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Stem Cells from Human Exfoliated Deciduous Teeth (SHEDs) and Dental Pulp Stem Cells (DPSCs) Display a Similar Profile with Pericytes

机译:来自人脱色齿齿(棚)和牙科纸浆干细胞(DPSC)的干细胞显示与周细相关的型材

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Background . Pericytes play an important role in forming functional blood vessels and establishing stable and effective microcirculation, which is crucial for vascular tissue engineering. The slow ex vivo expansion rate, limited proliferative capacity, and variability of tissue-specific phenotypes would hinder experimental studies and clinical translation of primary pericytes. In this study, the angiogenic and pericyte functions of stem cells from human exfoliated deciduous teeth (SHEDs) and postnatal human dental pulp stem cells (DPSCs) were investigated. Methods . Osteogenic and adipogenic induction assays were performed to evaluate the mesenchymal potential of SHEDs, DPSCs, and pericytes. An in vitro Matrigel angiogenesis assay was conducted to reveal the ability of SHEDs, DPSCs, and pericytes to stabilize vascular-like structures. Quantitative real-time polymerase chain reaction (RT-qPCR) was performed to evaluate mRNA expression. Flow cytometry, western blotting, and immunostaining were used to assess the protein expression. Wound healing and transwell assays were performed to evaluate the migration ability of SHEDs, DPSCs, and pericytes. Results . The osteogenic and adipogenic induction assays showed that SHEDs, DPSCs, and pericytes exhibited similar stem cell characteristics. The mRNA expression levels of PDGFR- β , α -SMA, NG2, and DEMSIN in SHEDs and DPSCs cultured in EC medium were significantly higher than those in the control groups on day 7 ( ), but significantly higher than those in the pericytes group on day 14 ( ). Flow cytometry showed that high proportions of SHEDs and DPSCs were positive for various pericyte markers on day 7. The DPSCs, SHEDs, and pericytes displayed strong migration ability; however, there was no significant difference among the groups ( ). Conclusion . The SHEDs and DPSCs display a profile similar to that of pericytes. Our study lays a solid theoretical foundation for the clinical use of dental pulp stem cells as a potential candidate to replace pericytes.
机译:背景 。细胞在形成功能血管和建立稳定且有效的微循环中起重要作用,这对于血管组织工程至关重要。慢性体内膨胀率,有限的增殖能力和组织特异性表型的可变性将阻碍原发性周细胞的实验研究和临床翻译。在该研究中,研究了干细胞从人出剥落的齿(棚)和产后人牙髓干细胞(DPSC)的血管生成和周刊官能。方法 。进行成骨和脂肪发生诱导测定以评估棚孢子,DPSC和周刊的间充质潜力。进行体外Matrigel血管生成测定以揭示血液,DPSC和周细胞的能力稳定血管状结构。进行定量实时聚合酶链反应(RT-QPCR)以评估mRNA表达。流式细胞术,蛋白质印迹和免疫染料用于评估蛋白质表达。进行伤口愈合和Transwell测定以评估棚孢子,DPSC和周刊的迁移能力。结果 。成骨和脂肪发生的诱导测定显示出血小板,DPSC和围网表现出类似的干细胞特征。 PDGFR-β,α-β,NG2和DEMSIN的MRNA表达水平在EC培养基中培养的SHEDS和DPSCs在第7天()中显着高于对照组,但显着高于细胞组中的对照组第14天()。流式细胞术显示,第7天的各种周刊标志物的高比例为梭菌和DPSC是阳性的。DPSCS,Sheds和围网显示出强烈的迁移能力;但是,组()之间没有显着差异。结论 。 Sheds和DPSCS显示类似于周刊的轮廓。我们的研究为牙科纸浆干细胞作为潜在候选者施用牙科纸浆干细胞的纯粹理论基础。

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