TSLP/dendritic cell axis promotes CD4+ T cell tolerance to the gut microbiome
Jonathan L. Messerschmidt, … , Kaitlin E. Dempsey, Shadmehr Demehri
Jonathan L. Messerschmidt, … , Kaitlin E. Dempsey, Shadmehr Demehri
Published July 10, 2023
Citation Information: JCI Insight. 2023;8(13):e160690. https://doi.org/10.1172/jci.insight.160690.
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Research Article Gastroenterology Immunology

TSLP/dendritic cell axis promotes CD4+ T cell tolerance to the gut microbiome

Abstract

Thymic stromal lymphopoietin (TSLP) overexpression is widely associated with atopy. However, TSLP is expressed in normal barrier organs, suggesting a homeostatic function. To determine the function of TSLP in barrier sites, we investigated the impact of endogenous TSLP signaling on the homeostatic expansion of CD4+ T cells in adult mice. Surprisingly, incoming CD4+ T cells induced lethal colitis in adult Rag1-knockout animals that lacked the TSLP receptor (Rag1KOTslprKO). Endogenous TSLP signaling was required for reduced CD4+ T cell proliferation, Treg differentiation, and homeostatic cytokine production. CD4+ T cell expansion in Rag1KOTslprKO mice was dependent on the gut microbiome. The lethal colitis was rescued by parabiosis between Rag1KOTslprKO and Rag1KO animals and wild-type dendritic cells (DCs) suppressed CD4+ T cell–induced colitis in Rag1KOTslprKO mice. A compromised T cell tolerance was noted in TslprKO adult colon, which was exacerbated by anti–PD-1 and anti–CTLA-4 therapy. These results reveal a critical peripheral tolerance axis between TSLP and DCs in the colon that blocks CD4+ T cell activation against the commensal gut microbiome.

Authors

Jonathan L. Messerschmidt, Marjan Azin, Kaitlin E. Dempsey, Shadmehr Demehri

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Figure 2

CD4+ T cells massively expand in TSLP receptor–deficient colon.

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CD4+ T cells massively expand in TSLP receptor–deficient colon. (A) Repr...
(A) Representative CD3/CD4 staining of Rag1KOTslprKO and Rag1KO colons at the moribund state or 15 days after CD4+ T cell transfer. Scale bar: 50 μm. (B) CD4+ T cell counts in Rag1KOTslprKO (n = 5) and Rag1KO (n = 5) colons from 1 experiment that was validated in a second independent experiment. CD4+CD3+ cells were counted in 10 randomly selected high-powered fields (HPFs, overall magnification ×200) per colon. Each dot represents 1 HPF. (CE) Flow cytometric quantification of CD4+ T (C), Ki67+CD4+ T (D), and Foxp3+CD4+ Treg (E) frequency of MLNs from Rag1KOTslprKO (n = 5) and Rag1KO (n = 5) mice. Experimental data were verified in a second independent experiment. (FH) Flow cytometric quantification of CD4+ T (F), Ki67+CD4+ T (G), and Foxp3+CD4+ Treg (H) frequency in Rag1KOTslprKO (n = 5) and Rag1KO (n = 5) colons. Experimental data were verified in a second independent experiment. (IL) Flow cytometric quantification of IFN-γ+ (I), IL-17A+ (J), IL-10+ (K), and IL-4+ (L) CD4+ T cell frequency of MLNs from Rag1KOTslprKO (n = 5) and Rag1KO (n = 5) mice. Experimental data were verified in a second independent experiment. (MP) Flow cytometric quantification of IFN-γ+ (M), IL-17A+ (N), IL-10+ (O), and IL-4+ (P) CD4+ T cell frequency in Rag1KOTslprKO (n = 5) and Rag1KO (n = 5) colons. Experimental data were verified in a second independent experiment. Single-cell suspensions from MLNs and colon were stimulated for 4 hours with PMA/ionomycin + brefeldin A and analyzed for cytokine production. Each dot represents 1 mouse; bar graphs show mean + SD. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001 by unpaired, 2-tailed t test. NS, not significant.