内皮蛋白二硫键异构酶 A1 通过 SLC3A2 和 LAMC1 增强高血糖中的膜硬度和血小板-内皮细胞相互作用。
Endothelial protein disulfide isomerase A1 enhances membrane stiffness and platelet-endothelium interaction in hyperglycemia via SLC3A2 and LAMC1.
机构信息
Laboratorio de Biologia Vascular (LVascBio), LIM-64, Instituto do Coração (InCor), Hospital das Clinicas HCFMUSP, Faculdade de Medicina, Universidade de São Paulo, São Paulo, Brazil.
Federal University of Maranhão, Physics Department, Laboratory of Biophysics and Nanosystems, São Luís, Brazil.
出版信息
J Thromb Haemost. 2024 Nov;22(11):3305-3321. doi: 10.1016/j.jtha.2024.08.001. Epub 2024 Aug 14.
BACKGROUND
Diabetes carries an increased risk of cardiovascular disease and thromboembolic events. Upon endothelial dysfunction, platelets bind to endothelial cells to precipitate thrombus formation; however, it is unclear which surface proteins regulate platelet-endothelium interaction. We and others have shown that peri/epicellular protein disulfide isomerase A1 (pecPDI) influences the adhesion and migration of vascular cells.
OBJECTIVES
We investigated whether pecPDI regulates adhesion-related molecules on the surface of endothelial cells and platelets that influence the binding of these cells in hyperglycemia.
METHODS
Immunofluorescence was used to assess platelet-endothelium interaction in vitro, cytoskeleton reorganization, and focal adhesions. Hydrogen peroxide production was assessed via Amplex Red assays (ThermoFisher Scientific). Cell biophysics was assessed using atomic force microscopy. Secreted proteins of interest were identified through proteomics (secretomics), and targets were knocked down using small interfering RNA. Protein disulfide isomerase A1 (PDI) contribution was assessed using whole-cell PDI or pecPDI inhibitors or small interfering RNA.
RESULTS
Platelets of healthy donors adhered more onto hyperglycemic human umbilical vein endothelial cells (HUVECs). Endothelial, but not platelet, pecPDI regulated this effect. Hyperglycemic HUVECs showed marked cytoskeleton reorganization, increased HO production, and elongated focal adhesions. Indeed, hyperglycemic HUVECs were stiffer compared with normoglycemic cells. PDI and pecPDI inhibition reversed the abovementioned processes in hyperglycemic cells. A secretomics analysis revealed 8 proteins secreted in a PDI-dependent manner by hyperglycemic cells. Among these, we showed that genetic deletion of LAMC1 and SLC3A2 decreased platelet-endothelium interaction and did not potentiate the effects of PDI inhibitors.
CONCLUSION
Endothelial pecPDI regulates platelet-endothelium interaction in hyperglycemia through adhesion-related proteins and alterations in endothelial membrane biophysics.
背景
糖尿病会增加心血管疾病和血栓栓塞事件的风险。在内皮功能障碍时,血小板与内皮细胞结合,导致血栓形成;然而,目前尚不清楚哪些表面蛋白调节血小板-内皮细胞相互作用。我们和其他人已经表明,周质/细胞周蛋白二硫键异构酶 A1(pecPDI)影响血管细胞的黏附和迁移。
目的
我们研究了 pecPDI 是否调节内皮细胞和血小板表面的黏附相关分子,这些分子影响高血糖状态下这些细胞的结合。
方法
使用免疫荧光法评估体外血小板-内皮细胞相互作用、细胞骨架重排和焦点黏附。通过 Amplex Red 测定法(ThermoFisher Scientific)评估过氧化氢的产生。使用原子力显微镜评估细胞生物物理学。通过蛋白质组学(分泌组学)鉴定感兴趣的分泌蛋白,并使用小干扰 RNA 敲低靶标。使用全细胞 PDI 或 pecPDI 抑制剂或小干扰 RNA 评估 PDI 贡献。
结果
健康供体的血小板更易黏附于高血糖人脐静脉内皮细胞(HUVECs)。内皮细胞而非血小板 pecPDI 调节了这种作用。高血糖 HUVECs 表现出明显的细胞骨架重排、HO 生成增加和延长的焦点黏附。事实上,与正常血糖细胞相比,高血糖 HUVECs 更硬。PDI 和 pecPDI 抑制逆转了高血糖细胞中的上述过程。分泌组学分析显示 8 种蛋白质以 PDI 依赖的方式由高血糖细胞分泌。在这些蛋白质中,我们表明 LAMC1 和 SLC3A2 的基因缺失减少了血小板-内皮细胞相互作用,并且不会增强 PDI 抑制剂的作用。
结论
内皮 pecPDI 通过与黏附相关的蛋白和内皮膜生物物理学的改变来调节高血糖中的血小板-内皮细胞相互作用。
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