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调控通过反蛋白石法制备的大孔无机膜的细胞响应。

Regulation of cellular responses to macroporous inorganic films prepared by the inverse-opal method.

机构信息

Division of Chemistry for Materials, Graduate School of Engineering, Mie University, Tsu, Mie, Japan.

出版信息

Colloids Surf B Biointerfaces. 2011 May 1;84(1):187-97. doi: 10.1016/j.colsurfb.2010.12.032. Epub 2011 Jan 7.

DOI:10.1016/j.colsurfb.2010.12.032
PMID:21273052
Abstract

Regenerative medicine for repairing damaged body tissues has recently become critically important. Cell culture scaffolds are required for the control of cell attachment, proliferation, and differentiation in in vitro cell cultures. A new strategy to control cell adhesion, morphology, and proliferation was developed by culturing mouse osteoblast-like MC3T3-E1 cells on novel cell culture scaffolds fabricated using ordered nanometer-sized pores (100, 300, 500, and 1000 nm). Results of this study indicate that after 72 h of incubation, the number of cells cultured on a silica film with a pore size of 1000 nm was similar to or slightly lower than that cultured on a non-porous control silica film. Films with 100-500 nm pore sizes, however, resulted in the cell growth inhibition. Morphology of the cultured cells revealed increased elongation and the formation of actin stress fibers was virtually absent on macroporous silica films with 100-500 nm pore size. Vinculin molecules expressed in cells cultured on the non-porous silica films showed many clear focal adhesions, whereas focal contacts were insufficiently formed in cells cultured on macroporous films. The influence of hydroxyapatite (HAp) and alumina scaffolds on the behavior of MC3T3-E1 cells was also evaluated. The proliferation rate of MC3T3-E1 cells cultured on HAp films with 1000 nm pore size was increased to approximately 20% above than that obtained of cells cultured on non-porous HAp films. These results demonstrate that the pore size and constituents of films play a role in controlling the morphology and proliferation rate of MC3T3-E1 cells.

摘要

再生医学对于修复受损的人体组织至关重要。细胞培养支架用于控制体外细胞培养中的细胞附着、增殖和分化。本研究通过在使用有序纳米级孔(100、300、500 和 1000nm)制造的新型细胞培养支架上培养鼠成骨样 MC3T3-E1 细胞,开发了一种控制细胞黏附、形态和增殖的新策略。结果表明,孵育 72 小时后,在孔径为 1000nm 的二氧化硅膜上培养的细胞数量与在无孔对照二氧化硅膜上培养的细胞数量相似或略低。然而,孔尺寸为 100-500nm 的薄膜导致细胞生长抑制。培养细胞的形态显示出伸长的增加,并且在具有 100-500nm 孔径的大孔二氧化硅膜上几乎不存在肌动蛋白应力纤维的形成。在无孔二氧化硅膜上培养的细胞中表达的 vinculin 分子显示出许多清晰的焦点粘附,而在大孔膜上培养的细胞中焦点接触形成不足。还评估了羟基磷灰石(HAp)和氧化铝支架对 MC3T3-E1 细胞行为的影响。在孔径为 1000nm 的 HAp 膜上培养的 MC3T3-E1 细胞的增殖率比在无孔 HAp 膜上培养的细胞的增殖率增加了约 20%。这些结果表明,薄膜的孔径和成分在控制 MC3T3-E1 细胞的形态和增殖率方面起着重要作用。

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