Dendritic cells expressing immunoreceptor CD300f are critical for controlling chronic gut inflammation
Ha-Na Lee, … , John E. Coligan, Konrad Krzewski
Ha-Na Lee, … , John E. Coligan, Konrad Krzewski
Published April 17, 2017
Citation Information: J Clin Invest. 2017;127(5):1905-1917. https://doi.org/10.1172/JCI89531.
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Research Article Immunology Inflammation

Dendritic cells expressing immunoreceptor CD300f are critical for controlling chronic gut inflammation

Abstract

Proinflammatory cytokine overproduction and excessive cell death, coupled with impaired clearance of apoptotic cells, have been implicated as causes of failure to resolve gut inflammation in inflammatory bowel diseases. Here we have found that dendritic cells expressing the apoptotic cell–recognizing receptor CD300f play a crucial role in regulating gut inflammatory responses in a murine model of colonic inflammation. CD300f-deficient mice failed to resolve dextran sulfate sodium–induced colonic inflammation as a result of defects in dendritic cell function that were associated with abnormal accumulation of apoptotic cells in the gut. CD300f-deficient dendritic cells displayed hyperactive phagocytosis of apoptotic cells, which stimulated excessive TNF-α secretion predominantly from dendritic cells. This, in turn, induced secondary IFN-γ overproduction by colonic T cells, leading to prolonged gut inflammation. Our data highlight a previously unappreciated role for dendritic cells in controlling gut homeostasis and show that CD300f-dependent regulation of apoptotic cell uptake is essential for suppressing overactive dendritic cell–mediated inflammatory responses, thereby controlling the development of chronic gut inflammation.

Authors

Ha-Na Lee, Linjie Tian, Nicolas Bouladoux, Jacquice Davis, Mariam Quinones, Yasmine Belkaid, John E. Coligan, Konrad Krzewski

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Figure 3

Identification of cells producing TNF-α and IFN-γ in the inflamed colon tissue.

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Identification of cells producing TNF-α and IFN-γ in the inflamed colon ...
Lamina propria cells were isolated from the colons of DSS-treated CD300f+/+ or CD300f–/– mice, collected on day 7 (A and C) or day 14 (B and D). The intracellular expression of TNF-α and IFN-γ was determined by flow cytometry in the following cell populations: macrophages (CD45+F4/80+CD11b+CD14+Ly6GCD11c), DCs (CD45+CD11c+F4/80Ly6GCD64), neutrophils (CD45+CD11b+Ly6G+CD11cF4/80), mast cells (CD45+CD11b+FcεRI+), T cells (CD45+CD3+), B cells (CD45+CD3CD19+), NK cells (CD45+CD3NK1.1+), and NKT cells (CD45+CD3+NK1.1+). The graphs show the percentages (left) and total numbers (right) of cells expressing TNF-α (A and B) or IFN-γ (C and D). Data are expressed as means + SEM (n = 3–8, each group). Two-tailed paired Student’s t test was used to determine statistical significance (*P < 0.05, **P < 0.01, ***P < 0.001).