IL-27 targets Foxp3+ Tregs to mediate antiinflammatory functions during experimental allergic airway inflammation
Quang Tam Nguyen, Eunjung Jang, Hongnga T. Le, Sohee Kim, Dongkyun Kim, Nina Dvorina, Mark A. Aronica, William M. Baldwin III, Kewal Asosingh, Suzy Comhair, Booki Min
Quang Tam Nguyen, Eunjung Jang, Hongnga T. Le, Sohee Kim, Dongkyun Kim, Nina Dvorina, Mark A. Aronica, William M. Baldwin III, Kewal Asosingh, Suzy Comhair, Booki Min
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Research Article Immunology

IL-27 targets Foxp3+ Tregs to mediate antiinflammatory functions during experimental allergic airway inflammation

Abstract

Foxp3+ CD4 Tregs are central regulators of inflammation, including allergic inflammation in the lung. There is increasing evidence that inflammatory factors undermine adequate Treg functions and homeostasis, resulting in prolonged and exacerbated inflammation. Therefore, identifying the factors is of the utmost important. IL-27 is an antiinflammatory cytokine implicated in immune regulation and tolerance. However, the cellular mechanisms underlying IL-27–mediated immune regulation in vivo remain largely unknown. Utilizing a cockroach antigen–induced allergic inflammation model in mice, we sought to test the roles of Tregs during IL-27–mediated regulation of allergic inflammation. Intranasally delivered IL-27 significantly reduced the development of airway inflammation. Unexpectedly, the IL-27–induced reduction occurred only in the presence of Tregs. Il27ra–/– and Treg-specific Il27ra–/– mice developed severe airway inflammation, and IL-27 treatment had little impact on diminishing the inflammatory responses. IL-27–induced treatment was restored following transfer of WT Tregs but not of Tregs deficient in Lag3, a molecule induced by IL-27 in Tregs. Finally, Tregs from asthmatic patients exhibited blunted STAT1 phosphorylation following IL-27 stimulation. Taken together, our results uncover that Tregs are the primary target cells of IL-27 in vivo to mediate its antiinflammatory functions, suggesting that altered IL-27 responsiveness in Tregs may underlie inadequate Treg functions and perpetuation of inflammation.

Authors

Quang Tam Nguyen, Eunjung Jang, Hongnga T. Le, Sohee Kim, Dongkyun Kim, Nina Dvorina, Mark A. Aronica, William M. Baldwin III, Kewal Asosingh, Suzy Comhair, Booki Min

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Figure 4

Treg-specific Il27ra−/− mice have exacerbated allergic airway inflammation.

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Treg-specific Il27ra−/− mice have exacerbated allergic airway inflammati...
Treg-specific Il27ra–/– (TregΔIl27ra) and littermate control mice were sensitized with CA in alum adjuvant and intranasally challenged as described above. (A) BAL cells were examined for Ly6G and Siglec F expression, and differential cell counts was performed by FACS. (B) Lung cells were stimulated ex vivo, and intracellular cytokine expression was determined. (C) Histology score was determined. (D) Foxp3+ Tregs were enumerated from the indicated tissues. (E) IL-27 was intranasally administered during antigen challenge as described in Figure 1. Relative CD4 accumulation in the lung, as well as cytokine expression, were compared. The data shown represent the mean ± SD of more than 2 independent experiments (n = 11–13). Each symbol represents an individually tested mouse. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001 as determined by Mann-Whitney nonparametric test. BAL, bronchoalveolar lavage; Eos, eosinophils; Neu, neutrophils.