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 8

Deficiency of PAD2 increases the susceptibility to allergic airway inflammation.

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Deficiency of PAD2 increases the susceptibility to allergic airway infla...
(AG) Allergic airway inflammation was induced in WT DBA/1J and PAD2-KO mice (n = 12 per group) according to the protocol described in Methods. Representative H&E staining of lung sections from immunized/unchallenged WT DBA/1J (imm), immunized/challenged WT DBA/1J (WT/imm+cha), and immunized/challenged PAD2-KO (KO/imm+cha) mice were shown in A. Scale bars: 100 μm. The total number of cells in bronchial lavage is shown in B. Eosinophils in bronchial lavage were identified with FACS as CD11b+Siglec-F+ cells. Representative FACS plots are shown in C. The percentage and total number of eosinophils in bronchial lavage are shown in D. Mucus-producing cells were identified with PAS stain (bright pink stain). Representative sections are shown in E. Scale bars: 100 µm. The transcript levels of indicated Th2 and Th17 cytokines in lung tissue were measured with real-time PCR and shown in F and G, respectively. Statistical analysis was performed with 2-tailed Student’s t test.