Abstract
The VLA integrin subfamily includes receptors for extracellular matrix proteins as well as receptors involved in cell-cell adhesive interactions. We have previously described the up-regulation of VLA integrin-mediated cell attachment to different ligands by the anti-beta 1 TS2/16 monoclonal antibody (mAb) (Arroyo, A. G., Sánchez-Mateos, P., Campanero, M. R., Martín-Padura, I., Dejana, E., and Sánchez-Madrid, F. (1992) J. Cell Biol. 117, 659-670). In this report, we have investigated the mechanism involved in this regulatory effect. The anti-beta 1-mediated regulatory effect on cell adhesion did not require "de novo" protein synthesis, since it was not affected by pretreatment with either cycloheximide or actinomycin D. To quantitate the effect of the regulatory anti-beta 1 TS2/16 mAb on the affinity of VLA-5 for its ligand, an RGD-containing fragment of fibronectin (FN80), we performed binding studies of radiolabeled soluble FN80 to U-937 cells. The affinity of VLA-5 for FN80 was enhanced about 4-fold in the presence of TS2/16 mAb (Kd = 0.98 +/- 0.07 microM) compared to the functionally irrelevant anti-beta 1 Alex 1/4 mAb (Kd = 4.23 +/- 0.92 microM), whereas no alteration in the number of binding sites was observed. Indeed, the anti-beta 1 TS2/16 mAb is inducing this high affinity state on VLA heterodimers by a direct change on the conformation of these receptors as demonstrated by affinity chromatography analysis using extracellular matrix proteins covalently bound to Sepharose. The yield of VLA-5 fibronectin receptor bound to FN80-Sepharose columns was strongly increased upon treatment of U-937 cell lysates with mAb TS2/16. Moreover, higher concentrations of EDTA were required for eluting the VLA-5 integrin from this matrix. This up-regulatory effect was also observed with F(ab')2 and Fab fragments of the anti-beta 1 TS2/16 mAb, and was also exerted on the purified VLA-5 receptor. Similarly, the yield of VLA-2 retained on a collagen I-Sepharose column was dramatically increased by pretreatment of A375 melanoma cell lysates with the mAb TS2/16. Altogether, these results indicate that the interaction of VLA beta 1 heterodimers with their ligands can be regulated by switching between differently active conformations inherent to the alpha beta 1 receptors.
Highlights
From the Hospital de la Princesa, Universidad Autonoma de Madrid, Madrid, Spain andthe SCentro de Investigaciones Bioldgicas, Consejo Superior de Znuestigaciones Cientificas,Madrid, Spain
One of the most important volved in cell-cell adhesive interactions.We have pre- families of adhesionreceptorsareintegrins, which include viously described the up-regulation of VLA integrin- receptors for extracellular matrix proteiansswell as receptors mediated cell attachment to different ligands by the involved in cell-cell adhesive interactions (1, 2)
All integrins anti-B1TS2/16 monoclonal antibody(Arroyo, A. are a8 heterodimers in which the a subunits are eachnonco
Summary
Mediatedenhancedadhesion was independent of denovo protein synthesis, we tested the effect of cycloheximide and actinomycin D, inhibitors of proteinandRNAsynthesis, respectively, on P1-mediated enhanced attachment of either U-937 cells to FN80 or A375 melanoma cells to COL I. Aliquots of lo7cells were pretreated with either 1pg/ml anti-fl,Alex 1/4 or TS2/16 mAb for 15 min at 4 "C.Different amounts of 1261-labeleFdNSO (specificactivity of 2.5 X lo6cpm/pg) were added demonstrated by inhibition of [35S]methionine(>85%) and [3H]thymidine (>94%) incorporation to U-937 cells, respectively. These results demonstrate that de nouo protein synthesis is not required for P1-mediatedregulatory effects on cell adhesion to ECM proteins.
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
