DOCK8 enforces immunological tolerance by promoting IL-2 signaling and immune synapse formation in Tregs
Erin Janssen, Sudha Kumari, Mira Tohme, Sumana Ullas, Victor Barrera, Jeroen M.J. Tas, Marcela Castillo-Rama, Roderick T. Bronson, Shariq M. Usmani, Darrell J. Irvine, Thorsten R. Mempel, Raif S. Geha
Erin Janssen, Sudha Kumari, Mira Tohme, Sumana Ullas, Victor Barrera, Jeroen M.J. Tas, Marcela Castillo-Rama, Roderick T. Bronson, Shariq M. Usmani, Darrell J. Irvine, Thorsten R. Mempel, Raif S. Geha
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Research Article Immunology

DOCK8 enforces immunological tolerance by promoting IL-2 signaling and immune synapse formation in Tregs

Abstract

Patients deficient in the guanine nucleotide exchange factor DOCK8 have decreased numbers and impaired in vitro function of Tregs and make autoantibodies, but they seldom develop autoimmunity. We show that, similarly, Dock8–/– mice have decreased numbers and impaired in vitro function of Tregs but do not develop autoimmunity. In contrast, mice with selective DOCK8 deficiency in Tregs develop lymphoproliferation, autoantibodies, and gastrointestinal inflammation, despite a normal percentage and in vitro function of Tregs, suggesting that deficient T effector cell function might protect DOCK8-deficient patients from autoimmunity. We demonstrate that DOCK8 associates with STAT5 and is important for IL-2–driven STAT5 phosphorylation in Tregs. DOCK8 localizes within the lamellar actin ring of the Treg immune synapse (IS). Dock8–/– Tregs have abnormal TCR-driven actin dynamics, decreased adhesiveness, an altered gene expression profile, an unstable IS with decreased recruitment of signaling molecules, and impaired transendocytosis of the costimulatory molecule CD86. These data suggest that DOCK8 enforces immunological tolerance by promoting IL-2 signaling, TCR-driven actin dynamics, and the IS in Tregs.

Authors

Erin Janssen, Sudha Kumari, Mira Tohme, Sumana Ullas, Victor Barrera, Jeroen M.J. Tas, Marcela Castillo-Rama, Roderick T. Bronson, Shariq M. Usmani, Darrell J. Irvine, Thorsten R. Mempel, Raif S. Geha

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Figure 7

DOCK8-deficient Tregs have decreased expression of cytoskeleton- and Treg-associated genes.

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DOCK8-deficient Tregs have decreased expression of cytoskeleton- and Tre...
(A and B) CD4+CD25+CD39+YFP+ (DOCK8-deficient) and YFP (DOCK8-sufficient) Tregs were sorted from Foxp3YFP–Cre/+/Dock8flox/flox female mice. Tregs were cultured overnight in media alone (A) or with anti-CD3+CD28 beads (B). Heatmaps of selected genes differentially expressed in YFP+ and YFP Tregs from Foxp3YFP–Cre/+Dock8flox/flox female mice. The cutoff for significance was P < 0.05. P values were calculated using the Wald test for differential expression analysis. P values were corrected afterward for multiple testing. Expression of genes is centered and scaled by row to highlight differences in each gene sample. Each column represents an individual mouse. (C and D) CD4+CD25+CD39+ Tregs were FACS sorted from Dock8–/– and WT mice. RNA was prepared from Tregs directly after isolation (C) or after 24-hour culture with anti-CD3+CD28 beads (C and D). qPCR results are expressed as fold increase of mRNA of interest/b2microglobulin ratio relative to the unstimulated WT Tregs. (E) MFI of surface marker staining on YFP DOCK8-sufficient and YFP+ DOCK8-deficient CD4+CD25+CD39+ Tregs from Foxp3YFP–Cre/+/Dock8flox/flox female mice. Symbols represent individual mice. Bars in CE represent the mean and SEM. t test, NS P > 0.05, *P < 0.05, ***P < 0.001.