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Spreading proliferation and differentiation of human dental pulp stem cells on chitosan scaffolds immobilized with RGD or fibronectin

机译:人牙髓干细胞在RGD或纤连蛋白固定化的壳聚糖支架上的扩散增殖和分化

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摘要

Nowadays, human dental pulp stem cells (hDPSCs) became more attractive for therapeutic purposes because of their high proliferation and differentiation potential. Thus, coupling the desired cellular characteristics of hDPSCs with good biomaterial properties of the chitosan scaffolds provide an interesting approach for tissue engineering applications. On the other hand, scaffold surface modification is also needed to promote stem cell adhesion since chitosan lacks adhesion motifs to support direct cell anchorage. In this study, hDPSCs were isolated from third molars of healthy female individuals (aged 16–25) with enzymatic digestion. For cell culture studies, the chitosan scaffolds which have approximately 9 mm diameter and 2 mm thickness with interconnected structure were prepared by freeze-drying. To support cellular attachment the scaffolds were covalently immobilized with either RGD (arginine-glycine-aspartic acid) or fibronectin (Fn) molecules. Cells were seeded on chitosan scaffolds with or without immobilized RGD and fibronectin. Cell attachment, spreading, adhesion behaviors and proliferation capacity were examined by scanning electron microscopy, immunofluorescence staining and PrestoBlue® assays, respectively. In addition, differentiation potential of hDPSCs on Fn immobilized chitosan scaffolds was determined with real time reverse transcriptase polymerase chain reaction analysis. The results showed that chitosan scaffolds were not able to support stem cell attachment. hDPSCs on chitosan scaffolds formed spheroids more quickly and the size of spheroids were smaller than on chitosan-RGD while Fn-immobilized chitosan scaffolds strongly supported cellular attachment but not odontogenic differentiation. The results suggest that the Fn-immobilized chitosan scaffolds may serve as good three-dimensional substrates for dental pulp stem cell attachment and proliferation. In the case of dental regeneration, they must be supported by appropriate biosignals to induce odontogenic differentiation.
机译:如今,人类牙髓干细胞(hDPSCs)由于具有很高的增殖和分化潜能而变得更具治疗吸引力。因此,将hDPSCs的所需细胞特性与壳聚糖支架的良好生物材料特性结合在一起,为组织工程应用提供了一种有趣的方法。另一方面,由于壳聚糖缺乏支持直接细胞锚定的粘附基序,因此还需要支架表面修饰以促进干细胞粘附。在这项研究中,hDPSCs是通过酶消化从健康女性(16-25岁)的第三磨牙中分离得到的。为了进行细胞培养研究,通过冷冻干燥制备了直径约9毫米,厚度2毫米且具有相互连接结构的壳聚糖支架。为了支持细胞附着,将支架与RGD(精氨酸-甘氨酸-天冬氨酸)或纤连蛋白(Fn)分子共价固定。将细胞接种在具有或不具有固定的RGD和纤连蛋白的壳聚糖支架上。分别通过扫描电子显微镜,免疫荧光染色和PrestoBlue ®测定来检测细胞的附着,扩散,粘附行为和增殖能力。另外,通过实时逆转录酶聚合酶链反应分析确定了hDPSCs在Fn固定化壳聚糖支架上的分化潜力。结果表明,壳聚糖支架不能支持干细胞附着。与壳聚糖-RGD相比,壳聚糖支架上的hDPSCs形成球体的速度更快,且球体的大小更小,而固定化Fn的壳聚糖支架则强烈支持细胞附着,但不支持牙源性分化。结果表明,固定化Fn的壳聚糖支架可以作为牙髓干细胞附着和增殖的良好三维底物。在牙齿再生的情况下,它们必须由适当的生物信号支持以诱导牙源性分化。

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