Abstract
Two variants of the cytoplasmic domain of the integrin alpha 6 subunit have been identified (alpha 6A and alpha 6B). To determine the role of each variant in mediating cell adhesion to laminin, we have independently expressed the alpha 6A and alpha 6B subunits in K562 cells. Both variants associated with endogenous beta 1 and were present at comparable levels on the surface of transfected K562 cells. After activation with phorbol ester (phorbol 12-myristate 13-acetate; PMA) or the stimulatory anti-beta 1 antibody TS2/16, alpha 6A beta 1 as well as alpha 6B beta 1 mediated cell adhesion to laminin and more specifically to its fragment E8. Furthermore, both integrin variants interacted with the laminin isoforms kalinin and merosin. Cell adhesion to laminin isoforms was inhibited by the alpha 6-specific monoclonal antibody GoH3. PMA was less efficient in stimulating adhesion than TS2/16 and stimulated adhesion of alpha 6B transfectants better than of alpha 6A transfectants. In contrast, TS2/16 stimulated the adhesion of the alpha 6A and alpha 6B transfectants to laminin to a similar extent. These findings indicate that the cells may regulate the activation of the two alpha 6 variants independently. Activation by PMA was associated with the phosphorylation of both alpha 6A and alpha 6B subunits, but there was no relationship between the degree of phosphorylation and the ability of the transfectants to adhere to laminin since alpha 6A became phosphorylated much more strongly by PMA than alpha 6B. Thus, both alpha 6A beta 1 and alpha 6B beta 1 on K562 cells are activation-dependent receptors for different isoforms of laminin.
Highlights
Two variants of the cytoplasmic domain of the inte- laminin (Sonnenberg et al, 1988, 1990a)
TS2/16-activated a6A and a6B transfectants tohuman kali- Transfection of full-length a6A and a6BcDNAs into K562 nin was blocked by BM165, a mAb directed against the 165- cells enabled us to study and compare the function of the two kDa human kalinin A chain (Rousselle et aL, 1991), which a6 variants in the adhesion to various isoforms of laminin
Binding after phorbol 12-myristate 13-acetate (PMA) treatment is different for the two integrin
Summary
Transfections and Flow Cytometry-Plasmid DNA was transfected into K562 cells (5 X lo cells) by electroporation using the Bio-Rad. To select for cells in the same medium supplemented with 1 mg/ml Geneticin (G418 expressing high levels of a6, sorting on the FACS was performed sulfate, Life Technologies Inc.). 7) The mouse mAbs TS2/16 and A- number of integrated a6 cDNAs. 1A5 (Hemler et al, 1984), kindly provided by Dr.F. Sanchez-Madrid Immunoprecipitation of ’26Z-Labeled Cells and 32P-LabeledCells-. Hemler (Dana K562 cells and transfectants were surface labeled with ’%Iby the Farber Cancer Institute, Boston, MA) and rat mAb AIIB2 (Werb et lactoperoxidase/hydrogen peroxide method as described previously al., 1989), a gift from Dr C. Precleared cell lysates were added to protein A-Seph- for 10 min before plating onto coated plates for a 30-min adhesion arose beads incubated previouslywith rabbit anti-mouse IgG or rabbit assay. After incubation for 1h at room temperature, the beads carrying the immune complexes were
Sign-in/Register to view highlights & summary Sign-in/Register to access full text options 
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call
