Platelet-derived miR-223 promotes a phenotypic switch in arterial injury repair
Zhi Zeng, … , John Hwa, Wai Ho Tang
Zhi Zeng, … , John Hwa, Wai Ho Tang
Published January 15, 2019
Citation Information: J Clin Invest. 2019;129(3):1372-1386. https://doi.org/10.1172/JCI124508.
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Research Article Vascular biology

Platelet-derived miR-223 promotes a phenotypic switch in arterial injury repair

Abstract

Upon arterial injury, endothelial denudation leads to platelet activation and delivery of multiple agents (e.g., TXA2, PDGF), promoting VSMC dedifferentiation and proliferation (intimal hyperplasia) during injury repair. The process of resolution of vessel injury repair, and prevention of excessive repair (switching VSMCs back to a differentiated quiescent state), is poorly understood. We now report that internalization of APs by VSMCs promotes resolution of arterial injury by switching on VSMC quiescence. Ex vivo and in vivo studies using lineage tracing reporter mice (PF4-cre × mT/mG) demonstrated uptake of GFP-labeled platelets (mG) by mTomato red–labeled VSMCs (mT) upon arterial wire injury. Genome-wide miRNA sequencing of VSMCs cocultured with APs identified significant increases in platelet-derived miR-223. miR-223 appears to directly target PDGFRβ (in VSMCs), reversing the injury-induced dedifferentiation. Upon arterial injury, platelet miR-223–KO mice exhibited increased intimal hyperplasia, whereas miR-223 mimics reduced intimal hyperplasia. Diabetic mice with reduced expression of miR-223 exhibited enhanced VSMC dedifferentiation and proliferation and increased intimal hyperplasia. Our results suggest that horizontal transfer of platelet-derived miRNAs into VSMCs provides a novel mechanism for regulating VSMC phenotypic switching. Platelets thus play a dual role in vascular injury repair, initiating an immediate repair process and, concurrently, a delayed process to prevent excessive repair.

Authors

Zhi Zeng, Luoxing Xia, Xuejiao Fan, Allison C. Ostriker, Timur Yarovinsky, Meiling Su, Yuan Zhang, Xiangwen Peng, Yi Xie, Lei Pi, Xiaoqiong Gu, Sookja Kim Chung, Kathleen A. Martin, Renjing Liu, John Hwa, Wai Ho Tang

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Figure 2

APs transferred miR-143, miR-145, and miR-223 into VSMCs, and promoted VSMC differentiation.

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APs transferred miR-143, miR-145, and miR-223 into VSMCs, and promoted V...
(A) Heatmap of the top 10 differentially expressed miRNAs in VSMCs cocultured with or without APs for 24 hours (n = 3). (B) Expression of miR-143, miR-145, and miR-223 in VSMCs (Ctrl) and VSMCs cocultured with APs (n = 4). (C) Expression of miR-143, miR-145, and miR-223 in VSMCs (Ctrl) and VSMCs cocultured with RPs or APs after pretreatment with prostacyclin or RNase A (n = 4). (D) The expression of ACTA2 and KLF4 in control VSMCs (Ctrl) and VSMCs cocultured with RPs or APs after pretreatment with prostacyclin or RNase A and thrombin (n = 4). Data are presented as mean ± SD. *P <0.05, **P < 0.01, ***P < 0.001 vs. Ctrl; P < 0.05, ††P < 0.01 vs. RPs; #P < 0.05, ##P < 0.01 vs. APs. Statistical significance was determined using parametric t test (B) and 1-way ANOVA followed by Tukey-Kramer multiple-comparisons test (C and D).