Auteurs

[:fr]Anselmi G[:],
[:fr]Vaivode K[:],
[:fr]Ramos RN[:],
[:fr]Missolo-Koussou Y[:],
[:fr]Hidalgo S[:],
[:fr]Tosselo J[:],
[:fr]Nuñez N[:],
[:fr]Richer W[:],
[:fr]Vincent-Salomon A[:],
[:fr]Saxena A[:],
[:fr]Wood K[:],
[:fr]Lladser A[:],
[:fr]Piaggio E[:],
[:fr]Helft J[:],

[:fr]

Abstract

Dendritic cells (DCs) are antigen-presenting cells controlling T cell activation. In humans, the diversity, ontogeny, and functional capabilities of DC subsets are not fully understood. Here, we identified circulating CD88CD1c+CD163+ DCs (called DC3s) as immediate precursors of inflammatory CD88CD14+CD1c+CD163+FcεRI+ DCs. DC3s develop via a specific pathway activated by GM-CSF, independent of cDC-restricted (CDP) and monocyte-restricted (cMoP) progenitors. Like classical DCs but unlike monocytes, DC3s drove activation of naive T cells. In vitro, DC3s displayed a distinctive ability to prime CD8+ T cells expressing a tissue homing signature and the epithelial homing alpha-E integrin (CD103) through transforming growth factor β (TGF-β) signaling. In vivo, DC3s infiltrated luminal breast cancer primary tumors, and DC3 infiltration correlated positively with CD8+CD103+CD69+ tissue-resident memory T cells. Together, these findings define DC3s as a lineage of inflammatory DCs endowed with a strong potential to regulate tumor immunity.

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