Department of Neurology, Henry Ford Health System, Detroit, MI 48202, United States.
Department of Neurology, Henry Ford Health System, Detroit, MI 48202, United States.
Neurobiol Dis. 2019 May;125:154-162. doi: 10.1016/j.nbd.2019.01.019. Epub 2019 Jan 29.
The death of mature oligodendrocytes (OLs) leads to demyelination in the central nervous system (CNS) and subsequently to functional deficits. Remyelination requires the differentiation of oligodendrocyte progenitor cells (OPCs) into myelinating OLs, which in the CNS with neurodegenerative diseases such as multiple sclerosis (MS), is often inhibited. Among the inhibitors of OPC differentiation are toll-like receptor 2 (TLR2) and interleukin-1 receptor-associated kinase 1 (IRAK1) signaling, and both are negatively regulated by microRNA-146a (miR-146a). Therefore, we hypothesized that increase of miR-146a level in the CNS would foster OPC differentiation and remyelination by inhibiting the TLR2/IRAK1 signaling pathway. Here, we tested this hypothesis using exogenous miR-146a mimics and a mouse model of MS, experimental autoimmune encephalomyelitis (EAE) induced by immunization with myelin proteolipid protein peptide (PLP). EAE mice were treated by miR-146a mimics or miR-146a mimic negative controls, respectively, which initiated at day 14 post immunization, once a week for 6 consecutive weeks. Neurological function was monitored daily. Immunofluorescent staining, qRT-PCR and Western blot were used to measure the differentiation of OPCs and myelination, and to investigate the underlying mechanisms of action of miR-146a. Using a fluorescence tracing approach, we found that miR-146a mimics crossed the blood brain barrier and targeted OPCs and microglia/macrophages after systemic administration. MiR-146a mimic treatment substantially improved neurological functional outcome, increased the number of newly generated OLs which may facilitate remyelination in the CNS. The cell number, cytokine level and protein levels of M2 phonotype of microglia/macrophages significantly increased, while cytokine and protein levels of the M1 phenotype significantly decreased after miR-146a mimic treatment. Increased OPC differentiation and remyelination were associated with reduction of TLR2/IRAK1 signaling pathway activity by miR-146a mimic treatment. This study provides insight into the cellular and molecular bases for the therapeutic effects of miR-146a on OPC differentiation and remyelination, and suggests the potential of enhancing miR-146a as a treatment of demyelinating disorders.
成熟少突胶质细胞 (OLs) 的死亡会导致中枢神经系统 (CNS) 脱髓鞘,随后出现功能缺陷。髓鞘再生需要少突胶质前体细胞 (OPC) 分化为髓鞘形成 OLs,而在多发性硬化症 (MS) 等神经退行性疾病的 CNS 中,这种分化通常受到抑制。OPC 分化的抑制剂包括 Toll 样受体 2 (TLR2) 和白细胞介素-1 受体相关激酶 1 (IRAK1) 信号通路,两者均受 microRNA-146a (miR-146a) 的负调控。因此,我们假设 CNS 中 miR-146a 水平的增加会通过抑制 TLR2/IRAK1 信号通路促进 OPC 分化和髓鞘再生。在这里,我们使用外源性 miR-146a 模拟物和实验性自身免疫性脑脊髓炎 (EAE) 小鼠模型来测试这一假设,该模型通过用髓鞘蛋白脂蛋白肽 (PLP) 免疫诱导产生。EAE 小鼠分别用 miR-146a 模拟物或 miR-146a 模拟物阴性对照治疗,从免疫后第 14 天开始,每周一次,连续 6 周。每天监测神经功能。免疫荧光染色、qRT-PCR 和 Western blot 用于测量 OPC 分化和髓鞘形成,并研究 miR-146a 的作用机制。通过荧光示踪方法,我们发现 miR-146a 模拟物经系统给药后可穿过血脑屏障并靶向 OPCs 和小胶质细胞/巨噬细胞。miR-146a 模拟物治疗显著改善了神经功能结局,增加了新生成的 OLs 的数量,可能有助于 CNS 中的髓鞘再生。miR-146a 模拟物治疗后,小胶质细胞/巨噬细胞的 M2 表型细胞数量、细胞因子水平和蛋白水平显著增加,而 M1 表型的细胞因子和蛋白水平显著降低。OPC 分化和髓鞘再生的增加与 miR-146a 模拟物治疗降低 TLR2/IRAK1 信号通路活性有关。这项研究为 miR-146a 对 OPC 分化和髓鞘再生的治疗作用提供了细胞和分子基础方面的见解,并表明增强 miR-146a 作为脱髓鞘疾病治疗方法的潜力。
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