhibition of PAD2 but not PAD4. Mechanistically, PAD2 directly citrullinates GATA3 and RORγt, 2 key transcription factors determining the fate of differentiating Th cells. Citrullination of R330 of GATA3 weakens its DNA binding ability, whereas citrullination of 4 arginine residues of RORγt strengthens its DNA binding. Finally, PAD2-deficient mice also display altered Th2/Th17 immune response and heightened sensitivity to allergic airway inflammation. Thus, our data highlight the potential and caveat of PAD2 as a therapeutic target of Th cell–mediated diseases.

Authors

Bo Sun, Hui-Hsin Chang, Ari Salinger, Beverly Tomita, Mandar Bawadekar, Caitlyn L. Holmes, Miriam A. Shelef, Eranthie Weerapana, Paul R. Thompson, I-Cheng Ho

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Figure 4

PAD2 physically interacts with GATA3 and RORγt.

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PAD2 physically interacts with GATA3 and RORγt. Whole cells extract was ...
Whole cells extract was prepared from differentiated WT DBA/1J (W) and PAD2-KO (K) Th2 (A) and Th17 (B) cells and subjected to immunoprecipitation with anti-GATA3 (A), anti-RORγt (B) or control IgG (A and B). The immunoprecipitate was probed with anti-PAD2 in Western blotting (top panels). A fraction of the unprecipitated extract was probed with anti-GATA3 (A), anti-RORγt (B) and anti-Lamin B as input control (middle and bottom panels). Representative Western blots from 2 experiments are shown. (CE) GST-PAD2 (C and D), GST-GATA3 (E, left panels), or GST-RORγt (E, right panels) was used to pull down various truncated His-tagged GATA3 (C), RORγt (D), or PAD2 (E) expressed in HEK-293 cells. Whole cell extract from the transfected HEK-293T cells (the bottom panels) and pulldown extract (the top panels) were probed with anti-His. Schematic diagrams of truncated GATA3 (C), RORγt (D), and PAD2 (E) are also shown. The asterisks in the Western blots of CE mark exogenous His-GATA3 (C), His-RORγt (D), and His-PAD2 (E). Representative Western blots from 3 experiments are shown in CE. TA, transactivation domain; Zn, zinc finger; DBD, DNA binding domain; LBD, ligand binding domain; Ig, immunoglobulin domain; and FL, full length.