Protease-activated receptors 1 and 4 mediate activation of human platelets by thrombin
Mark L. Kahn, … , Hiroaki Ishihara, Shaun R. Coughlin
Mark L. Kahn, … , Hiroaki Ishihara, Shaun R. Coughlin
Published March 15, 1999
Citation Information: J Clin Invest. 1999;103(6):879-887. https://doi.org/10.1172/JCI6042.
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Article

Protease-activated receptors 1 and 4 mediate activation of human platelets by thrombin

Abstract

Because of the role of thrombin and platelets in myocardial infarction and other pathological processes, identifying and blocking the receptors by which thrombin activates platelets has been an important goal. Three protease-activated receptors (PARs) for thrombin — PAR1, PAR3, and PAR4 — are now known. PAR1 functions in human platelets, and the recent observation that a PAR4-activating peptide activates human platelets suggests that PAR4 also acts in these cells. Whether PAR1 and PAR4 account for activation of human platelets by thrombin, or whether PAR3 or still other receptors contribute, is unknown. We have examined the roles of PAR1, PAR3, and PAR4 in platelets. PAR1 and PAR4 mRNA and protein were detected in human platelets. Activation of either receptor was sufficient to trigger platelet secretion and aggregation. Inhibition of PAR1 alone by antagonist, blocking antibody, or desensitization blocked platelet activation by 1 nM thrombin but only modestly attenuated platelet activation by 30 nM thrombin. Inhibition of PAR4 alone using a blocking antibody had little effect at either thrombin concentration. Strikingly, simultaneous inhibition of both PAR1 and PAR4 virtually ablated platelet secretion and aggregation, even at 30 nM thrombin. These observations suggest that PAR1 and PAR4 account for most, if not all, thrombin signaling in platelets and that antagonists that block these receptors might be useful antithrombotic agents.

Authors

Mark L. Kahn, Mayumi Nakanishi-Matsui, Michael J. Shapiro, Hiroaki Ishihara, Shaun R. Coughlin

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Flow cytometric analysis of platelets for surface expression of PAR1, PA...
Flow cytometric analysis of platelets for surface expression of PAR1, PAR3, and PAR4. Fixed platelets were incubated with preimmune IgG (narrow lines) or PAR1 IgG (a), PAR3 IgG (b), or PAR4 IgG (c) (wide lines) and then analyzed as described in Methods. (d) Platelets were incubated with PAR4 IgG in the absence (wide line) or presence (thin line) of the peptide antigen (1 μM) used to generate the PAR4 antiserum, or after treatment with 20 nM thrombin for 10 min at 37°C (dotted line). Each curve represents an analysis of 10,000 events. This experiment was repeated twice with separate donors with equivalent results. (e) Flow cytometric analysis of Dami cells as a positive control for detection of PAR3. Fixed Dami cells were incubated with preimmune IgG (narrow line) or PAR3 IgG (wide line) and then analyzed as above. Dami cells were also positive for PAR1 and PAR4 (not shown).