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Role of the ERK1/2 Signaling Pathway in Osteogenesis of Rat Tendon-Derived Stem Cells in Normoxic and Hypoxic Cultures

机译:ERK1 / 2信号通路在常氧和低氧培养物中大鼠肌腱衍生干细胞成骨中的作用

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摘要

Background: Ectopic ossification and increased vascularization are two common phenomena in the chronic tendinopathic tendon. The increased vascularization usually leads to an elevated local oxygen tension which is one of micro-environments that can influence differentiate status of stem cells.Objective: This study aimed to investigate the osteogenesis capacity of rat tendon-derived stem cells TDSCs (rTDSCs) in normoxic and hypoxic cultures, and to study the role of ERK1/2 signaling pathway in this process.Methods: rTDSCs were subjected to osteogenesis inductive culture in hypoxic (3% O2) and normoxic (20% O2) conditions. The inhibitor U0126 was added along with culture medium to determine the role of ERK1/2 signaling pathway. Cell viability, cell proliferation, alizarin red staining, alkaline phosphatase (AKP) activity, gene expression (ALP, osteocalcin, collagen I and RUNX2) and protein expression (p-ERK1/2 and RUNX2) of osteogenic-cultured rTSDCs were analyzed in this study.Results: Hypoxic and normoxic culture had no effects on cell viability of rTDSCs, whereas the proliferation potential of rTDSCs was significantly increased in hypoxic culture. The osteogenesis capacity of rTDSCs in normoxic culture was significantly promoted compared with hypoxic culture, which was reflected by an increased alizarin red staining intensity, an elevated ALP activity, and the up-regulated gene (ALP, osteocalcin, collagen I and RUNX2) or protein (RUNX2) expression of osteogenic makers. However, the osteogenesis capacity of rTDSCs in both hypoxic and normoxic cultures was attenuated by the inhibitor U0126.Conclusion: Normoxic culture promotes osteogenic differentiation of rTDSCs compared with the hypoxic culture, and the ERK1/2 signaling pathway is involved in this process.
机译:背景:异位骨化和血管生成增加是慢性肌腱性肌腱的两种常见现象。血管形成的增加通常会导致局部氧张力升高,这是可能影响干细胞分化状态的微环境之一。目的:本研究旨在研究大鼠肌腱干细胞TDSCs(rTDSCs)在常氧状​​态下的成骨能力。方法:在低氧(3%O2)和常氧(20%O2)条件下,对rTDSCs进行成骨诱导培养,以研究ERK1 / 2信号通路在该过程中的作用。将抑制剂U0126与培养基一起添加,以确定ERK1 / 2信号通路的作用。在此分析了成骨培养的rTSDC的细胞活力,细胞增殖,茜素红染色,碱性磷酸酶(AKP)活性,基因表达(ALP,骨钙蛋白,胶原蛋白I和RUNX2)和蛋白质表达(p-ERK1 / 2和RUNX2)。结果:低氧和常氧培养对rTDSCs的细胞活力没有影响,而低氧培养物中rTDSCs的增殖潜力显着增加。与低氧培养相比,常氧培养中rTDSCs的成骨能力显着提高,这反映为茜素红染色强度增加,ALP活性升高以及基因(ALP,骨钙蛋白,胶原蛋白I和RUNX2)或蛋白上调(RUNX2)表达成骨细胞。然而,抑制剂U0126减弱了低氧和常氧培养物中rTDSCs的成骨能力。结论:与低氧培养相比,高氧培养促进rTDSCs的成骨分化,并且ERK1 / 2信号通路参与了这一过程。

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