The E3 ligases Itch and WWP2 cooperate to limit TH2 differentiation by enhancing signaling through the TCR

The mechanisms by which the sensitivity of naive CD4 + T cells to stimulation by the cognate antigen via the T cell antigen receptor (TCR) determines their differentiation into distinct helper T cell subsets remain elusive. Here we demonstrate functional collaboration of the ubiquitin E3 ligases Itc...

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Published inNature immunology Vol. 19; no. 7; pp. 766 - 775
Main Authors Aki, Daisuke, Li, Hui, Zhang, Wen, Zheng, Mingke, Elly, Chris, Lee, Jee H., Zou, Weiguo, Liu, Yun-Cai
Format Journal Article
LanguageEnglish
Published New York Nature Publishing Group US 20.06.2018
Nature Publishing Group
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Summary:The mechanisms by which the sensitivity of naive CD4 + T cells to stimulation by the cognate antigen via the T cell antigen receptor (TCR) determines their differentiation into distinct helper T cell subsets remain elusive. Here we demonstrate functional collaboration of the ubiquitin E3 ligases Itch and WWP2 in regulating the strength of the TCR signal. Mice lacking both Itch and WWP2 in T cells showed spontaneous autoimmunity and lung inflammation. CD4 + T cells deficient in Itch and WWP2 exhibited hypo-responsiveness to TCR stimulation and a bias toward differentiation into the T H 2 subset of helper T cells. Itch and WWP2 formed a complex and cooperated to enhance TCR-proximal signaling by catalyzing the conjugation of atypical ubiquitin chains to the phosphatase SHP-1 and reducing the association of SHP-1 with the tyrosine kinase Lck. These findings indicate that targeted ubiquitination regulates the strength of the TCR signal and differentiation toward the T H 2 lineage. Liu and colleagues show that the ubiquitin E3 ligases Itch and WWP2 act together in regulating the strength of the TCR signal and differentiation toward the T H 2 lineage.
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D.A., H.L., and W. Zhang performed experiments and analyzed data; M.Z., C.E. and J.H.L. prepared reagents and maintained mouse breeding colonies; W. Zou provided the Wwp2−/− mouse strain and performed initial proteomics analysis; and D.A. and Y.-C.L. designed the study and wrote the manuscript.
Author contributions
ISSN:1529-2908
1529-2916
DOI:10.1038/s41590-018-0137-8