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Nanoporosity of Alumina Surfaces Induces Different Patterns of Activation in Adhering Monocytes/Macrophages

机译:氧化铝表面的纳米多孔性在粘附的单核细胞/巨噬细胞中诱导不同的活化方式

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摘要

The present study shows that alumina nanotopography affects monocyte/macrophage behavior. Human mononuclear cells cultured on alumina membranes with pore diameters of 20 and 200 nm were evaluated in terms of cell adhesion, viability, morphology, and release of proinflammatory cytokines. After 24 hours, cell adhesion was assessed by means of light microscopy and cell viability by measuring LDH release. The inflammatory response was evaluated by quantifying interleukin-1β and tumour necrosis factor-α. Finally, scanning electron microscopy was used to study cell morphology. Results showed pronounced differences in cell number, morphology, and cytokine release depending on the nanoporosity. Few but highly activated cells were found on the 200 nm porous alumina, while relatively larger number of cells were found on the 20 nm porous surface. However, despite their larger number, the cells adhering on the 20 nm surface exhibited reduced pro-inflammatory activity. The data of this paper implies that nanotopography could be exploited for controlling the inflammatory response to implants.
机译:本研究表明氧化铝纳米形貌影响单核细胞/巨噬细胞的行为。在细胞粘附,生存力,形态和促炎细胞因子释放方面评估了在直径为20和200nm的氧化铝膜上培养的人单核细胞。 24小时后,通过光学显微镜评估细胞粘附,并通过测量LDH释放来评估细胞生存力。通过定量白介素-1β和肿瘤坏死因子-α来评估炎症反应。最后,使用扫描电子显微镜研究细胞形态。结果表明,取决于纳米孔隙度,细胞数量,形态和细胞因子释放存在明显差异。在200 nm的多孔氧化铝上发现很少但高度活化的细胞,而在20 nm的多孔表面上发现了相对大量的细胞。然而,尽管数量更多,但粘附在20 thenm表面的细胞却显示出降低的促炎活性。本文的数据暗示可以利用纳米形貌来控制对植入物的炎症反应。

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