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Blue Laser Irradiation Enhances Extracellular Calcification of Primary Mesenchymal Stem Cells

机译:蓝色激光辐照增强原代间充质干细胞的细胞外钙化

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摘要

Background Data and Objective: Mesenchymal stem cells (MSCs) are multipotent cells present in adult bone marrow that replicate as undifferentiated cells and can differentiate to lineages of mesenchymal tissues. Homeostatic control of bone remodeling maintains bone mass by ensuring that bone resorption and bone formation occur sequentially and in a balanced manner. As most homeostatic functions occur in a circadian manner, a circadian clock could control bone mass. Here we show that laser irradiation can direct the extracellular calcification of mouse MSCs by altering the intracellular localization of the circadian rhythm protein cryptochrome 1 (CRY1). Materials and Methods: MSCs were irradiated with a blue laser (wavelength 405nm) for 180sec via a fiber attached to the bottom of the culture dish. After laser irradiation, the MSCs were incubated in osteogenic differentiation medium for 5d. After laser irradiation, circadian rhythm protein CRY1 was immunostained and histochemical staining for extracellular calcification was observed. Results: Laser irradiation promoted extracellular calcification of MSCs, induced the translocation of CRY1 protein from the cytoplasm to the nucleus, and decreased CRY1 mRNA levels quantified by real-time PCR. Since the timing of nuclear accumulation of clock proteins constitutes an important step in the transcription-translation feedback loop driving the circadian core oscillator, laser irradiation could provide a simple and effective technology for clock protein localization and turnover. Our results also indicate that CRY1 is a master regulator of circadian rhythm that regulates the extracellular calcification of MSCs. Conclusion: Laser irradiation could provide a simple and effective means of controlling the fate of MSCs as a therapeutic strategy, and act as a “molecular switch” of regulatory proteins by suppressing CRY transcription. Furthermore, this model system may be useful for exploring the cross-talk between circadian rhythm and cell function.
机译:背景资料和目的:间充质干细胞(MSCs)是成年骨髓中存在的多能细胞,可复制为未分化细胞,并可分化为间充质组织。通过确保骨骼吸收和骨骼形成顺序且平衡地发生,骨骼重建的稳态控制可保持骨骼质量。由于大多数稳态功能是以生物钟方式发生的,因此生物钟可以控制骨量。在这里,我们显示出激光照射可以通过改变昼夜节律蛋白cryptochrome 1(CRY1)的细胞内定位来指导小鼠MSC的细胞外钙化。材料和方法:通过附着在培养皿底部的光纤,用蓝色激光(波长405nm)照射MSC 180秒。激光照射后,将MSC在成骨分化培养基中孵育5天。激光照射后,对生物节律蛋白CRY1进行了免疫染色,并观察到了细胞外钙化的组织化学染色。结果:激光照射促进了MSCs的细胞外钙化,诱导了CRY1蛋白从细胞质到细胞核的转运,并降低了实时PCR定量的CRY1 mRNA水平。由于时钟蛋白核累积的时间构成了驱动生物钟核心振荡器的转录-翻译反馈回路中的重要步骤,因此激光照射可以为时钟蛋白的定位和周转提供简单有效的技术。我们的结果还表明,CRY1是昼夜节律的主要调节因子,可调节MSC的细胞外钙化。结论:激光照射可为控制MSC的命运提供一种简单有效的手段,作为治疗策略,并通过抑制CRY转录而充当调节蛋白的“分子开关”。此外,该模型系统对于探索昼夜节律与细胞功能之间的相互影响可能是有用的。

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  • 来源
    《Photomedicine and Laser Surgery》 |2009年第3期|493-498|共6页
  • 作者单位

    PRESTO, Japan Science and Technology Agency, Saitama, Japan.;

    Division of Sustainable Energy and Environmental Engineering, Graduate School of Engineering, Osaka University, Osaka, Japan.;

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