The VWF/LRP4/αVβ3-axis represents a novel pathway regulating proliferation of human vascular smooth muscle cells

血管平滑肌 新生内膜 细胞生物学 内膜增生 血管性血友病因子 受体 邻近连接试验 血管生成 化学 内科学 生物 细胞生长 内分泌学 癌症研究 免疫学 医学 生物化学 血小板 支架 再狭窄 平滑肌
作者
Jérémy Lagrange,Morel E. Worou,Jean‐Baptiste Michel,Alexandre Raoul,Mélusine Didelot,Vincent Muczynski,Paulette Legendre,François Plénat,Guillaume Gauchotte,Marc‐Damien Lourenco‐Rodrigues,Olivier D. Christophe,Peter J. Lenting,Patrick Lacolley,Cécile V. Denis,Véronique Regnault
出处
期刊:Cardiovascular Research [Oxford University Press]
卷期号:118 (2): 622-637 被引量:33
标识
DOI:10.1093/cvr/cvab042
摘要

Abstract Aims Von Willebrand factor (VWF) is a plasma glycoprotein involved in primary haemostasis, while also having additional roles beyond haemostasis namely in cancer, inflammation, angiogenesis, and potentially in vascular smooth muscle cell (VSMC) proliferation. Here, we addressed how VWF modulates VSMC proliferation and investigated the underlying molecular pathways and the in vivo pathophysiological relevance. Methods and results VWF induced proliferation of human aortic VSMCs and also promoted VSMC migration. Treatment of cells with a siRNA against αv integrin or the RGT-peptide blocking αvβ3 signalling abolished proliferation. However, VWF did not bind to αvβ3 on VSMCs through its RGD-motif. Rather, we identified the VWF A2 domain as the region mediating binding to the cells. We hypothesized the involvement of a member of the LDL-related receptor protein (LRP) family due to their known ability to act as co-receptors. Using the universal LRP-inhibitor receptor-associated protein, we confirmed LRP-mediated VSMC proliferation. siRNA experiments and confocal fluorescence microscopy identified LRP4 as the VWF-counterreceptor on VSMCs. Also co-localization between αvβ3 and LRP4 was observed via proximity ligation analysis and immuno-precipitation experiments. The pathophysiological relevance of our data was supported by VWF-deficient mice having significantly reduced hyperplasia in carotid artery ligation and artery femoral denudation models. In wild-type mice, infiltration of VWF in intimal regions enriched in proliferating VSMCs was found. Interestingly, also analysis of human atherosclerotic lesions showed abundant VWF accumulation in VSMC-proliferating rich intimal areas. Conclusion VWF mediates VSMC proliferation through a mechanism involving A2 domain binding to the LRP4 receptor and integrin αvβ3 signalling. Our findings provide new insights into the mechanisms that drive physiological repair and pathological hyperplasia of the arterial vessel wall. In addition, the VWF/LRP4-axis may represent a novel therapeutic target to modulate VSMC proliferation.
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