Abstract
Dendritic cells (DC) are antigen presenting cells (APC) with the unique ability to initiate an immune response. Immature DC are localized in peripheral tissues where they exert a sentinel function for incoming antigens (Ag). After Ag capture and exposure to inflammatory stimuli DC undergo maturation and migrate to regional lymph nodes where the presentation of antigenic peptides to T lymphocytes takes place. Thus their correct functioning as APC involves localization in tissues and trafficking via the lymph or blood to lymphoid organs. In the present study we have investigated the ability of DC to interact in vitro with human vascular endothelial cells (EC) and extracellular matrix (ECM). DC are differentiated from monocytes by in vitro exposure to GM-CSF and IL-13 for 7 days. In adhesion assays a considerable proportion of DC binds to resting EC monolayers and this adhesion is inhibited by anti-CD11a and CD11b, but not anti-CD11c mAbs. Binding to a natural ECM, derived from cultured EC involves VLA-4 and VLA-5 integrins. In a transmigration assay, 10 % of input cells are able to cross the EC monolayer in the absence of exogenous stimuli. The amount of DC transmigrated through a monolayer of EC was increased of 2-3 fold by C-C chemokines RANTES, MIP1α, and MIP-1β. Most importantly, in view of the trafficking pattern of these cells, a significant proportion of DC can migrate in a reverse transmigration assay, i.e. across the endothelial basement membrane and subsequently, across endothelial cells. Upon exposure to immune or inflammatory signals peripheral DC undergo maturation and migration to lymphoid organs. Functional maturation is associated with loss of responsiveness to chemokines present at sites of inflammation (e.g. MIP1α, MIP1β and RANTES) and acquisition of a receptor repertoire which renders these cells responsive to signals which guide their localization in lymphoid organs (e.g. MIP3β). A better understanding of the molecular basis of DC trafficking may provide molecular and conceptual tools to direct and modulate DC localization as a strategy to upregulate and orient specific immunity.
Highlights
Dendritic cells (DC) are professional antigen presenting cells (APC) which play a key role in the initiation of an immune response
In previous experiments we showed that DC
The identification of adhesion molecules involved in the binding to endothelial cells (EC) and to extracellular matrix (ECM) was performed by using functional blocking mAb
Summary
Dendritic cells (DC) are professional antigen presenting cells (APC) which play a key role in the initiation of an immune response. Upon exposure to immune or inflammatory signals peripheral DC undergo maturation and migrate as veiled cells to the T cell areas of lymph nodes (Steinman, 1991; Austyn, 1996; Hart, 1997; Banchereau et al 1998; Sallusto et al 1999). This trafficking of DC to lymph nodes is critical to their overall function as APC, it is established that surgical removal of afferent lymphatic vessels prevents sensitization to skin transplants or to contact allergens (Frey et al 1957; Barker et al 1968). The homing to lymphoid organs and the activation of T cells is apparently the final goal of DC biological program since, very likely, they undergo apoptosis within the T cell areas
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