4.5 Article

High-efficiency unassisted transfection of platelets with naked double-stranded miRNAs modulates signal-activated translation and platelet function

Journal

PLATELETS
Volume 32, Issue 6, Pages 794-806

Publisher

TAYLOR & FRANCIS INC
DOI: 10.1080/09537104.2020.1809642

Keywords

Exosomes; microvesicles; miRNA; mRNA; transfection; translation

Funding

  1. National Heart, Lung, and Blood Institute [R01HL137207, R01HL144574]

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The study demonstrates the ability of ex vivo platelets to internalize ectopic miRNAs and modulate signal-activated translation and platelet function, with a focus on the new role of miR-223-3p in extracellular vesicle generation.
We sought novel approaches to improve transfection efficiencies of microRNAs (miRNAs) in platelets, and to apply these approaches to investigate the roles of miRNAs in regulating signal-activated protein translation and functional effects. We found thatex vivohuman platelets support gymnosis---internalization of ectopic miRNAs following co-incubation in the absence of conventional transfection reagents or schemes---and subsequently incorporate transfected miRNA into ARGONAUTE2 (AGO2)-based RNA-induced silencing complexes (RISC). Thrombin/fibrinogen stimulation activated translation of miR-223-3p target SEPTIN2, which was suppressed by miR-223-3p transfection in an AGO2/RISC-dependent manner. Thrombin/fibrinogen-induced exosome and microvesicle generation was inhibited by miR-223-3p transfection, and this effect was reversed with a RISC inhibitor. Platelet gymnosis of naked miRNAs appeared to be mediated in part by endocytic pathways including clathrin-dependent and fluid-phase endocytosis and caveolae. These results demonstrate the ability ofex vivoplatelets to internalize ectopic miRNAs by unassisted transfection, and utilize them to modulate signal-activated translation and platelet function. Our results identify new roles for miR-223-3p in extracellular vesicle generation in stimulated platelets. High-efficiency gymnotic transfection of miRNAs inex vivoplatelets may be a broadly useful tool for exploring molecular genetic regulation of platelet function.

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