Selectin ligands on human melanoma cells

Abstract

Twelve established human melanoma lines were screened for surface expression of the carbohydrate antigens Lewis^a (Le^a), sialyl Lewis^a (SLe^a), dimeric sialyl Lewis^a (diSLe^a), sialyl Lewis^X (SLe^X) and dimeric sialyl Lewis^X (diSLe^X). None of the lines expressed SLe^X, but 11/12 were positive for diSLe^X and 7/12 were positive for SLe^a. Although both diSLe^X and SLe^a have been reported to bind to E-selectin, none of the melanoma lines exhibited E-selectin-dependent adhesion to activated human umbilical vein endothelial cells (HUVECs). Three melanoma lines infected with a retroviral vector carrying the cDNA for the human Lewis fucosyltransferase (FucT-III) subsequently expressed SLe^X at their cell surface and exhibited E-selectin-dependent adhesion to activated HUVECs. Treatment of these transduced cells with inhibitors of O-linked or N-linked protein glycosylation significantly inhibited E-selectin-meiiated adhesion, though fluorescence-activated cell sorter analysis indicated no decrease in cell surface expression of SLe^X, SLe^a or diSLe^X. This suggests that the majority of SLe^X/SLe^a-type glycans endogenously procuded by human melanoma cells are not protein-associated and do not mediate E-selectin-dependent adhesion. These results support the hypothesis that E-selectin-dependent adhesion requires presentation of SLe^X-type moieties on appropriate glycoproteins.