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金鱼视觉通路中视网膜轴突退变和再生过程中少突胶质细胞的命运

Fate of oligodendrocytes during retinal axon degeneration and regeneration in the goldfish visual pathway.

作者信息

Ankerhold R, Stuermer C A

机构信息

Carl Zeiss Jena, Tatzendpromenade 1a, 07745 Jena, Germany.

出版信息

J Neurobiol. 1999 Dec;41(4):572-84.

PMID:10590180
Abstract

Retinal axons in goldfish regenerate after optic nerve lesion, restore synaptic connections, and become myelinated by oligodendrocytes. The fate of oligodendrocytes during these events is not known and may require generation of new oligodendrocytes or dedifferentiation and redifferentiation of the existing ones. To determine the reaction of oligodendrocytes to optic nerve lesion, we used the terminal transferase technique to detect apoptosis, bromodeoxyuridine incorporation to reveal mitosis, antibodies to identify myelin and oligodendrocytes, and Lucifer yellow injections to reveal cell morphology. Along with the reappearance of the myelin molecules 36K protein, galactocerebroside, and myelin basic protein, myelinating oligodendrocytes (identified by Lucifer yellow injections) reappear 21 days postlesion. Prior to this time, the dye-filled cells had few processes oriented along the regenerating axons. They resembled oligodendrocytes seen both in vitro and in vivo which express the L1-related E587 antigen and synthesize the 36K myelin protein in coculture with axons. No signs of oligodendrocyte apoptosis were detected after lesion and only few of the oligodendrocytes present had recently arisen. 36K/E587 double-labeled oligodendrocytes which were most likely dedifferentiating oligodendrocytes were identified in 8-day postlesion nerves among E587-positive elongate cells whose numbers increased until 14 days postlesion. These findings suggest that oligodendrocytes dedifferentiate-like Schwann cells-from cells which express myelin molecules to elongate cells which express the L1/E587 antigen. They redifferentiate to myelinate axons from roughly 3 weeks onward. These findings suggest an adaptive plasticity of goldfish oligodendrocytes beneficial to the repair of the visual pathway.

摘要

金鱼视网膜轴突在视神经损伤后会再生,恢复突触连接,并被少突胶质细胞髓鞘化。在这些过程中少突胶质细胞的命运尚不清楚,可能需要产生新的少突胶质细胞,或者使现有的少突胶质细胞去分化并重新分化。为了确定少突胶质细胞对视神经损伤的反应,我们使用末端转移酶技术检测细胞凋亡,用溴脱氧尿苷掺入法揭示有丝分裂,用抗体鉴定髓磷脂和少突胶质细胞,并用荧光黄注射来显示细胞形态。随着髓磷脂分子36K蛋白、半乳糖脑苷脂和髓磷脂碱性蛋白的重新出现,损伤后21天出现了髓鞘化的少突胶质细胞(通过荧光黄注射鉴定)。在此之前,充满染料的细胞沿再生轴突排列的突起很少。它们类似于在体外和体内看到的少突胶质细胞,这些少突胶质细胞在与轴突共培养时表达与L1相关的E587抗原并合成36K髓磷脂蛋白。损伤后未检测到少突胶质细胞凋亡的迹象,并且只有少数现存的少突胶质细胞是最近产生的。在损伤后8天的神经中,在E587阳性的细长细胞中鉴定出最有可能正在去分化的36K/E587双标记少突胶质细胞,其数量一直增加到损伤后14天。这些发现表明,少突胶质细胞会像施万细胞一样去分化,从表达髓磷脂分子的细胞转变为表达L1/E587抗原的细长细胞。从大约3周开始,它们会重新分化以髓鞘化轴突。这些发现表明金鱼少突胶质细胞具有适应性可塑性,有利于视觉通路的修复。

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Fate of oligodendrocytes during retinal axon degeneration and regeneration in the goldfish visual pathway.金鱼视觉通路中视网膜轴突退变和再生过程中少突胶质细胞的命运
J Neurobiol. 1999 Dec;41(4):572-84.
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E587 antigen is upregulated by goldfish oligodendrocytes after optic nerve lesion and supports retinal axon regeneration.E587抗原在视神经损伤后被金鱼少突胶质细胞上调,并支持视网膜轴突再生。
Glia. 1998 Jul;23(3):257-70.
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Fish optic nerve oligodendrocytes support axonal regeneration of fish and mammalian retinal ganglion cells.鱼类视神经少突胶质细胞支持鱼类和哺乳动物视网膜神经节细胞的轴突再生。
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Growth cones of regenerating retinal axons contact a variety of cellular profiles in the transected goldfish optic nerve.再生视网膜轴突的生长锥与横断的金鱼视神经中的多种细胞形态接触。
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Growth of regenerating goldfish axons is inhibited by rat oligodendrocytes and CNS myelin but not but not by goldfish optic nerve tract oligodendrocytelike cells and fish CNS myelin.再生金鱼轴突的生长受到大鼠少突胶质细胞和中枢神经系统髓磷脂的抑制,但不受金鱼视神经束少突胶质细胞样细胞和鱼类中枢神经系统髓磷脂的抑制。
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Similarities and differences between fish oligodendrocytes and Schwann cells in vitro.鱼类少突胶质细胞与雪旺细胞在体外的异同
Glia. 1994 Aug;11(4):300-14. doi: 10.1002/glia.440110403.
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Trying to understand axonal regeneration in the CNS of fish.试图了解鱼类中枢神经系统中的轴突再生。
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Axonal regrowth in the amyelinated optic nerve of the myelin-deficient rat: ultrastructural observations and effects of ganglioside administration.髓磷脂缺乏大鼠无髓鞘视神经中的轴突再生:超微结构观察及神经节苷脂给药的影响
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Robust regeneration of CNS axons through a track depleted of CNS glia.中枢神经系统轴突通过缺乏中枢神经系统胶质细胞的通道实现强劲再生。
Exp Neurol. 2000 Jan;161(1):49-66. doi: 10.1006/exnr.1999.7230.

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