Quantification of platelet composition in experimental venous thrombosis by real-time polymerase chain reaction

Abstract Introduction Platelets play a key role in thrombus formation. Determination of the platelet component in a thrombus provides pathophysiological insights to the thrombotic event and aids in selecting an appropriate therapeutic intervention. In this study a sensitive and reliable method to characterize the cellular components of experimental thrombi was developed using real-time polymerase chain reaction (PCR). Methods and results Vena cava thrombosis was induced by either oxidative injury to topical FeCl 2 (FeCl 2 -VT) or stenosis-limited blood flow and a hypotonic pressure stress (stasis-VT) in rats. High levels of platelets were identified in the thrombus containing vessels by real-time PCR analysis of target gene amplification using the 2 − ΔΔCT values by normalizing the data with gene expression in naive vessels and with a housekeeping gene, ribosomal protein L32. By this analysis, the levels of PF-4 (as a platelet marker) mRNA were significantly higher in FeCl 2 -VT (2 − ΔΔCT  = 7.8) than in stasis-VT (2 − ΔΔCT  = 4.2, p 2 -VT was also confirmed qualitatively by scanning electronic microscopic analysis. In addition, real-time PCR using a panel of genes representing vascular injury, inflammation and thrombosis showed marked induction (2 − ΔΔCT  > 5) in MCP-1, IL-1β, iNOS and P-selectin mRNA expression in both models. Conclusions These data demonstrate the utility of real-time PCR to quantitate platelets and other cell components in vascular thrombosis, which may facilitate the characterization and thus therapeutic intervention of a particular thrombotic event in both preclinical animal models and clinical conditions.