Bristol Heart Institute, University of Bristol, UK (L.M.R., H.W., K.W., A.F., Z.L., J.L.J., S.J.G.).
School of Medicine and Biodiscovery Institute, Faculty of Medicine & Health Sciences, University of Nottingham, UK (K.G., P.-S.J.).
Arterioscler Thromb Vasc Biol. 2023 Mar;43(3):456-473. doi: 10.1161/ATVBAHA.122.318367. Epub 2023 Jan 26.
Late vein graft failure is caused by intimal thickening resulting from endothelial cell (EC) damage and inflammation which promotes vascular smooth muscle cell (VSMC) dedifferentiation, migration, and proliferation. Nonphosphorylatable PRH (proline-rich homeodomain) S163C:S177C offers enhanced stability and sustained antimitotic effect. Therefore, we investigated whether adenovirus-delivered PRH S163C:S177C protein attenuates intimal thickening via VSMC phenotype modification without detrimental effects on ECs.
PRH S163C:S177C was expressed in vitro (human saphenous vein-VSMCs and human saphenous vein-ECs) and in vivo (ligated mouse carotid arteries) by adenoviruses. Proliferation, migration, and apoptosis were quantified and phenotype was assessed using Western blotting for contractile filament proteins and collagen gel contraction. EC inflammation was quantified using VCAM (vascular cell adhesion protein)-1, ICAM (intercellular adhesion molecule)-1, interleukin-6, and monocyte chemotactic factor-1 measurement and monocyte adhesion. Next Generation Sequencing was utilized to identify novel downstream mediators of PRH action and these and intimal thickening were investigated in vivo.
PRH S163C:S177C inhibited proliferation, migration, and apoptosis and promoted contractile phenotype (enhanced contractile filament proteins and collagen gel contraction) compared with virus control in human saphenous vein-VSMCs. PRH S163C:S177C expression in human saphenous vein-ECs significantly reduced apoptosis, without affecting cell proliferation and migration, while reducing TNF (tumor necrosis factor)-α-induced VCAM-1 and ICAM-1 and monocyte adhesion and suppressing interleukin-6 and monocyte chemotactic factor-1 protein levels. PRH S163C:S177C expression in ligated murine carotid arteries significantly impaired carotid artery ligation-induced neointimal proliferation and thickening without reducing endothelial coverage. Next Generation Sequencing revealed STAT-1 (signal transducer and activator of transcription 1) and HDAC-9 (histone deacetylase 9) as mediators of PRH action and was supported by in vitro and in vivo analyses.
We observed PRH S163C:S177C attenuated VSMC proliferation, and migration and enhanced VSMC differentiation at least in part via STAT-1 and HDAC-9 signaling while promoting endothelial repair and anti-inflammatory properties. These findings highlight the potential for PRH S163C:S177C to preserve endothelial function whilst suppressing intimal thickening, and reducing late vein graft failure.
晚期静脉移植物失功是由内皮细胞(EC)损伤和炎症引起的内膜增厚引起的,后者促进血管平滑肌细胞(VSMC)去分化、迁移和增殖。非磷酸化 PRH(富含脯氨酸的同源域)S163C:S177C 提供了增强的稳定性和持续的抗有丝分裂作用。因此,我们研究了腺病毒递送的 PRH S163C:S177C 蛋白是否通过 VSMC 表型修饰来减轻内膜增厚,而不会对 EC 产生不利影响。
通过腺病毒在体外(人隐静脉-VSMCs 和人隐静脉-ECs)和体内(结扎的小鼠颈总动脉)表达 PRH S163C:S177C。通过增殖、迁移和凋亡的定量以及 Western 印迹法评估收缩丝蛋白和胶原凝胶收缩来评估表型。通过 VCAM(血管细胞黏附蛋白)-1、ICAM(细胞间黏附分子)-1、白细胞介素-6 和单核细胞趋化因子-1 测量和单核细胞黏附来量化 EC 炎症。利用下一代测序鉴定 PRH 作用的新下游介质,并在体内研究这些介质和内膜增厚。
与病毒对照相比,PRH S163C:S177C 在人隐静脉-VSMCs 中抑制增殖、迁移和凋亡,并促进收缩表型(增强收缩丝蛋白和胶原凝胶收缩)。PRH S163C:S177C 在人隐静脉-ECs 中的表达显著减少细胞凋亡,而不影响细胞增殖和迁移,同时降低 TNF(肿瘤坏死因子)-α诱导的 VCAM-1 和 ICAM-1 和单核细胞黏附和抑制白细胞介素-6 和单核细胞趋化因子-1 蛋白水平。PRH S163C:S177C 在结扎的小鼠颈总动脉中的表达显著损害颈动脉结扎诱导的新生内膜增殖和增厚,而不减少内皮细胞覆盖。下一代测序揭示了 STAT-1(信号转导和转录激活因子 1)和 HDAC-9(组蛋白去乙酰化酶 9)作为 PRH 作用的介质,体外和体内分析均支持这一结果。
我们观察到 PRH S163C:S177C 至少部分通过 STAT-1 和 HDAC-9 信号通路抑制 VSMC 增殖和迁移,并增强 VSMC 分化,同时促进内皮修复和抗炎特性。这些发现强调了 PRH S163C:S177C 保留内皮功能的潜力,同时抑制内膜增厚和减少晚期静脉移植物失功。
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