Department of Chemical and Materials Engineering, Chang Gung University, Kwei-San, Taoyuan 33302, Taiwan.
Department of Plastic and Reconstructive Surgery and Craniofacial Research Center, Chang Gung Memorial Hospital, Linkou, Chang Gung University School of Medicine, Kwei-San, Taoyuan 33305, Taiwan.
Int J Mol Sci. 2018 Jan 26;19(2):370. doi: 10.3390/ijms19020370.
In this study, we first used gelatin/chondroitin-6-sulfate/hyaluronan/chitosan highly elastic cryogels, which showed total recovery from large strains during repeated compression cycles, as 3D scaffolds to study the effects of cyclic dynamic compressive loading on chondrocyte gene expression and extracellular matrix (ECM) production. Dynamic culture of porcine chondrocytes was studied at 1 Hz, 10% to 40% strain and 1 to 9 h/day stimulation duration, in a mechanical-driven multi-chamber bioreactor for 14 days. From the experimental results, we could identify the optimum dynamic culture condition (20% and 3 h/day) to enhance the chondrocytic phenotype of chondrocytes from the expression of marker (, , , , and ) genes by quantitative real-time polymerase chain reactions (qRT-PCR) and production of ECM (GAGs and Col II) by biochemical analysis and immunofluorescence staining. With up-regulated growth factor ( and ) genes, co-culture of chondrocytes with porcine adipose-derived stem cells (ASCs) was employed to facilitate chondrogenic differentiation of ASCs during dynamic culture in cryogel scaffolds. By replacing half of the chondrocytes with ASCs during co-culture, we could obtain similar production of ECM (GAGs and Col II) and expression of , but reduced expression of , and . Subcutaneous implantation of cells/scaffold constructs in nude mice after mono-culture (chondrocytes or ASCs) or co-culture (chondrocytes + ASCs) and subject to static or dynamic culture condition in vitro for 14 days was tested for tissue-engineering applications. The constructs were retrieved 8 weeks post-implantation for histological analysis by Alcian blue, Safranin O and Col II immunohistochemical staining. The most abundant ectopic cartilage tissue was found for the chondrocytes and chondrocytes + ASCs groups using dynamic culture, which showed similar neo-cartilage formation capability with half of the chondrocytes replaced by ASCs for co-culture. This combined co-culture/dynamic culture strategy is expected to cut down the amount of donor chondrocytes needed for cartilage-tissue engineering.
在这项研究中,我们首先使用明胶/软骨素-6-硫酸盐/透明质酸/壳聚糖高弹性冷冻凝胶作为 3D 支架,研究了周期性动态压缩载荷对软骨细胞基因表达和细胞外基质 (ECM) 产生的影响。在机械驱动的多腔生物反应器中,以 1Hz、10%至 40%应变和 1 至 9 小时/天的刺激持续时间,对猪软骨细胞进行动态培养,持续 14 天。从实验结果中,我们可以确定最佳的动态培养条件(20%和 3 小时/天),通过定量实时聚合酶链反应 (qRT-PCR) 检测标记基因 (、、、、和) 的表达和生化分析和免疫荧光染色检测 ECM(GAGs 和 Col II)的产生,来增强软骨细胞的软骨细胞表型。通过上调生长因子(和)基因,将软骨细胞与猪脂肪来源干细胞 (ASC) 共培养,以促进 ASC 在冷冻凝胶支架中的动态培养过程中的软骨分化。通过在共培养过程中用 ASC 替代一半的软骨细胞,我们可以获得类似的 ECM(GAGs 和 Col II)产生和表达,但减少了表达。在单培养(软骨细胞或 ASC)或共培养(软骨细胞+ASC)后,将细胞/支架构建体植入裸鼠皮下,并在体外进行静态或动态培养 14 天,用于组织工程应用。在植入后 8 周,通过阿尔辛蓝、番红 O 和 Col II 免疫组织化学染色对构建体进行组织学分析。在动态培养条件下,发现软骨细胞和软骨细胞+ASC 组的异位软骨组织最多,其中共培养时用 ASC 替代一半的软骨细胞,显示出相似的新软骨形成能力。这种联合共培养/动态培养策略有望减少软骨组织工程所需的供体软骨细胞数量。
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