A Monte Carlo study of ligand-dependent integrin signal initiation

Biology – Quantitative Biology – Quantitative Methods

Scientific paper

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Scientific paper

Integrins are allosteric cell adhesion receptors that control many important processes, including cell migration, proliferation, and apoptosis. Ligand binding activates integrins by stabilizing an integrin conformation with separated cytoplasmic tails, thus enabling the binding of proteins that mediate cytoplasmic signaling. Experiments demonstrate a high sensitivity of integrin signaling to ligand density and this has been accounted mainly to avidity effects. Based on experimental data we have developed a quantitative Monte Carlo model for integrin signal initiation. We show that within the physiological ligand density range avidity effects cannot explain the sensitivity of cellular signaling to small changes in ligand density. Src kinases are among the first proteins to be activated, possibly by trans auto-phosphorylation. We calculate the extent of integrin and ligand clustering as well as the speed and extent of Src kinase activation by trans auto-phosphorylation or direct binding at different experimentally monitored ligand densities. We find that the experimentally observed ligand density dependency can be reproduced if Src kinases are activated by trans auto-phosphorylation or some other mechanism limits integrin-dependent Src kinase activation. We propose that Src kinase and thus cell activation by trans auto-phosphorylation may provide a mechanism to enable ligand-density dependent responses at physiological ligand densities. The capacity to detect small differences in ligand density at a ligand density that is large enough to permit cell adhesion is likely to be important for haptotaxis.

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