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Analysis of Senescence-Related Differentiation Potentials and Gene Expression Profiles in Human Dental Pulp Stem Cells

机译:人牙髓干细胞中衰老相关分化电位和基因表达谱的分析

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Introduction: Dental pulp stem cell (DPSC)-mediated dental pulp regeneration is considered a promising method for the treatment of deep caries with pulpitis. However, mesenchymal stem cell (MSC) senescence is an adverse factor from the perspective of cell-based therapies. In this study, we investigated the characteristics and expression profiles of DPSCs from young and old donors. Methods: DPSCs from young and old donors were cultured in differentiation medium, and their differentiation potentials were assessed. Long noncoding RNA (LncRNA) microarray assays and a bioinformatic analysis were performed to investigate differences in LncRNA and mRNA expression profiles between DPSCs from young and old donors. Results: We found that DPSCs from young donors exhibited more powerful proliferation ability and greater osteogenic and adipogenic differentiation potentials than DPSCs from old donors. In DPSCs from young donors, numerous LncRNAs were significantly up- (n = 389) or down-regulated (n = 172) compared to DPSCs from old donors. Furthermore, 304 mRNAs were differentially expressed, including 247 up- regulated genes and 57 down-regulated genes in DPSCs from young donors. The bioinformatic analysis identified that several pathways may be associated with DPSC characteristics, such as those involved in the cell cycle and RNA transport, and revealed nuclear transcription factor Y subunit beta, general transcription factor IIB, and nuclear receptor subfamily 3 group C member 1 as core regulatory factors and FR249114, FR299091, and ENST00000450004 as core LncRNAs. Conclusions: Our results indicated that senescence impaired the proliferation and differentiation potentials of DPSCs and that donor age is an important factor that affects their use for tooth regeneration. We also provide insight into the mechanisms responsible for senescence in DPSCs. (C) 2016 S. Karger AG, Basel
机译:介绍:牙科纸浆干细胞(DPSC)介导的牙髓再生被认为是治疗具有牙髓炎的深龋的有希望的方法。然而,间充质干细胞(MSC)衰老是从基于细胞的疗法的角度来看的不利因素。在这项研究中,我们调查了来自年轻人和旧捐助者的DPSC的特征和表达谱。方法:来自少年和旧捐赠者的DPSC在分化培养基中培养,评估其分化潜力。进行长的非分量RNA(LNCRNA)微阵列测定和生物信息分析以研究来自年轻和旧捐赠者的DPSC之间的LNCRNA和mRNA表达谱的差异。结果:我们发现,来自年轻捐赠者的DPSCs表现出比旧捐赠者的DPSC更强大的增殖能力和更大的成骨和脂肪分化潜力。与来自旧捐赠者的DPSC相比,在来自年轻捐献者的DPSC中,许多LNCRNA显着增加 - (n = 389)或下调(n = 172)。此外,304mRNA差异表达,包括来自年轻供体的DPSC中的247个上调基因和57个下调基因。生物信息分析鉴定出几种途径可以与DPSC特征相关,例如参与细胞周期和RNA传输的DPSC特征,并揭示了核转录因子Y亚基β,一般转录因子IIB和核受体亚家族3组C成员1核心监管因素和FR249114,FR299091和ENST00000450004作为核心LNCRNA。结论:我们的结果表明,衰老损害了DPSC的增殖和分化潜力,并且供体年龄是影响其用于牙齿再生的重要因素。我们还提供了对负责DPSC中衰老的机制的洞察力。 (c)2016年S. Karger AG,巴塞尔

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  • 来源
    《Cells tissues organs》 |2017年第1期|共11页
  • 作者单位

    Cent S Univ Xiangya Stomatol Hosp 72 Xiang Ya Rd Changsha 410078 Hunan Peoples R China;

    Cent S Univ Xiangya Stomatol Hosp 72 Xiang Ya Rd Changsha 410078 Hunan Peoples R China;

    Cent S Univ Xiangya Stomatol Hosp 72 Xiang Ya Rd Changsha 410078 Hunan Peoples R China;

    Capital Med Univ Sch Stomatol Lab Mol Signaling &

    Stem Cell Therapy Beijing Peoples R China;

    Capital Med Univ Sch Stomatol Lab Mol Signaling &

    Stem Cell Therapy Beijing Peoples R China;

    Capital Med Univ Sch Stomatol Lab Mol Signaling &

    Stem Cell Therapy Beijing Peoples R China;

    Capital Med Univ Sch Stomatol Lab Mol Signaling &

    Stem Cell Therapy Beijing Peoples R China;

    Capital Med Univ Beijing Key Lab Tooth Regenerat &

    Funct Reconstru Mol Lab Gene Therapy &

    Tooth;

    Cent S Univ Xiangya Stomatol Hosp 72 Xiang Ya Rd Changsha 410078 Hunan Peoples R China;

    Capital Med Univ Sch Stomatol Lab Mol Signaling &

    Stem Cell Therapy Beijing Peoples R China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 人体形态学;
  • 关键词

    Dental pulp stem cells; Differentiation potentials; Expression profile; Long noncoding RNA; Senescence;

    机译:牙科纸浆干细胞;分化势;表达谱;长的非编码RNA;衰老;

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