Advanced Flow Cytometry Using the SYTO-13 Dye for the Assessment of Platelet Reactivity and Maturity in Whole Blood

Overview

Journal Methods Protoc

Specialty General Medicine

Date 2023 Jan 17

PMID 36648957

Authors

Oliver Buchhave Pedersen

Leonardo Pasalic

Erik Lerkevang Grove

Steen Dalby Kristensen

Anne-Mette Hvas

Peter H Nissen

Affiliations

Soon will be listed here.

Abstract

Newly produced immature platelets are larger, contain higher amounts of residual RNA, and are more reactive than mature platelets. Flow cytometry using the SYTO-13 dye is a method for the subdivision of immature platelets from mature platelets based on the labelling of intracellular platelet RNA, enabling the simultaneous investigation of the reactivity of each platelet population. This method provides detailed information on several aspects of platelet physiology using a combination of platelet surface markers and agonists. Currently, no standardized protocol exists across laboratories. Here, we describe a flow cytometry protocol in detail to investigate platelet reactivity and its relation to platelet maturity. We analyzed 20 healthy individuals with the protocol and compared the platelet subpopulation with the highest SYTO-13 labelling (in the first quintile, "SYTO-high") corresponding to the most immature platelets (highest RNA content) with the platelet subpopulation with the lowest SYTO-13 labelling (in the fifth quintile, "SYTO-low") corresponding to the mature platelets with the lowest RNA content. SYTO-high platelets had overall significantly increased platelet reactivity compared with that of SYTO-low platelets. The presented method may be a valuable research tool for the analysis of platelet reactivity and its relation to platelet maturity.

Citing Articles

Changes in platelet maturity and reactivity following acute ST-segment elevation myocardial infarction.

Pedersen O, Nissen P, Pasalic L, Hvas A, Kristensen S, Grove E Res Pract Thromb Haemost. 2025; 9(1):102652.

PMID: 39845649 PMC: 11751529. DOI: 10.1016/j.rpth.2024.102652.

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