首页> 外文期刊>Tissue engineering, Part A >Acellular bone colonization and aggregate culture conditions diversely influence murine periosteum mesenchymal stem cell differentiation potential in long-term in vitro osteoinductive conditions
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Acellular bone colonization and aggregate culture conditions diversely influence murine periosteum mesenchymal stem cell differentiation potential in long-term in vitro osteoinductive conditions

机译:在长期体外骨诱导条件下,脱细胞骨定植和聚集培养条件对鼠骨膜间充质干细胞分化潜能的影响不同

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摘要

Periosteum contains mesenchymal stem cells (Pe-MSCs) that contribute to normal bone growth, healing, and turnover; understanding Pe-MSC capabilities may shed light over the treatment of bone defects using tissue engineering. Bone tissue regeneration needs in vitro bone precursors or stem cell coculture onto specific scaffolds but, despite extensive research in the field, very little is known about the matrix structure of the tissue-engineered tissues and the scaffold's effects on cell differentiation. To this purpose we have selected a clonal population (murine Pe-MSCs) that was seeded and differentiated onto an acellular bone scaffold. Cell differentiation was assessed after 3 months and 1 year by molecular, histological, biochemical, and biophysical analyses and results were compared with the same osteoinduced clonal cells cultured as cellular aggregates. Our data show that Pe-MSCs cultured onto acellular bone scaffold develop a complex three-dimensional matrix and an osteoblastic phenotype but do not produce hydroxyapatite (HA); moreover, they seem able to reabsorb the colonized bone scaffold. On the contrary, cells cultured as three-dimensional aggregates differentiate and produce osteoblastic markers and HA nanocrystals.
机译:骨膜含有间充质干细胞(Pe-MSC),可促进正常的骨生长,愈合和周转。了解Pe-MSC的功能可能会阐明使用组织工程技术治疗骨缺损的方法。骨组织再生需要在特定支架上进行体外骨前体或干细胞共培养,但是,尽管在该领域进行了广泛研究,但对组织工程组织的基质结构以及支架对细胞分化的影响知之甚少。为此,我们选择了一个克隆种群(鼠类Pe-MSC),将其播种并分化到无细胞的骨支架上。在3个月和1年后,通过分子,组织学,生化和生物物理分析评估细胞分化,并将结果与​​培养为细胞聚集体的相同骨诱导性克隆细胞进行比较。我们的数据表明,在无细胞骨骼支架上培养的Pe-MSC可以形成复杂的三维矩阵和成骨细胞表型,但不会产生羟磷灰石(HA)。而且,它们似乎能够重新吸收定植的骨支架。相反,培养成三维聚集体的细胞分化并产生成骨细胞标志物和HA纳米晶体。

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