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Dentin tubule orientation determines odontoblastic differentiation in vitro: A morphological study

机译:牙本质小管取向决定体外成牙本质细胞分化:一项形态学研究

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摘要

Odontoblasts are post-mitotic cells responsible for maintenance of the dentin, and are therefore important for dental health. In some cases, irreversible pulpitis leads to necrosis and consequently death of odontoblasts. Regenerative endodontics (RE) uses the concept of tissue engineering to restore the root canals to a healthy state, allowing for continued development of the root and surrounding tissue. Human dental pulp stem cells (hDPSCs) have been successfully used in RE to restore odontoblast function. Surface microgeometry is one of the most important factors involved in the induction of differentiation of hDPSCs into odontoblast-like cells. Although different authors have demonstrated the importance of a dentin-like surface with accessible dentin tubules to induce differentiation of hDPSCs, the ultrastructural characteristics of the cells and the secreted extracellular matrix have not been studied in depth. Here, we used an acellular dentin scaffold containing dentin tubules in different spatial geometries, which regulated their accessibility to cells. hDPSCs were cultured on the scaffolds for up to 6 weeks. Systematic characterization of differentiated cells was performed using both optical (hematoxylin and eosin, Masson trichrome, and immunohistochemical determination of dentin sialoprotein [DSSP]) and transmission electron microscopy. The results presented here indicated that cells grown on the dentin surface containing accessible dentin tubules developed a characteristic odontoblastic phenotype, with cellular processes similar to native odontoblasts. The cell organization and characteristics of secreted extracellular matrix were also similar to those of native dentin tissue. Cells grown on non-accessible dentin tubule surfaces secreted a more abundant and dense extracellular matrix, and developed a different phenotype consisting of secretory flat cells organized in layers. Cells grown far from the scaffold, i.e., directly on the culture well surface, developed a secretory phenotype probably influenced by biochemical factors released by the dentin scaffold or differentiated cells. The results presented here support the use of hDPSCs to regenerate dentin and show the utility of scaffold microgeometry for determining the differentiation and secretory phenotype of cultured cells.
机译:成牙本质细胞是负责维持牙本质的有丝分裂后细胞,因此对于牙齿健康很重要。在某些情况下,不可逆的牙髓炎会导致坏死,从而导致成牙本质细胞死亡。再生牙髓学(RE)使用组织工程学的概念将根管恢复到健康状态,从而使根管和周围组织得以持续发展。人牙髓干细胞(hDPSCs)已成功用于RE中恢复成牙本质细胞功能。表面微观几何结构是诱导hDPSCs分化为成牙本质细胞样细胞的最重要因素之一。尽管不同的作者已经证明了具有可触及的牙本质小管的牙本质样表面对诱导hDPSCs分化的重要性,但尚未深入研究细胞和分泌的细胞外基质的超微结构特征。在这里,我们使用了包含不同空间几何形状的牙本质小管的脱细胞牙本质支架,从而调节了它们对细胞的可及性。 hDPSCs在支架上培养长达6周。使用光学显微镜(苏木精和曙红,Masson三色和牙本质唾液蛋白[DSSP]的免疫组织化学测定)和透射电子显微镜对分化的细胞进行系统表征。此处显示的结果表明,在含有可触及的牙本质小管的牙本质表面上生长的细胞发展出特征性的牙胚细胞表型,其细胞过程类似于天然成牙本质细胞。分泌的细胞外基质的细胞组织和特征也与天然牙本质组织的相似。在不可触及的牙本质小管表面生长的细胞分泌更丰富和密集的细胞外基质,并发展出由表层组织的分泌性扁平细胞组成的不同表型。远离支架生长的细胞,即直接在培养孔表面生长的细胞,出现了分泌型,可能受牙本质支架或分化细胞释放的生化因子的影响。这里介绍的结果支持hDPSCs再生牙本质的使用,并显示了支架微几何学在确定培养细胞的分化和分泌表型方面的实用性。

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