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Scaffold-free approach produces neocartilage tissue of similar quality as the use of HyStem™ and Hydromatrix™ scaffolds

机译:无支架的方法可产生与使用HyStem™和Hydromatrix™支架相似质量的新软骨组织

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摘要

AbstractNumerous biomaterials are being considered for cartilage tissue engineering, while scaffold-free systems have also been introduced. Thus, it is important to know do the scaffolds improve the formation of manufactured neocartilages. This study compares scaffold-free cultures to two scaffold-containing ones. Six million bovine primary chondrocytes were embedded in HyStem™ or HydroMatrix™ scaffolds, or suspended in scaffold-free chondrocyte culture medium, and then loaded into agarose gel supported culture well pockets. Neocartilages were grown in the presence of hypertonic high glucose DMEM medium for up to 6 weeks. By the end of culture periods, the formed tissues were analyzed by histological staining for proteoglycans (PGs) and type II collagen, gene expression measurements of aggrecan, Sox9, procollagen α1(II), and procollagen α2(I) were performed using quantitative RT-PCR, and analyses of PG contents and structure were conducted by spectrophotometric and agarose gel electrophoretic methods. Histological stainings showed that the PGs and type II collagen were abundantly present in both the scaffold-free and the scaffold-containing tissues. The PG content gradually increased following the culture period. However, the mRNA expression levels of the cartilage-specific genes of aggrecan, procollagen α1(II) and Sox9 gradually decreased following culture period, while procollagen α2(I) levels increased. After 6-week-cultivations, the PG concentrations in neocartilage tissues manufactured with HyStem™ or HydroMatrix™ scaffolds, and in scaffold-free agarose gel-supported cell cultures, were similar to native cartilage. No obvious benefits could be seen on the extracellular matrix assembly in HyStem™ or HydroMatrix™ scaffolds cultures.
机译:摘要许多生物材料正在考虑用于软骨组织工程,同时还引入了无支架系统。因此,重要的是要知道脚手架会改善人造新软骨的形成。这项研究比较了无支架文化与两种含支架文化。将六百万种牛原代软骨细胞嵌入HyStem™或HydroMatrix™支架中,或悬浮在无支架的软骨细胞培养基中,然后装入琼脂糖凝胶支持的培养孔袋中。新软骨在高渗高葡萄糖DMEM培养基的存在下生长长达6周。在培养期结束时,通过组织学染色分析形成的组织中的蛋白聚糖(PGs)和II型胶原蛋白,使用定量RT进行聚集蛋白聚糖,Sox9,前胶原α1(II)和前胶原α2(I)的基因表达测量通过分光光度法和琼脂糖凝胶电泳法进行-PCR,分析PG的含量和结构。组织学染色显示PGs和II型胶原在无支架和含支架的组织中大量存在。 PG含量在培养期后逐渐增加。然而,培养期后,聚集蛋白聚糖,前胶原α1(II)和Sox9的软骨特异性基因的mRNA表达水平逐渐降低,而前胶原α2(I)水平升高。培养6周后,用HyStem™或HydroMatrix™支架制造的新软骨组织和无支架琼脂糖凝胶支持的细胞培养物中的PG浓度与天然软骨相似。在HyStem™或HydroMatrix™支架培养物中的细胞外基质组装上看不到明显的益处。

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