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凝血酶减少的 miR-27b 通过增强血小板合成抗血管生成的血小板反应蛋白-1 来减弱血小板的体外血管生成活性。

Thrombin-reduced miR-27b attenuates platelet angiogenic activities in vitro via enhancing platelet synthesis of anti-angiogenic thrombospondin-1.

机构信息

Department of Medicine-Solna, Clinical Pharmacology Group, Karolinska Institutet, Stockholm, Sweden.

Department of Pathology, Zhejiang Provincial Key Laboratory of Pathophysiology, Ningbo University School of Medicine, Ningbo, China.

出版信息

J Thromb Haemost. 2018 Apr;16(4):791-801. doi: 10.1111/jth.13978. Epub 2018 Mar 15.

DOI:10.1111/jth.13978
PMID:29442415
Abstract

UNLABELLED

Essentials It is unclear if platelet micro-RNAs can regulate de novo protein synthesis of platelets. Platelet de novo protein synthesis of thrombospondin-1 (TSP-1) was induced by thrombin. Thrombin stimulation in vitro altered platelet microRNA profiles, including decreased miR-27b. Decreased miR-27b hampers platelet angiogenic activities via enhancing de novo TSP-1 synthesis.

SUMMARY

Background Platelets can synthesize proteins upon activation. Platelets contain a number of microRNAs (miRNA) and a fully functional miRNA effector machinery. It is, however, unclear if platelet miRNAs can regulate protein synthesis of platelets, and whether the regulation may produce a physiological impact. Objectives To investigate if and how platelet miRNAs regulate de novo syntheses of angiogenic regulators and subsequently modulate platelet angiogenic activities. Methods and Results Microarray-based miRNA profiling showed that thrombin stimulation in vitro down- or up-regulated a number of platelet miRNAs, both in the total platelet miRNAs and in Ago2-associated miRNAs. Among those altered miRNAs, miR-27b was down-regulated in both the total and Ago2-immunoprecipitated miRNA profiles of platelets, which was confirmed by reverse transcription-quantitative PCR (RT-qPCR). Using western blotting assays, we showed that thrombin induced platelet de novo synthesis of thrombospondin-1, and that the level of thrombospondin-1 synthesis could reach a level of 3-5-fold higher than that before thrombin stimulation. With either the platelet precursor megakaryocyte cell line MEG-01 cells or mature platelets, we demonstrated that transfection of miR-27b mimic, but not the negative control of miRNA mimic, markedly reduced thrombospondin-1 protein levels. The latter subsequently enhanced platelet-dependent endothelial tube formation on matrigel. Conclusions Thrombin stimulation in vitro reduces platelet miR-27b levels that may markedly enhance thrombin-evoked platelet de novo synthesis of thrombospondin-1. Elevation of platelet miR-27b by transfection inhibits thrombospondin-1 synthesis, and subsequently enhances platelet pro-angiogenic activities. Hence, platelet activation-dependent reduction of miR-27b levels may represent a novel negative regulatory mechanism of platelet angiogenic activities.

摘要

目的

血小板激活后可以合成蛋白质。血小板含有多种 microRNAs(miRNA)和功能齐全的 miRNA 效应器机制。然而,目前尚不清楚血小板 miRNA 是否可以调节血小板蛋白质的合成,以及这种调节是否会产生生理影响。

方法

通过 microarray 进行 miRNA 图谱分析,结果显示体外凝血酶刺激可下调或上调多种血小板 miRNA,包括 miR-27b。

结果

miR-27b 下调后,血小板的血管生成活性增强。

结论

凝血酶刺激会降低血小板中的 miR-27b 水平,从而促进血小板合成新的血栓调节蛋白-1。miR-27b 抑制血小板新合成的血栓调节蛋白-1,从而增强血小板的促血管生成活性。

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