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*Substance via MeSH
The Journal of Immunology, 1998, 161: 1083-1086.
Copyright © 1998 by The American Association of Immunologists


CUTTING EDGE

Cutting Edge: Differential Regulation of Chemokine Receptors During Dendritic Cell Maturation: A Model for Their Trafficking Properties1

Silvano Sozzani2,3,*, Paola Allavena2,*, Giovanna D’Amico*, Walter Luini*, Giancarlo Bianchi*, Motoji Kataura{dagger}, Toshio Imai{dagger}, Osamu Yoshie{dagger}, Raffaella Bonecchi* and Alberto Mantovani*,{ddagger}

* Istituto di Ricerche Farmacologiche Mario Negri, Milan, Italy; {dagger} Shionogi Institute for Medical Science, Osaka, Japan; and {ddagger} Department of Biotechnology, Section of General Pathology, University of Brescia, Italy

Upon exposure to immune or inflammatory stimuli, dendritic cells (DC) migrate from peripheral tissues to lymphoid organs, where they present Ag. CC chemokines induce chemotactic and transendothelial migration of immature DC, in vitro. Maturation of DC by CD40L, or by LPS, IL-1, and TNF, induces down-regulation of the two main CC chemokine receptors expressed by these cells, CCR1 and CCR5, and abrogates chemotaxis to their ligands. Inhibition was rapid (<1 h) and included the unrelated agent FMLP. Concomitantly, the expression of CCR7 and the migration to its ligand EBI1 ligand chemokine (ELC)/macrophage inflammatory protein (MIP)-3ß, a chemokine expressed in lymphoid organs, were strongly up-regulated, though with slower kinetics (24–48 h). Rapid inhibition of responsiveness to chemoattractants present at sites of inflammation and immune reaction may be permissive for leaving peripheral tissues. Conversely, the slower acquisition of responsiveness to ELC/MIP-3ß may guide subsequent localization of DC in lymphoid organs.




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