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软骨细胞在 3D 中的再分化:黏附位点密度和基质弹性的影响。

Chondrocyte redifferentiation in 3D: the effect of adhesion site density and substrate elasticity.

机构信息

Institute for Biomechanics, ETH Zurich, Zurich, Switzerland.

出版信息

J Biomed Mater Res A. 2012 Jan;100(1):38-47. doi: 10.1002/jbm.a.33226. Epub 2011 Oct 4.

DOI:10.1002/jbm.a.33226
PMID:21972220
Abstract

To obtain sufficient cell numbers for cartilage tissue engineering with autologous chondrocytes, cells are typically expanded in monolayer culture. As a result, they lose their chondrogenic phenotype in a process called dedifferentiation, which can be reversed upon transfer into a 3D environment. We hypothesize that the properties of this 3D environment, namely adhesion site density and substrate elasticity, would influence this redifferentiation process. To test this hypothesis, chondrocytes were expanded in monolayer and their phenotypical transition was monitored. Agarose hydrogels manipulated to give different RGD adhesion site densities and mechanical properties were produced, cells were incorporated into the gels to induce redifferentiation, and constructs were analyzed to determine cell number and extracellular matrix production after 2 weeks of 3D culture. The availability of adhesion sites within the gels inhibited cellular redifferentiation. Glycosaminoglycan production per cell was diminished by RGD in a dose-dependent manner and cells incorporated into gels with the highest RGD density, remained positive for collagen type I and produced the least collagen type II. Substrate stiffness, in contrast, did not influence cellular redifferentiation, but softer gels contained higher cell numbers and ECM amounts after 2 weeks of culture. Our results indicate that adhesion site density but not stiffness influences the redifferentiation process of chondrocytes in 3D. This knowledge might be used to optimize the redifferentiation process of chondrocytes and thus the formation of cartilage-like tissue.

摘要

为了从自体软骨细胞中获得足够数量的细胞用于软骨组织工程,细胞通常在单层培养中进行扩增。因此,它们在称为去分化的过程中失去了软骨形成表型,可以在转移到 3D 环境中时逆转。我们假设这种 3D 环境的特性,即粘附位点密度和基质弹性,会影响这种再分化过程。为了验证这一假设,我们在单层中扩增了软骨细胞,并监测其表型转变。制作了琼脂糖水凝胶以获得不同的 RGD 粘附位点密度和机械性能,将细胞掺入凝胶中以诱导再分化,并分析构建体以确定在 3D 培养 2 周后的细胞数量和细胞外基质产生。凝胶内粘附位点的可用性抑制了细胞的再分化。糖胺聚糖的产生每细胞被 RGD 以剂量依赖性的方式减少,并且掺入 RGD 密度最高的凝胶中的细胞仍然对胶原蛋白 I 呈阳性,并产生最少的胶原蛋白 II。相比之下,基质刚度不会影响细胞的再分化,但在培养 2 周后,较软的凝胶中含有更高的细胞数量和 ECM 量。我们的结果表明,粘附位点密度而不是刚度会影响 3D 中软骨细胞的再分化过程。这些知识可用于优化软骨细胞的再分化过程,从而形成类软骨组织。

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