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Engineering of a dermal equivalent: seeding and culturing fibroblasts in PEGT/PBT copolymer scaffolds.

机译:真皮等效产品的工程设计:在PEGT / PBT共聚物支架中播种和培养成纤维细胞。

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摘要

The engineering of dermal skin substitutes, using autologous fibroblasts, requires high seeding efficiencies, a homogeneous cell distribution in the scaffolds, and optimal culture conditions. Dynamic seeding in spinner flasks was used to seed and subsequently culture fibroblasts in three-dimensional scaffolds. Several seeding and culture variables were investigated. Simulation of medium movement with microspheres showed that three different regions existed in medium (outer, middle, and inner), where overall particle movement was different. In the middle region the flow was turbulent and scaffolds were best placed in this region. After fibroblast seeding, methylene blue staining and scanning electron microscopy analysis of the scaffolds showed that at a low stirring speed (20 rpm) fibroblasts attached mainly onto the upper part of the scaffold, and at 40 and 60 rpm fibroblasts attached and spread throughout the scaffolds. Measurements of total DNA content per scaffold showed that lower stirring speeds (20 and 40 rpm) resulted in significantly higher cell-seeding efficiencies (20 rpm, 99.8 +/- 11.3%; 40 rpm, 93.8 +/- 10.5%) compared with 60 rpm (85.9 +/- 5.3%). Seeding kinetics were comparable for all three speeds investigated. In subsequent studies, 40 rpm was chosen for seeding. Using initial cell numbers ranging from 0.3 x 10(6) to 1.5 x 10(6) fibroblasts per scaffold, seeding efficiencies higher than 85% were consistently found (n = 4). The culture of fibroblast-seeded scaffolds at different stirring speeds (10-80 rpm) showed that stirring speeds higher than 10 rpm significantly stimulated fibroblast proliferation and glycosaminoglycan and collagen deposition as compared with 10 rpm. After 21 days, scaffolds cultured at 80 rpm showed significantly more collagen deposition as compared with those maintained at lower speeds. In conclusion, to achieve high seeding efficiencies, uniform fibroblast distribution and tissue formation in a three-dimensional scaffold, fibroblasts can be dynamically seeded at 40 rpm and subsequently cultured at a stirring speed of 60-80 rpm in spinner flasks. This flexible system shows that it is feasible to tissue engineer autologous dermal substitutes in a clinically acceptable time frame.
机译:使用自体成纤维细胞的皮肤皮肤替代品的工程化需要高播种效率,支架中均匀的细胞分布以及最佳的培养条件。在旋转瓶中动态播种用于播种,随后在三维支架中培养成纤维细胞。研究了几种播种和栽培变量。用微球对介质运动的模拟表明,介质(外部,中间和内部)中存在三个不同的区域,其中总体粒子运动不同。在中间区域,流动湍流,最好在该区域放置脚手架。成纤维细胞接种后,对支架进行亚甲蓝染色和扫描电子显微镜分析表明,在低搅拌速度(20 rpm)下,成纤维细胞主要附着在支架的上部,而在40和60 rpm时成纤维细胞附着并分布在整个支架上。测量每个支架的总DNA含量表明,较低的搅拌速度(20和40 rpm)导致细胞接种效率(60 rpm,99.8 +/- 11.3%; 40 rpm,93.8 +/- 10.5%)明显高于60 rpm(85.9 +/- 5.3%)。研究的所有三种速度的播种动力学均相当。在随后的研究中,选择40 rpm进行播种。使用每个支架从0.3 x 10(6)到1.5 x 10(6)的成纤维细胞的初始细胞数,始终发现播种效率高于85%(n = 4)。在不同的搅拌速度(10-80 rpm)下培养的成纤维细胞接种支架显示,高于10 rpm的搅拌速度与10 rpm相比显着刺激了成纤维细胞增殖,糖胺聚糖和胶原蛋白沉积。 21天后,与保持较低速度的支架相比,以80 rpm培养的支架显示出明显更多的胶原蛋白沉积。总之,为了在三维支架中实现高播种效率,均匀的成纤维细胞分布和组织形成,可以以40 rpm的速度动态播种成纤维细胞,然后在旋转瓶中以60-80 rpm的搅拌速度进行培养。这种灵活的系统表明,在临床可接受的时间范围内,组织工程自体皮肤替代品是可行的。

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