Glycosylation of β-1 integrins in B16-F10 mouse melanoma cells as determinant of differential binding and acquisition of biological activity

Studying B16-FIO cells we could identify p-l integrins as laminin, fibronectin and collagen receptors. Gradient ionic strength elution analysis of affinity chromatography showed differential interactions between laminin-binding p-I integrins (two p-I polypeptides of I05 and I20 kDa) and fibronectin and collagen-binding p-I integrins (elution of one major p-I polypeptide of I20 kDa) and their respective ligands. To evaluate this diversity we Submitted 816-FIO extracts to IEF and SDS-PAGE and found that one p-I integrin formed acidic and larger isoforms, while another formed basic and smaller isoforms. To study this difference we also submitted material eluted from WGA-Sepharose columns to IEF but now only the acidic 9-1 isoform was found. Extracts of B 16-F I 0 treated with neuraminidase showed only the basic fL I isoform, suggesting that terminal sialic acid residues may be responsible for this acidic pattern, an interpretation supported by the fact that MAA (Maackia arnrnurensis agglutinin) reacts only with the acidic isoform. Differential glycosylation of p-I integrin isoforms in B 16-F 10 was also demonstrated since the smaller lamininbinding p-I integrin isoform reacted only with GNA (Galanthus nivalis agglutinin), whereas the mature larger form reacted with DSA (Datum strarnoniurn agglutinin) and MAA; thus this heterogeneity of @-I chains is essentially due to variable glycosylation. Autoradiography and immunoblotting analysis of material separated by 2-dimensional electrophoresis show that only the processed forms of p-I integrins are expressed at the cell surface.