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Investigating the Effects of Tissue-Specific Extracellular Matrix on the Adipogenic and Osteogenic Differentiation of Human Adipose-Derived Stromal Cells Within Composite Hydrogel Scaffolds

机译:研究组织特异性细胞外基质对复合水凝胶支架中人脂肪衍生的基质细胞脂肪发生和骨质发生分化的影响

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摘要

While it has been postulated that tissue-specific bioscaffolds derived from the extracellular matrix (ECM) can direct stem cell differentiation, systematic comparisons of multiple ECM sources are needed to more fully assess the benefits of incorporating tissue-specific ECM in stem cell culture and delivery platforms. To probe the effects of ECM sourced from decellularized adipose tissue (DAT) or decellularized trabecular bone (DTB) on the adipogenic and osteogenic differentiation of human adipose-derived stem/stromal cells (ASCs), a novel detergent-free decellularization protocol was developed for bovine trabecular bone that complemented our established detergent-free decellularization protocol for human adipose tissue and did not require specialized equipment or prolonged incubation times. Immunohistochemical and biochemical characterization revealed enhanced sulphated glycosaminoglycan content in the DTB, while the DAT contained higher levels of collagen IV, collagen VI and laminin. To generate platforms with similar structural and biomechanical properties to enable assessment of the compositional effects of the ECM on ASC differentiation, micronized DAT and DTB were encapsulated with human ASCs within methacrylated chondroitin sulfate (MCS) hydrogels through UV-initiated crosslinking. High ASC viability (>90%) was observed over 14 days in culture. Adipogenic differentiation was enhanced in the MCS+DAT composites relative to the MCS+DTB composites and MCS controls after 14 days of culture in adipogenic medium. Osteogenic differentiation studies revealed a peak in alkaline phosphatase (ALP) enzyme activity at 7 days in the MCS+DTB group cultured in osteogenic medium, suggesting that the DTB had bioactive effects on osteogenic protein expression. Overall, the current study suggests that tissue-specific ECM sourced from DAT or DTB can act synergistically with soluble differentiation factors to enhance the lineage-specific differentiation of human ASCs within 3-D hydrogel systems.
机译:虽然已经假设来自细胞外基质(ECM)的组织特异性Bioscods可以直接茎细胞分化,所以需要进行多种ECM源的系统比较,以更充分地评估在干细胞培养和产物中掺入组织特异性ECM的益处平台。为了探测ECM来自脱脂脂肪组织(DAT)或脱细胞小梁(DTB)对人脂肪和成骨细胞(ASCS)的脂肪发生和成骨分化的影响,开发了一种新型的无溶血性脱细胞化方案牛小梁骨,其补充了我们已建立的无洗涤剂的脱细胞化方案,用于人类脂肪组织,不需要专门的设备或延长的孵育时间。免疫组织化学和生化表征在DTB中显示出增强的硫酸化糖胺聚糖含量,而DED含有较高水平的胶原IV,胶原蛋白VI和层粘连蛋白。为了产生具有相似结构和生物力学性质的平台,以实现ECM对ASC分化对ECM对ASC分化的组成效应的评估,通过UV引发的交联在甲基丙烯酸甲酸硫酸盐(MCS)水凝胶中包封了微粉化DAT和DTB。在培养14天内观察到高ASC活力(> 90%)。在脂肪培养基中培养14天后,MCS + DAT复合材料中,在MCS + DTB复合材料中增强了脂肪生成分化。成骨分化研究显示在骨质发生介质中培养的MCS + DTB组的7天内碱性磷酸酶(ALP)酶活性的峰,表明DTB对骨质发生蛋白表达具有生物活性作用。总的来说,目前的研究表明,来自DAT或DTB的组织特异性ECM可以协同作用,以可溶性分化因子协同作用,以增强3-D水凝胶系统内人ASC的谱系特异性分化。

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