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动脉壁切应力增强了黏附于 VEGF 结合表面的内皮祖细胞的分化。

Arterial shear stress augments the differentiation of endothelial progenitor cells adhered to VEGF-bound surfaces.

机构信息

Genome Biotechnology Laboratories, Kanazawa Institute of Technology, 3-1 Yatsukaho, Hakusan, Ishikawa 924-0838, Japan.

出版信息

Biochem Biophys Res Commun. 2012 Jun 22;423(1):91-7. doi: 10.1016/j.bbrc.2012.05.088. Epub 2012 May 23.

DOI:10.1016/j.bbrc.2012.05.088
PMID:22634005
Abstract

Our ongoing studies show that vascular endothelial cell growth factor (VEGF)-bound surfaces selectively capture endothelial progenitor cells (EPCs) in vitro and in vivo, and that surface-bound VEGF stimulates intracellular signal transduction pathways over prolonged culture periods, resulting in inductive differentiation of EPCs. In this article, we investigated whether simulated arterial shear stress augments the differentiation of EPCs adhered to a VEGF-bound surface. Human peripheral blood-derived mononuclear cells adhered to a VEGF-bound surface were exposed to 1 day of shear stress (15 dynes/cm(2), corresponding to shear load in arteries). Shear stress suppressed the expression of mRNAs encoding CD34 and CD133, which are markers for EPCs, and augmented the expression of mRNAs encoding CD31 and von Willebrand factor (vWF) as well as vWF protein, which are markers for endothelial cells (ECs). Shear stress enhanced expression of ephrinB2 mRNA, a marker for arterial ECs, but did not significantly change expression of EphB4 mRNA, a marker for venous ECs. Focused protein array analysis showed that mechanotransduction by shear stress activated the p38 and MAPK pathways in EPCs. Thus, arterial shear stress, in concert with surface-bound VEGF, augments the differentiation of EPCs. These results strongly support previous observation of rapid differentiation of EPCs captured on VEGF-bound stents in a porcine model.

摘要

我们正在进行的研究表明,血管内皮细胞生长因子(VEGF)结合表面在体外和体内选择性地捕获内皮祖细胞(EPC),并且表面结合的 VEGF 在延长的培养期间刺激细胞内信号转导途径,导致 EPC 的诱导分化。在本文中,我们研究了模拟动脉切应力是否会增强附着在 VEGF 结合表面上的 EPC 的分化。将附着在 VEGF 结合表面上的人外周血单核细胞暴露于 1 天的切应力(15 dynes/cm 2 ,对应于动脉中的切负荷)。切应力抑制了 EPC 标志物 CD34 和 CD133 的 mRNA 表达,并增强了内皮细胞(EC)标志物 CD31 和血管性血友病因子(vWF)以及 vWF 蛋白的 mRNA 表达。切应力增强了动脉 EC 的标志物 EphrinB2 mRNA 的表达,但 EphB4 mRNA 的表达,即静脉 EC 的标志物,没有显著变化。聚焦蛋白质阵列分析表明,切应力的机械转导激活了 EPC 中的 p38 和 MAPK 途径。因此,动脉切应力与表面结合的 VEGF 一起增强了 EPC 的分化。这些结果强烈支持了以前在猪模型中观察到的 VEGF 结合支架上捕获的 EPC 快速分化的观察结果。

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