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      Dendritic cells rapidly recruited into epithelial tissues via CCR6/CCL20 are responsible for CD8+ T cell crosspriming in vivo.

      Immunity
      Adjuvants, Immunologic, Animals, CD8-Positive T-Lymphocytes, immunology, Cell Movement, Chemokine CCL20, Chemokines, CC, metabolism, physiology, Clodronic Acid, pharmacology, Dendritic Cells, Dermis, Dinitrofluorobenzene, Epithelium, Female, H-2 Antigens, genetics, Immunization, Langerhans Cells, Macrophage Inflammatory Proteins, Mice, Mice, Inbred C57BL, Mice, Knockout, Mice, Transgenic, Mouth Mucosa, cytology, Nucleoproteins, Receptors, CCR6, Receptors, Chemokine, Stem Cells

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          Abstract

          The nature of dendritic cell(s) (DC[s]) that conditions efficient in vivo priming of CD8+ CTL after immunization via epithelial tissues remains largely unknown. Here, we show that myeloid DCs rapidly recruited by adjuvants into the buccal mucosa or skin are essential for CD8+ T cell crosspriming. Recruitment of circulating DC precursors, including Gr1+ monocytes, precedes the sequential accumulation of CD11c+ MHC class II+ DCs in dermis and epithelium via a CCR6/CCL20-dependent mechanism. Remarkably, a defect in CCR6, local neutralization of CCL20, or depletion of monocytes prevents in vivo priming of CD8+ CTL against an innocuous protein antigen administered with adjuvant. In addition, transfer of CCR6-sufficient Gr1+ monocytes restores CD8+ T cell priming in CCR6( degrees / degrees ) mice via a direct Ag presentation mechanism. Thus, newly recruited DCs likely derived from circulating monocytes are responsible for efficient crosspriming of CD8+ CTL after mucosal or skin immunization.

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