Literature DB >> 15122174

A novel modification of the Thrombelastograph assay, isolating platelet function, correlates with optical platelet aggregation.

Robert M Craft1, Jack J Chavez, Stuart J Bresee, Dale C Wortham, Eli Cohen, Roger C Carroll.   

Abstract

Flow cytometry, singlet platelet counting, and optical aggregation have been used to monitor clopidogrel and glycoprotein IIb/IIIa (GPIIb/IIIa) platelet antagonists. Optical aggregation is considered the gold standard, but neither it nor flow cytometry is convenient in larger-scale clinical studies or point-of-care systems. Singlet platelet counting, a point-of-care assay correlated with optical platelet aggregation, only provides a measurement of platelet function at a single point in time. The Thrombelastograph is used to assay whole blood for thrombin-generated maximal clot-shear elasticity, referred to as the maximal amplitude (MA). Although platelet dysfunction, thrombocytopenia, and the in vitro effect of strong inhibitors such as IIb/IIIa antagonists can be observed, with thrombin generation milder platelet inhibitors cannot be assessed. We modified the Thromboelastograph assay, using reptilase and factor XIIIa, to form a clot, without thrombin generation, in heparinized whole blood. The resulting clot MA is dependent on added platelet agonists such as ADP or arachidonic acid, is sensitive to platelet antagonists, and provides a continuous measure of platelet function more analogous and better correlated with optical aggregation. This novel modification of the Thromboelastograph assay should prove to be a useful point-of-care whole-blood assay with which to monitor the effects of GPIIb/IIIa, ADP, and thromboxane A(2)-receptor-inhibiting drugs in patients.

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Year:  2004        PMID: 15122174     DOI: 10.1016/j.lab.2004.01.011

Source DB:  PubMed          Journal:  J Lab Clin Med        ISSN: 0022-2143


  31 in total

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2.  Evaluation of the profile of thrombin generation during the process of whole blood clotting as assessed by thrombelastography.

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