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Optimization of culture media to enhance the growth of tissue engineered cartilage

机译:优化培养基,增强组织工程软骨的生长

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摘要

Tissue engineering is a promising option for cartilage repair. However, several hurdles still need to be overcome to develop functional tissue constructs suitable for implantation. One of the most common challenges is the general low capacity of chondrocytes to synthesize cartilage-specific extracellular matrix (ECM). While different approaches have been explored to improve the biosynthetic response of chondrocytes, several studies have demonstrated that the nutritional environment (e.g., glucose concentration and media volume) can have a profound effect on ECM synthesis. Thus, the purpose of this study was to optimize the formulation of cell culture media to upregulate the accumulation of cartilaginous ECM constituents (i.e., proteoglycans and collagen) by chondrocytes in 3D culture. Using response surface methodology, four different media factors (basal media, media volume, glucose, and glutamine) were first screened to determine optimal media formulations. Constructs were then cultured under candidate optimal media formulations for 4 weeks and analyzed for their biochemical and structural properties. Interestingly, the maximal accumulation of proteoglycans and collagen appeared to be elicited by different media formulations. Most notably, proteoglycan accumulation was favored by high volume, low glucose-containing DMEM/F12 (1:1) media whereas collagen accumulation was favored by high volume, high glucose-containing F12 media. While high glutamine-containing media elicited increased DNA content, glutamine concentration had no apparent effect on ECM accumulation. Therefore, optimizing the nutritional environment during chondrocyte culture appears to be a promising, straight-forward approach to improve cartilaginous tissue formation. Future work will investigate the combined effects of the nutritional environment and external stimuli.
机译:组织工程是软骨修复的有希望的选择。然而,需要克服几个障碍以开发适合植入的功能组织构造。最常见的挑战之一是软骨细胞的一般低容量,以合成软骨特异性细胞外基质(ECM)。虽然已经探索了不同的方法来改善软骨细胞的生物合成反应,但是有几个研究表明营养环境(例如,葡萄糖浓度和介质体积)可以对ECM合成具有深远的影响。因此,本研究的目的是优化细胞培养基的制剂,以通过3D培养物中的软骨细胞来上调软骨内ECM成分(即,,蛋白转基因组和胶原蛋白)的积累。使用响应表面方法,首先首先筛选四种不同的媒体因子(基础介质,培养基,葡萄糖和谷氨酰胺)以确定最佳介质配方。然后在候选最佳培养基制剂下培养构建体4周并分析它们的生化和结构性。有趣的是,蛋白质酚和胶原蛋白的最大积累似乎被不同的培养基配方引发。最值得注意的是,蛋白生成的积累受大容量,含低葡萄糖的DMEM / F12(1:1)培养基,而胶原蛋白积累受大容量,含有高葡萄糖的F12培养基的青睐。虽然高谷氨酰胺的培养基引发了增加的DNA含量,但谷氨酰胺浓度对ECM积累没有明显影响。因此,优化软骨细胞培养过程中的营养环境似乎是提高软骨组织形成的有希望的直接方法。未来的工作将研究营养环境和外部刺激的综合影响。

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