CCR6-deficient mice have impaired leukocyte homeostasis and altered contact hypersensitivity and delayed-type hypersensitivity responses
Rosa Varona, Ricardo Villares, Laura Carramolino, Íñigo Goya, Ángel Zaballos, Julio Gutiérrez, Miguel Torres, Carlos Martínez-A., Gabriel Márquez
Rosa Varona, Ricardo Villares, Laura Carramolino, Íñigo Goya, Ángel Zaballos, Julio Gutiérrez, Miguel Torres, Carlos Martínez-A., Gabriel Márquez
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CCR6-deficient mice have impaired leukocyte homeostasis and altered contact hypersensitivity and delayed-type hypersensitivity responses

Abstract

CCR6 expression in dendritic, T, and B cells suggests that this β-chemokine receptor may regulate the migration and recruitment of antigen-presenting and immunocompetent cells during inflammatory and immunological responses. Here we demonstrate that CCR6–/– mice have underdeveloped Peyer’s patches, in which the myeloid CD11b+ CD11c+ dendritic-cell subset is not present in the subepithelial dome. CCR6–/– mice also have increased numbers in T-cell subpopulations within the intestinal mucosa. In 2,4-dinitrofluorobenzene–induced contact hypersensitivity (CHS) studies, CCR6–/– mice developed more severe and more persistent inflammation than wild-type (WT) animals. Conversely, in a delayed-type hypersensitivity (DTH) model induced with allogeneic splenocytes, CCR6–/– mice developed no inflammatory response. The altered responses seen in the CHS and DTH assays suggest the existence of a defect in the activation and/or migration of the CD4+ T-cell subsets that downregulate or elicit the inflammation response, respectively. These findings underscore the role of CCR6 in cutaneous and intestinal immunity and the utility of CCR6–/– mice as a model to study pathologies in these tissues.

Authors

Rosa Varona, Ricardo Villares, Laura Carramolino, Íñigo Goya, Ángel Zaballos, Julio Gutiérrez, Miguel Torres, Carlos Martínez-A., Gabriel Márquez

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Figure 2

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Similar LC complements in the skin, but altered positioning of the myelo...
Similar LC complements in the skin, but altered positioning of the myeloid DC subpopulation within the PPs of CCR6–/– mice. (a) Samples of skin epidermis (panel 1) and dermis (panel 2) were stained with the NLDC145 Ab and analyzed by fluorescence microscopy. In panel 3, dorsal ear skin preparations were cultured for 72 hours in RPMI-1640. Dermal sheets were then separated from epidermis and stained with anti-Iab to reveal the existence of LC cords. (b) Staining of WT (CCR6+/+) and knockout (CCR6–/–) mouse PPs with anti-B220 (red) and anti-Thy1.2 (green) reveals B cells in follicles (F) and T cells in the IFR. For orientation, lumen (L) position is indicated. In panel 2, staining with anti-CD11c (red) and anti-CD8α (green) localizes lymphoid DC mainly in the IFR. In panels 3 and 4, staining with anti-CD11c (red) and anti-CD11b (green) shows a defect in the positioning of myeloid DC in CCR6–/– mice, where they are located mainly in the IFR and not in SED. Scale bars = 100 μm.