Tenocyte-imprinted底物:脂肪组织来源的间充质干细胞中一种基于地形的腱源性分化诱导剂。

ty10086 提交于 周三, 08/25/2021 - 17:23
文章英文标题
Tenocyte-imprinted substrate: a topography-based inducer for tenogenic differentiation in adipose tissue-derived mesenchymal stem cells.
正文
以干细胞分化为基础的肌腱组织工程近年来极大的关注。先前的研究已经考察了细胞印迹聚二甲基硅氧烷( PDMS )基底对干细胞诱导分化的影响。在本研究中,我们用腱细胞形态作为正模,在PDMS上构建了腱细胞印迹基底。利用扫描电子显微镜( SEM )和原子力显微镜对这种在PDMS上的腱细胞复制品的形貌和形貌进行了评价。研究了脂肪间充质干细胞( ADSCs )中腱细胞复制品的诱导分化能力,并与其他诱导剂进行了比较,包括与腱细胞复制品相似的组织复制品( SEM )、脱细胞肌腱、骨形态发生蛋白( BMP ) - 12等。这种比较给我们估计了与其他诱导剂相比,腱细胞印迹PDMS (本研究称为细胞复制)诱导分化的能力。为此,ADSCs分为5组,分别为对照、细胞复制、组织复制、脱细胞肌腱和BMP-12。ADSCs分别接种于各组,7、14 d后采用实时逆转录聚合酶链反应( RT-PCR )技术进行调查。我们的研究结果表明,尽管生长因子对腱源性分化的影响较高,但细胞复制物也能诱导ADSCs的腱细胞标志物表达(巩膜轴和腱调素)。而且,细胞复制品的诱导分化能力大于组织复制品。免疫细胞化学分析显示,ADSCs在细胞复制品上培养14天,可在蛋白水平上诱导巩膜轴突和腱调蛋白表达。另外,免疫组织化学表明,与体外有希望的结果相反,在腱细胞印迹PDMS上培养的ADSCs与未经处理的ADSCs相差不大。这些研究结果可能导致生产廉价的细胞培养板或生物材料,可以诱导干细胞分化而不需要生长因子或其他补充。
文章内容(英文)
Tendon tissue engineering based on stem cell differentiation has attracted a great deal of attention in recent years. Previous studies have examined the effect of cell-imprinted polydimethylsiloxane (PDMS) substrate on induction differentiation in stem cells. In this study, we used tenocyte morphology as a positive mold to create a tenocyte-imprinted substrate on PDMS. The morphology and topography of this tenocyte replica on PDMS was evaluated with scanning electron microscopy (SEM) and atomic force microscopy. The tenogenic differentiation induction capacity of the tenocyte replica in adipose tissue-derived mesenchymal stem cells (ADSCs) was then investigated and compared with other groups, including tissue replica (which was produced similarly to the tenocyte replica and was evaluated by SEM), decellularized tendon, and bone morphogenic protein (BMP)-12, as other potential inducers. This comparison gives us an estimate of the ability of tenocyte-imprinted PDMS (called cell replica in the present study) to induce differentiation compared to other inducers. For this reason, ADSCs were divided into five groups, including control, cell replica, tissue replica, decellularized tendon and BMP-12. ADSCs were seeded on each group separately and investigated by the real-time reverse transcription polymerase chain reaction (RT-PCR) technique after seven and 14 days. Our results showed that in spite of the higher effect of the growth factor on tenogenic differentiation, the cell replica can also induce tenocyte marker expression (scleraxis and tenomodulin) in ADSCs. Moreover, the tenogenic differentiation induction capacity of the cell replica was greater than tissue replica. Immunocytochemistry analysis revealed that ADSCs seeding on the cell replica for 14 days led to scleraxis and tenomodulin expression at the protein level. In addition, immunohistochemistry indicated that contrary to the promising results in vitro, there was little difference between ADSCs cultured on tenocyte-imprinted PDMS and untreated ADSCs. The results of such studies could lead to the production of inexpensive cell culture plates or biomaterials that can induce differentiation in stem cells without growth factors or other supplements.
来源出处
Journal|[J]Biomedical MaterialsVolume 15, Issue 3. 2020. PP 035014-035014
DOI
https://doi.org/10.1088/1748-605X/AB6709

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备注说明:

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