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Circulation. 2004;110:2597-2600
Published online before print July 19, 2004, doi: 10.1161/01.CIR.0000138027.80056.31
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(Circulation. 2004;110:2597-2600.)
© 2004 American Heart Association, Inc.


Cardiovascular Surgery

Clinical Inhibition of the Seven-Transmembrane Thrombin Receptor (PAR1) by Intravenous Aprotinin During Cardiothoracic Surgery

J.R.S. Day, MRCS; P.P. Punjabi, FRCS; A.M. Randi, PhD; D.O. Haskard, DM; R.C. Landis, PhD; K.M. Taylor, MD

From the British Heart Foundation Cardiac Surgery (J.R.S.D., P.P.P., K.M.T.) and Cardiovascular Medicine (A.M.R., D.O.H.) Units, Eric Bywaters Centre, Imperial College, London, UK; and Edmund Cohen Laboratory for Vascular Research (R.C.L.), Chronic Disease Research Centre, UWI, Bridgetown, Barbados.

Correspondence to J.R.S. Day, British Heart Foundation Cardiac Surgery Unit, Eric Bywaters Centre, Imperial College, London W12 0NN, UK. E-mail j.day{at}imperial.ac.uk

Received March 23, 2004; de novo received April 22, 2004; revision received June 16, 2004; accepted June 17, 2004.

Background— Protease-activated receptor-1 (PAR1) is the principal thrombin receptor in the vasculature, and antagonists against this receptor are in preclinical trials. Aprotinin, already approved for clinical use to reduce transfusion requirements in cardiopulmonary bypass (CPB) surgery, has been shown to inhibit PAR1 activation in vitro. Here, we exploit CPB as a model for thrombin generation in humans to examine whether aprotinin can inhibit platelet PAR1 activation clinically.

Methods and Results— PAR1 expression and function on platelets was examined in coronary artery bypass grafting (CABG) patients randomized into 2 groups: (1) those receiving saline infusion during CPB (n=17) and (2) those receiving aprotinin (2x106 kallikrein inhibitor units [KIU] in pump prime, 2x106 KIU loading dose, followed by 0.5x106 KIU/h [n=13]). Platelets in the saline group showed loss of PAR1-specific function at 2 hours after CPB, but this was preserved in the aprotinin group (P<0.001). These effects were most likely targeted at PAR1 receptor cleavage, because (1) the level of thrombin generated during CPB did not vary significantly between groups, (2) expression of SPAN12, which detects only uncleaved PAR1 receptors, was preserved in the aprotinin but not the placebo group (P<0.05), and (3) supporting evidence in vitro showed reduced thrombin-induced PAR1 cleavage (P<0.001) and platelet aggregation (P<0.001) in the presence of aprotinin.

Conclusions— This study demonstrates that platelet PAR1 activation by thrombin can be inhibited by aprotinin. Our results extend the clinical mechanism of action of aprotinin and provide the first proof of principle that PAR1 can be inhibited clinically. This has implications beyond cardiac surgery for the development of therapeutic PAR1 blockade.


Key Words: thrombin • platelets • cardiopulmonary bypass


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