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首页> 外文期刊>Biomaterials >The spatial and temporal control of cell migration by nanoporous surfaces through the regulation of ERK and integrins in fibroblasts
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The spatial and temporal control of cell migration by nanoporous surfaces through the regulation of ERK and integrins in fibroblasts

机译:通过调节成纤维细胞中的ERK和整联蛋白来控制纳米多孔表面对细胞迁移的时空控制

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摘要

Nanotopography controls cell behaviours, such as cell adhesion and migration. However, the mechanisms responsible for topology-mediated cellular functions are not fully understood. A variety of nanopores was fabricated on 316L stainless steel to investigate the effects of spatial control on the growth and function of fibroblasts, the temporal regulation of integrins, and their effects on migration. The NIH-3T3 fibroblast cell line was cultured on the nanopore surfaces, whose pore diameters ranged from 40 to 210 nm. The 40 and 75 nm nanopores enhanced cell proliferation, focal adhesion formation and protein expression of vinculin and β-tubulin after 24 h of incubation. Integrin expression was analysed by qPCR, which showed the extent of spatial and temporal regulation achieved by the nanopores. The protein expression of pERK1/2 was greatly attenuated in cells grown on 185 and 210 nm nanopore surfaces at 12 and 24 h. In summary, the 40 and 75 nm nanopore surfaces promoted cell adhesion and migration in fibroblasts by controlling the temporal expression of integrins and ERK1/2. The current study provides insight into the improvement of the design of stainless steel implants and parameters that affect biocompatibility. The ability to regulate the expression of integrin and ERK1/2 using nanopore surfaces could lead to further applications of surface modification in the fields of biomaterials science and tissue engineering.
机译:纳米形貌控制细胞行为,例如细胞粘附和迁移。但是,尚未完全了解负责拓扑介导的细胞功能的机制。在316L不锈钢上制造了各种纳米孔,以研究空间控制对成纤维细胞生长和功能,整联蛋白的时间调控及其对迁移的影响。在纳米孔表面上培养NIH-3T3成纤维细胞系,其孔径范围为40至210nm。孵育24小时后,40和75 nm纳米孔可增强细胞增殖,粘着斑形成以及长春花素和β-微管蛋白的蛋白表达。通过qPCR分析整联蛋白表达,其显示了纳米孔实现的时空调节的程度。在12和24小时,在185和210 nm纳米孔表面生长的细胞中,pERK1 / 2的蛋白表达大大减弱。总之,通过控制整联蛋白和ERK1 / 2的时间表达,40和75 nm纳米孔表面促进了成纤维细胞中的细胞粘附和迁移。本研究为不锈钢植入物的设计改进和影响生物相容性的参数提供了见识。使用纳米孔表面调节整联蛋白和ERK1 / 2的表达的能力可能导致表面修饰在生物材料科学和组织工程领域的进一步应用。

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