Bitar Malak, Brown Robert A, Salih Vehid, Kidane Asmeret G, Knowles Jonathan C, Nazhat Showan N
Division of Biomaterials and Tissue Engineering, UCL Eastman Dental Institute, 256 Gray's Inn Road, London, WC1X 8LD, United Kingdom.
Biomacromolecules. 2008 Jan;9(1):129-35. doi: 10.1021/bm701112w. Epub 2007 Dec 21.
Plastic compression of hyperhydrated collagen gels produces tissue-like scaffolds of enhanced biomechanical properties. By increasing collagen density, these scaffolds could be developed into highly Biomimetic cell-seeded templates. When utilizing three-dimensional (3-D) scaffold systems for tissue repair, and indeed when investigating the cytocompatibility of two-dimensional (2-D) surfaces, the cell seeding density is often overlooked. In this study, we investigated this potentially critical parameter using MG-63 cells seeded in the dense collagen scaffolds. This is conducted within the overall scope of developing these scaffolds for bone repair. Cell proliferation, osteoblastic differentiation, and matrix remodelling capacity in relation to various seeding densities, ranging from 10(5) to 10(8) cells/ml compressed collagen, were evaluated in vitro. This was performed using the AlamarBlue assay, quantitative polymerase chain reaction (qPCR), and tensile mechanical analysis respectively. Variations in cell seeding density significantly influenced cell proliferation where lower initial seeding density resulted in higher proliferation rates as a function of time in culture. Gene transcription levels for alkaline phosphatase (ALPL), runt-related transcription factor 2 (RUNX2), and osteonectin (SPARC) were also found to be dependent on the cell density. While ALPL transcription was down-regulated with culturing time for all seeding densities, there was an increase in RUNX2 and SPARC transcription, particularly for scaffolds with cell densities in the range 10(6)-10(7) cells/ml collagen. Furthermore, this range of seeding density affected cell capacity in conducting collagenous matrix degradation as established by analyzing matrix metalloproteinase 1 (MMP1) transcription and scaffold mechanical properties. This study has shown that the seeded cell population in the three-dimensional dense collagen scaffolds clearly affected the degree of osteoblastic cell proliferation, differentiation, and some aspects of matrix remodelling activity. The seeding density played a major role in influencing the corresponding cell differentiation and cell-matrix interaction.
对过度水化的胶原凝胶进行塑性压缩可产生具有增强生物力学性能的组织样支架。通过增加胶原蛋白密度,这些支架可被开发成高度仿生的细胞接种模板。在利用三维(3-D)支架系统进行组织修复时,以及在研究二维(2-D)表面的细胞相容性时,细胞接种密度常常被忽视。在本研究中,我们使用接种在致密胶原支架中的MG-63细胞研究了这个潜在的关键参数。这是在为骨修复开发这些支架的总体范围内进行的。在体外评估了与各种接种密度相关的细胞增殖、成骨细胞分化和基质重塑能力,接种密度范围为每毫升压缩胶原10⁵至10⁸个细胞。分别使用AlamarBlue检测、定量聚合酶链反应(qPCR)和拉伸力学分析来进行此项研究。细胞接种密度的变化显著影响细胞增殖,较低的初始接种密度导致在培养过程中随着时间推移增殖率更高。还发现碱性磷酸酶(ALPL)、 runt相关转录因子2(RUNX2)和骨连接蛋白(SPARC)的基因转录水平取决于细胞密度。虽然所有接种密度下ALPL转录随培养时间下调,但RUNX2和SPARC转录增加,特别是对于细胞密度在每毫升胶原10⁶ - 10⁷个细胞范围内的支架。此外,通过分析基质金属蛋白酶1(MMP1)转录和支架力学性能确定,这个接种密度范围影响细胞进行胶原基质降解的能力。本研究表明,三维致密胶原支架中的接种细胞群体明显影响成骨细胞增殖、分化程度以及基质重塑活动的某些方面。接种密度在影响相应的细胞分化和细胞 - 基质相互作用中起主要作用。
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