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在少突胶质细胞转录因子1基因缺失的小鼠中,大脑中少突胶质细胞的髓鞘形成和轴突识别功能相互分离。

Myelinogenesis and axonal recognition by oligodendrocytes in brain are uncoupled in Olig1-null mice.

作者信息

Xin Mei, Yue Tao, Ma Zhenyi, Wu Fen-fen, Gow Alexander, Lu Q Richard

机构信息

Center for Developmental Biology, Department of Molecular Biology, University of Texas Southwestern Medical Center at Dallas, Dallas, Texas 75390, USA.

出版信息

J Neurosci. 2005 Feb 9;25(6):1354-65. doi: 10.1523/JNEUROSCI.3034-04.2005.

Abstract

Myelin-forming oligodendrocytes facilitate saltatory nerve conduction and support neuronal functions in the mammalian CNS. Although the processes of oligodendrogliogenesis and differentiation from neural progenitor cells have come to light in recent years, the molecular mechanisms underlying oligodendrocyte myelinogenesis are poorly defined. Herein, we demonstrate the pivotal role of the basic helix-loop-helix transcription factor, Olig1, in oligodendrocyte myelinogenesis in brain development. Mice lacking a functional Olig1 gene develop severe neurological deficits and die in the third postnatal week. In the brains of these mice, expression of myelin-specific genes is abolished, whereas the formation of oligodendrocyte progenitors is not affected. Furthermore, multilamellar wrapping of myelin membranes around axons does not occur, despite recognition and contact of axons by oligodendrocytes, and Olig1-null mice develop widespread progressive axonal degeneration and gliosis. In contrast, myelin sheaths are formed in the spinal cord, although the extent of myelination is severely reduced. At the molecular level, we find that Olig1 regulates transcription of the major myelin-specific genes, Mbp, Plp1, and Mag, and suppresses expression of a major astrocyte-specific gene, Gfap. Together, our data indicate that Olig1 is a central regulator of oligodendrocyte myelinogenesis in brain and that axonal recognition and myelination by oligodendrocytes are separable processes.

摘要

形成髓鞘的少突胶质细胞促进哺乳动物中枢神经系统中的跳跃式神经传导并支持神经元功能。尽管近年来少突胶质细胞发生和从神经祖细胞分化的过程已为人所知,但少突胶质细胞髓鞘形成的分子机制仍不清楚。在此,我们证明了碱性螺旋-环-螺旋转录因子Olig1在脑发育过程中少突胶质细胞髓鞘形成中的关键作用。缺乏功能性Olig1基因的小鼠会出现严重的神经功能缺陷,并在出生后第三周死亡。在这些小鼠的大脑中,髓鞘特异性基因的表达被消除,而少突胶质细胞祖细胞的形成不受影响。此外,尽管少突胶质细胞识别并接触轴突,但轴突周围并未发生髓鞘膜的多层包裹,且Olig1基因敲除小鼠出现广泛的进行性轴突变性和胶质增生。相比之下,虽然脊髓中的髓鞘形成程度严重降低,但仍形成了髓鞘。在分子水平上,我们发现Olig1调节主要髓鞘特异性基因Mbp、Plp1和Mag的转录,并抑制主要星形胶质细胞特异性基因Gfap的表达。总之,我们的数据表明Olig1是脑少突胶质细胞髓鞘形成的核心调节因子,并且少突胶质细胞对轴突的识别和髓鞘形成是可分离的过程。

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