School of Pharmaceutical Sciences (Shenzhen), Sun Yat-sen University, Shenzhen, 510631, China.
Clinical Research Institute, First People's Hospital of Foshan, Foshan, 528000, China.
Theranostics. 2022 Mar 28;12(7):3131-3149. doi: 10.7150/thno.69217. eCollection 2022.
: Demyelination is a major component of white matter injury, characterized by oligodendrocyte (OL) death and myelin sheath loss, which result in memory loss and cognitive impairment in the context of ischemic stroke. Accumulating evidence has shown that OLs can be generated by the direct activation of defined transcription factors (TFs) in human induced pluripotent stem cells (hiPSCs); however, the rapid acquisition of single TF-induced OL progenitor cells (OPCs) as cell therapy for ischemic stroke remains to be thoroughly explored. : A stable, chemically defined protocol was used to generate a substantial number of transplantable and functional OLs through the partial inhibition of sonic hedgehog (Shh) activity by GANT61 during neural induction from hiPSCs and sequential induction of TF Olig2 overexpression. Transcriptome and metabolome analyses further revealed a novel molecular event in which Olig2 regulates OL differentiation from hiPSC-derived neural progenitor cells (NPCs). Olig2-induced NG2 OPCs (Olig2-OPCs) were then evaluated for their therapeutic potential in cell-based therapy for ischemic stroke. GANT61 treatment resulted in a motor neuron (MN)-OL fate switch during neural induction, and induced overexpression of Olig2 accelerated oligodendroglial lineage cell specification. Olig2-OPCs expressed typical oligodendroglial lineage marker genes, including , , and , and displayed superior ability to differentiate into mature OLs . Mechanistically, Olig2-OPCs showed increased gene expression of the peroxisome proliferator-activated receptor γ (PPARγ) signaling pathway, and activated CEPT1-mediated phospholipogenesis. Functionally, inhibiting PPARγ and knocking down further compromised the terminal differentiation of Olig2-OPCs. Most importantly, when transplanted into a rat model of transient middle cerebral artery occlusion (tMCAO), Olig2-OPCs efficiently promoted neurological functional recovery by reducing neuronal death, promoting remyelination, and rescuing spatial memory decline. We developed a stable, chemically defined protocol to generate OPCs/OLs with partial inhibition of Shh activity by GANT61 from hiPSCs and sequentially induced the expression of the single TF Olig2. Olig2-OPC transplantation may be an ideal alternative approach for ischemic stroke rehabilitation therapy.
髓鞘脱失是白质损伤的主要组成部分,其特征是少突胶质细胞(OL)死亡和髓鞘鞘丢失,导致缺血性中风背景下的记忆丧失和认知障碍。越来越多的证据表明,OL 可以通过在人诱导多能干细胞(hiPSC)中直接激活特定的转录因子(TFs)来产生;然而,快速获得单一 TF 诱导的 OL 祖细胞(OPC)作为缺血性中风的细胞治疗仍有待深入探索。我们使用一种稳定的、化学定义的方案,通过 GANT61 在 hiPSC 神经诱导过程中部分抑制 sonic hedgehog(Shh)活性,并随后诱导 TF Olig2 的过表达,来生成大量可移植和功能的 OL。转录组和代谢组分析进一步揭示了一个新的分子事件,其中 Olig2 调节 hiPSC 衍生的神经祖细胞(NPC)向 OL 分化。然后评估 Olig2 诱导的 NG2 OPC(Olig2-OPC)在缺血性中风的基于细胞的治疗中的治疗潜力。GANT61 处理导致神经诱导过程中的运动神经元(MN)-OL 命运转换,并且诱导的 Olig2 过表达加速少突胶质谱系细胞的特化。Olig2-OPC 表达典型的少突胶质谱系标记基因,包括 、 、和 ,并显示出向成熟 OL 分化的优越能力。从机制上讲,Olig2-OPC 表现出过氧化物酶体增殖物激活受体 γ(PPARγ)信号通路基因表达增加,并且激活 CEPT1 介导的磷脂生成。从功能上讲,抑制 PPARγ 和敲低 进一步损害了 Olig2-OPC 的终末分化。最重要的是,当移植到短暂性大脑中动脉闭塞(tMCAO)大鼠模型中时,Olig2-OPC 通过减少神经元死亡、促进髓鞘再生和挽救空间记忆下降,有效地促进了神经功能的恢复。我们开发了一种稳定的、化学定义的方案,通过 GANT61 从 hiPSC 中部分抑制 Shh 活性并顺序诱导单个 TF Olig2 的表达来生成 OPC/OL。Olig2-OPC 移植可能是缺血性中风康复治疗的理想替代方法。
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