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CD103+ dendritic cell–fibroblast crosstalk via TLR9, TDO2, and AHR signaling drives lung fibrogenesis
Hannah Carter, Rita Medina Costa, Taylor S. Adams, Talon M. Gilchrist, Claire E. Emch, Monica Bame, Justin M. Oldham, Steven K. Huang, Angela L. Linderholm, Imre Noth, Naftali Kaminski, Bethany B. Moore, Stephen J. Gurczynski
Hannah Carter, Rita Medina Costa, Taylor S. Adams, Talon M. Gilchrist, Claire E. Emch, Monica Bame, Justin M. Oldham, Steven K. Huang, Angela L. Linderholm, Imre Noth, Naftali Kaminski, Bethany B. Moore, Stephen J. Gurczynski
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Research Article Immunology Pulmonology

CD103+ dendritic cell–fibroblast crosstalk via TLR9, TDO2, and AHR signaling drives lung fibrogenesis

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Abstract

Idiopathic pulmonary fibrosis (IPF) is characterized by progressive scarring and loss of lung function. With limited treatment options, patients die from the disease within 2–5 years. The molecular pathogenesis underlying the immunologic changes that occur in IPF is poorly understood. We characterize noncanonical aryl-hydrocarbon receptor (ncAHR) signaling in DCs as playing a role in the production of IL-6 and increased IL-17+ cells, promoting fibrosis. TLR9 signaling in myofibroblasts is shown to regulate production of TDO2, which converts tryptophan into the endogenous AHR ligand kynurenine. Mice with augmented ncAHR signaling were created by crossing mice harboring a floxed AHR exon 2 deletion (AHRΔex2) with mice harboring a CD11c-Cre. Bleomycin (blm) was used to study fibrotic pathogenesis. Isolated CD11c+ cells and primary fibroblasts were treated ex vivo with relevant TLR agonists and AHR-modulating compounds to study how AHR signaling influenced inflammatory cytokine production. Human datasets were also interrogated. Inhibition of all AHR signaling rescued fibrosis; however, AHRΔex2 mice treated with blm developed more fibrosis, and DCs from these mice were hyperinflammatory and profibrotic upon adoptive transfer. Treatment of fibrotic fibroblasts with TLR9 agonist increased expression of TDO2, and fibrotic fibroblasts activated IL-6 production in CD103+ DCs. Study of human samples corroborated the relevance of these findings in patients with IPF. We also show, for the first time to our knowledge, that AHR exon 2 floxed mice retain the capacity for ncAHR signaling.

Authors

Hannah Carter, Rita Medina Costa, Taylor S. Adams, Talon M. Gilchrist, Claire E. Emch, Monica Bame, Justin M. Oldham, Steven K. Huang, Angela L. Linderholm, Imre Noth, Naftali Kaminski, Bethany B. Moore, Stephen J. Gurczynski

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Figure 5

ncAHR signaling in CD103+ DCs drives IL-17 production from ILC3 in the lung.

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ncAHR signaling in CD103+ DCs drives IL-17 production from ILC3 in the l...
(A) WT B6 or AHRΔex2 mice (n = 3–5 per group) were treated (oropharyngeal delivery) with 0.75 U/kg blm. Seven days after blm treatment, lungs were harvested, and lung leukocytes were analyzed by flow cytometry for the following populations: Th17 (CD45+, Thy1.2+, CD3+, CD4+, IL-17A+), IL-17+ γδ T cell (CD45+, Thy1.2+, CD3+, CD4-, γδ-TCR+, IL-17A+), IL-17+ ILC3 (CD45+, Thy1.2+, CD3–, CD4–, IL-17+), IL-17A+ iNKT (CD45+, Thy1.2+, CD4–, CD3+, γδ TCR+, IL-17A+). (B) Quantification of cell populations identified in A. (C) WT B6 or AHRΔex2 mice were treated with 0.75 U/kg blm, and CH223191 (CH223) was administered from day 10 to day 18 after blm. Lungs were harvested at 21 days after blm treatment, and expression of IL-17 transcript was quantified via qRT-PCR. (D) Mice (n = 5–8 per group) were treated with 0.75 U/kg blm. Twenty-one days after blm treatment, lungs were harvested, and expression of IL-17 transcript from whole lung was analyzed via qRT-PCR. (E–G) Mice (n = 5 per group) were treated with 0.75 U/kg blm. Fourteen days after treatment, lung leukocytes were isolated via collagenase digestion and analyzed for the indicated cell population by flow cytometry: IL-17 γδ TCR+ (Thy1.2+, CD3+, CD4/8–, γδ TCR+, IL-17+), Th17 (Thy1.2+, CD3+, CD4+, IL-17+), ILC3 (Thy1.2+, CD3-, CD4/8–, IL-17+). All data are representative of at least 3 independent experiments; statistical significance was determined via ANOVA (*P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001).

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