Cellular Reprogramming and Embryo Biotechnology Laboratory, Dental Research Institute and CLS21, Seoul National University School of Dentistry, Seoul, Republic of Korea.
Tissue Eng Part A. 2012 Feb;18(3-4):331-41. doi: 10.1089/ten.TEA.2011.0074. Epub 2011 Oct 18.
Embryonic stem cells (ESCs) are pluripotent and can differentiate into all somatic cell types. ESCs are an alternative solution to hard tissue regeneration and skeletal tissue repair to treat bone diseases and defects using regenerative strategies. Parthenogenetic ESCs (PESCs) may be a useful alternative stem cell source for tissue repair and regeneration. The defects in full-term development of this cell type enable researchers to avoid the ethical concerns related to ESC research. Moreover, in female patients, if the PESCs are derived from oocytes, then they will have that patient's genetic information. Here, we present data demonstrating that osteogenic differentiation of PESCs can be promoted by insulin-like growth factor 2 (IGF2). PESCs were plated onto Petri dishes with ESC culture medium supplemented with or without IGF2, followed by culturing of the cells for 1 week. PESCs formed floating aggregates called embryoid bodies (EBs). An osteogenic lineage was induced from the EBs by incubating them in medium containing serum, ascorbic acid, β-glycerophosphate, and retionic acid, with or without IGF2, for 20 days. Gene expression of specific osteoblastic markers such as osteocalcin, osteopontin, osteonectin, bone sialoprotein, collagen type-I, alkaline phosphatase, and Runx2 (Cbfa-I) was analyzed by real-time polymerase chain reaction. The expression level of osteocalcin, osteopontin, osteonectin, and alkaline phosphatase was twofold higher in IGF2-treated PESC derivatives than IGF2-naive PESC derivatives. In vivo experiments were also performed using a critical-sized calvarial defect mouse model. Ten weeks after cell transplantation, more bone tissue regeneration was observed in the IGF2-treated PESC transplantation group than in IGF2-naive PESC transplantation group. Both our in vitro and in vivo data indicate that IGF2 induces osteogenic differentiation of PESCs. Addition of IGF2 may reactivate imprinting genes in PESCs that are only expressed in the paternal genome and are normally silent in PESCs. Our findings provide insights into the mechanisms of skeletal tissue repair and the imprinting mechanisms active in stem cells.
胚胎干细胞(ESCs)具有多能性,可以分化为所有体细胞类型。ESCs 是一种替代方法,可以使用再生策略治疗骨疾病和缺陷,从而进行硬组织再生和骨骼组织修复。孤雌生殖胚胎干细胞(PESCs)可能是组织修复和再生的有用替代干细胞来源。这种细胞类型在完全发育过程中的缺陷使研究人员能够避免与 ESC 研究相关的伦理问题。此外,在女性患者中,如果 PESCs 来源于卵母细胞,那么它们将具有该患者的遗传信息。在这里,我们提供的数据表明胰岛素样生长因子 2(IGF2)可以促进 PESC 的成骨分化。将 PESCs 铺在含有 ESC 培养基的 Petri 培养皿上,培养基中添加或不添加 IGF2,然后培养细胞 1 周。PESCs 形成称为类胚体(EBs)的悬浮聚集物。通过在含有血清、抗坏血酸、β-甘油磷酸和维甲酸的培养基中孵育 EBs,诱导其向成骨谱系分化,添加或不添加 IGF2,持续 20 天。通过实时聚合酶链反应分析特定成骨细胞标志物的基因表达,如骨钙素、骨桥蛋白、骨连接蛋白、骨涎蛋白、I 型胶原、碱性磷酸酶和 Runx2(Cbfa-I)。IGF2 处理的 PESC 衍生物中的骨钙素、骨桥蛋白、骨连接蛋白和碱性磷酸酶的表达水平比 IGF2 未处理的 PESC 衍生物高两倍。还进行了体内实验,使用临界大小颅骨缺损小鼠模型。细胞移植后 10 周,在 IGF2 处理的 PESC 移植组中观察到更多的骨组织再生,而在 IGF2 未处理的 PESC 移植组中则没有。我们的体外和体内数据均表明 IGF2 诱导 PESC 的成骨分化。添加 IGF2 可能会重新激活仅在父本基因组中表达且在 PESC 中通常沉默的 PESC 印迹基因。我们的发现为骨骼组织修复的机制和干细胞中活跃的印迹机制提供了深入的了解。
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