Podoplanin is a negative regulator of Th17 inflammation
Alyssa N. Nylander, … , David Pitt, David A. Hafler
Alyssa N. Nylander, … , David Pitt, David A. Hafler
Published September 7, 2017
Citation Information: JCI Insight. 2017;2(17):e92321. https://doi.org/10.1172/jci.insight.92321.
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Research Article Immunology

Podoplanin is a negative regulator of Th17 inflammation

Abstract

Recent data indicate that there are different subpopulations of Th17 cells that can express a regulatory as opposed to an inflammatory gene signature. The transmembrane glycoprotein PDPN is critical in the development of multiple organs including the lymphatic system and has been described on T cells in mouse models of autoimmune Th17 inflammation. Here, we demonstrate that unlike in mice, PDPN+ T cells induced under classic Th17-polarizing conditions express transcription factors associated with Th17 cells but do not produce IL-17. Moreover, these cells express a transcriptional profile enriched for immunosuppressive and regulatory pathways and express a distinct cytokine profile compared with potentially pathogenic PDPN– Th17 cells. Ligation of PDPN by its ligand CLEC-2 ameliorates the Th17 inflammatory response. IL-17 secretion is restored with shRNA gene silencing of PDPN. Furthermore, PDPN expression is reduced via an Sgk1-mediated pathway under proinflammatory, high sodium chloride conditions. Finally, CD3+PDPN+ T cells are devoid of IL-17 in skin biopsies from patients with candidiasis, a prototypical Th17-driven skin disease. Thus, our data support the hypothesis that PDPN may serve as a marker of a nonpathogenic Th17 cell subset and may also functionally regulate pathogenic Th17 inflammation.

Authors

Alyssa N. Nylander, Gerald D. Ponath, Pierre-Paul Axisa, Mayyan Mubarak, Mary Tomayko, Vijay K. Kuchroo, David Pitt, David A. Hafler

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Figure 3

The reduction in PDPN expression under high salt Th17 conditions correlates with increased IL-17 production and is mediated through Sgk1.

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The reduction in PDPN expression under high salt Th17 conditions correla...
(A) Naive CD4+ T cells were cultured for 1 week under Th17 conditions with or without an additional 40 mM NaCl. Flow cytometry plot is representative of n = 15. (B) Frequency of PDPN+ CD4+ T cells under Th17 and Th17 + NaCl conditions was determined by flow cytometry. Analyzed by unpaired 2-tailed t test. n = 10. (C) Linear regression in which each data point represents the percentage of PDPN+ and IL-17A+ CD4+ T cells in a separate culture. (D and E) Sgk1 shRNA or nontarget control shRNA was added to CD4+ T cells and cultured under Th17 or Th17 + NaCl conditions. Gene expression was evaluated by quantitative PCR relative to β2-microglobulin (β2M) on day 4 and 7. Analyzed by 2-way ANOVA. n = 3–4. (F) Expression of PDPN and cytokines shown in representative flow cytometry plot under Th17 + NaCl conditions. n = 4. **P < 0.01, ****P < 0.0001. Graph shows mean ± SEM.