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Generation of procoagulant collagen- and thrombin-activated platelets in platelet concentrates derived from buffy coat: the role of processing, pathogen inactivation, and storage. | LitMetric

AI Article Synopsis

  • Collagen- and thrombin-activated platelets (COAT PLTs) enhance clotting at injury sites, with implications for stroke risk and bleeding disorders.
  • The study examined the effects of processing, pathogen inactivation, and storage on platelet concentrates from buffy coat, focusing on COAT PLT generation and reactivity.
  • Findings showed that the preparation and storage of platelet concentrates led to a significant reduction in COAT PLTs and impaired platelet response to certain stimulants, with minimal differences between treated and untreated samples.

Article Abstract

Background: Collagen- and thrombin-activated (COAT) platelets (PLTs), generated by dual-agonist stimulation with collagen and thrombin (THR), enhance THR generation at the site of vessel wall injury. There is evidence that higher amounts of procoagulant COAT PLTs are associated with stroke, while a decreased ability to generate them is associated with bleeding diathesis. Our aim was to study PLT functions, particularly the ability to generate COAT PLTs, in PLT concentrates (PCs) from buffy coat. Thus, we investigated the effect of processing, pathogen inactivation treatment (amotosalen-UVA), and PC storage.

Study Design And Methods: Two PCs from five donors each were pooled and split in two bags; one of them was pathogen inactivated and the other one was left untreated (n = 5). Flow cytometric analyses were performed immediately after PC preparation (Day 1) and thereafter on Days 2, 5, 7, and 9 in treated and untreated PCs to measure the reactivity of PLTs (CD62P and PAC-1), the content and secretion of dense granule after stimulation with different agonists, and the percentage of COAT PLTs after dual stimulation with convulxin (agonist of the collagen receptor GPVI) and THR.

Results: Preparation of PCs resulted in a significant decrease of COAT PLTs and in an impaired response to adenosine 5'-diphosphate sodium (ADP). Storage further decreased ADP response. Minor differences were observed between untreated or amotosalen-UVA-treated PCs.

Conclusion: Preparation of PCs from buffy coats decreased the ability to generate COAT PLTs and impaired PLT response to ADP.

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Source
http://dx.doi.org/10.1111/trf.14883DOI Listing

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