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Migration of immature mouse DC across resting endothelium is mediated by ICAM-2 but independent of beta2-integrins and murine DC-SIGN homologues
Authors:Wethmar Klaus  Helmus Yvonne  Lühn Kerstin  Jones Claire  Laskowska Anna  Varga Georg  Grabbe Stephan  Lyck Ruth  Engelhardt Britta  Bixel M Gabriele  Butz Stefan  Loser Karin  Beissert Stefan  Ipe Ute  Vestweber Dietmar  Wild Martin K
Affiliation:Max Planck Institute for Molecular Biomedicine, Münster, Germany, and Institute of Cell Biology, ZMBE, University of Münster, Münster, Germany.
Abstract:Immature dendritic cells (DC) reside in tissues where they initiate immune responses by taking up foreign antigens. Since DC have a limited tissue half-life, the DC pool in tissues has to be replenished constantly. This implies that precursor/immature DC must be able to cross non-activated endothelium using as yet unknown mechanisms. Here we show that immature, but not mature bone marrow-derived murine DC migrate across resting endothelial monolayers in vitro. We find that endothelial intercellular adhesion molecule-2 (ICAM-2) is a major player in transendothelial migration (TEM) of immature DC, accounting for at least 41% of TEM. Surprisingly, the ICAM-2-mediated TEM was independent of beta2-integrins, the known ICAM-2 ligands, since neither blocking of beta2-integrins with antibodies nor the use of CD18-deficient DC affected the ICAM-2-specific TEM. In humans, the C-type lectin DC-specific ICAM-3-grabbing nonintegrin (DC-SIGN) was shown to interact with ICAM-2, suggesting a similar role in mice. However, we find that none of the murine DC-SIGN homologues mDC-SIGN, murine DC-SIGN-related molecule-1 (mSIGN-R1) and mSIGN-R3 is expressed on the surface of bone marrow-derived mouse DC. Taken together, this study shows that ICAM-2 strongly supports transmigration of immature DC across resting endothelium by interacting with ligands that are distinct from beta2-integrins and DC-SIGN homologues.
Keywords:CD18  DC‐SIGN  Dendritic cells  ICAM‐2  Transmigration
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