Studies of Adhesion-Dependent Platelet Activation : Distinct Roles for Different Participating Receptors Can Be Dissociated by Proteolysis of Collagen

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Arteriosclerosis, Thrombosis, and Vascular Biology. 1999;19:3033-3043

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	Biochemistry and metabolism
	Platelets

(Arteriosclerosis, Thrombosis, and Vascular Biology. 1999;19:3033.)
© 1999 American Heart Association, Inc.

Thrombosis

Studies of Adhesion-Dependent Platelet Activation

Distinct Roles for Different Participating Receptors Can Be Dissociated by Proteolysis of Collagen

Pia Siljander; Riitta Lassila

From the Wihuri Research Institute (P.S., R.L.) and the Electron Microscopy Unit, Institute of Biotechnology, University of Helsinki (P.S.), Helsinki, Finland.

Correspondence to Dr Riitta Lassila, Wihuri Research Institute, Kalliolinnantie 4, SF-00140 Helsinki 14, Finland. E-mail riitta.lassila{at}wri.fimnet.fi

Abstract—The molecular differences between native-typecollagen type I fibrils (NC) and their pepsinated monomers (PC)were used to uncover receptors involved in platelet-collageninteraction along the adhesion-activation axis. The platelet-depositingcapacity of NC and PC under blood flow and their adhesive propertiesand respective morphologies, aggregation, procoagulant capacity,and tyrosine phosphorylation were compared under different cationicmilieus, including or excluding the glycoprotein (GP) Ia/IIa.NC was consistently a more preferable and activating substratethan PC during flow (5 minutes) and in platelet aggregation.In PPACK-treated blood, both NC (3.3-fold) and PC (2.7-fold)increased platelet attachment on elevation of the shear ratefrom 500 to 1640 s^-1, whereas in citrated blood, adhesion andthrombus growth on PC were negligible under the high shear rate,unlike on NC (1.9-fold increase). The complete lack of plateletdeposition on PC in citrated blood could be overcome by restoringphysiological Mg²⁺ concentration, and in contrast to NC, platelets interactingwith PC were highly dependent on Mg²⁺ during adhesion, aggregation,and procoagulant response. Monoclonal antibody (mAb 131.7) againstGP IV inhibited platelet deposition to NC in citrated blood(2 minutes) by 49%, which was not further increased by coincubationwith mAb against GP Ia (6F1). These results stress the importanceof GP Ia/IIa in shear-resistant platelet deposition on collagenmonomers. In native fibers, however, the preserved quaternarystructure with telopeptides activates additional platelet receptorscapable of substituting GP Ia/IIa and GP IV.

Key Words: hemostasis • platelet • collagen • receptor • divalent cations

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