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The Effect of Substrate Stiffness Thickness and Cross-Linking Density on Osteogenic Cell Behavior

机译:基质刚度厚度和交联密度对成骨细胞行为的影响

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摘要

Osteogenic cells respond to mechanical changes in their environment by altering their spread area, morphology, and gene expression profile. In particular, the bulk modulus of the substrate, as well as its microstructure and thickness, can substantially alter the local stiffness experienced by the cell. Although bone tissue regeneration strategies involve culture of bone cells on various biomaterial scaffolds, which are often cross-linked to enhance their physical integrity, it is difficult to ascertain and compare the local stiffness experienced by cells cultured on different biomaterials. In this study, we seek to characterize the local stiffness at the cellular level for MC3T3-E1 cells plated on biomaterial substrates of varying modulus, thickness, and cross-linking concentration. Cells were cultured on flat and wedge-shaped gels made from polyacrylamide or cross-linked collagen. The cross-linking density of the collagen gels was varied to investigate the effect of fiber cross-linking in conjunction with substrate thickness. Cell spread area was used as a measure of osteogenic differentiation. Finite element simulations were used to examine the effects of fiber cross-linking and substrate thickness on the resistance of the gel to cellular forces, corresponding to the equivalent shear stiffness for the gel structure in the region directly surrounding the cell. The results of this study show that MC3T3 cells cultured on a soft fibrous substrate attain the same spread cell area as those cultured on a much higher modulus, but nonfibrous substrate. Finite element simulations predict that a dramatic increase in the equivalent shear stiffness of fibrous collagen gels occurs as cross-linking density is increased, with equivalent stiffness also increasing as gel thickness is decreased. These results provide an insight into the response of osteogenic cells to individual substrate parameters and have the potential to inform future bone tissue regeneration strategies that can optimize the equivalent stiffness experienced by a cell.
机译:成骨细胞通过改变其扩散区域,形态和基因表达谱来响应其环境中的机械变化。特别地,基板的体积模量以及其微观结构和厚度可以实质上改变电池所经历的局部刚度。尽管骨组织再生策略涉及在各种生物材料支架上培养骨细胞,这些支架通常被交联以增强其物理完整性,但很难确定和比较在不同生物材料上培养的细胞所经历的局部硬度。在这项研究中,我们寻求表征镀覆在具有不同模量,厚度和交联浓度的生物材料基质上的MC3T3-E1细胞在细胞水平上的局部刚度。将细胞培养在由聚丙烯酰胺或交联胶原蛋白制成的扁平楔形凝胶上。改变胶原蛋白凝胶的交联密度以研究纤维交联与底物厚度的关系。细胞扩散面积用作成骨分化的量度。有限元模拟被用来检查纤维交联和基底厚度对凝胶对细胞力的抵抗力的影响,对应于细胞周围直接区域中凝胶结构的等效剪切刚度。这项研究的结果表明,在软纤维基质上培养的MC3T3细胞与在模量高得多但非纤维基质上培养的MC3T3细胞具有相同的扩散细胞面积。有限元模拟预测,随着交联密度的增加,纤维胶原蛋白凝胶的当量剪切刚度会急剧增加,当凝胶厚度减小时,当量刚度也会增加。这些结果提供了对成骨细胞对单个底物参数反应的深入了解,并有可能为将来的骨组织再生策略提供参考,该策略可以优化细胞所经历的等效刚度。

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