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少突胶质前体细胞群(由NG2标记定义)对成年脊髓脱髓鞘的反应。

Response of the oligodendrocyte progenitor cell population (defined by NG2 labelling) to demyelination of the adult spinal cord.

作者信息

Keirstead H S, Levine J M, Blakemore W F

机构信息

MRC Cambridge Centre for Brain Repair, and Department of Clinical Veterinary Medicine, University of Cambridge, United Kingdom.

出版信息

Glia. 1998 Feb;22(2):161-70.

PMID:9537836
Abstract

Elucidation of the response of oligodendrocyte progenitor cell populations to demyelination in the adult central nervous system (CNS) is critical to understanding why remyelination fails in multiple sclerosis. Using the anti-NG2 monoclonal antibody to identify oligodendrocyte progenitor cells, we have documented their response to antibody-induced demyelination in the dorsal column of the adult rat spinal cord. The number of NG2+ cells in the vicinity of demyelinated lesions increased by 72% over the course of 3 days following the onset of demyelination. This increase in NG2+ cell numbers did not reflect a nonspecific staining of reactive cells, as GFAP, OX-42, and Rip antibodies did not co-localise with NG2 + cells in double immunostained tissue sections. NG2 + cells incorporated BrdU 48-72 h following the onset of demyelination. After the onset of remyelination (10-14 days), the number of NG2+ cells decreased to 46% of control levels and remained consistently low for 2 months. When spinal cords were exposed to 40 Grays of x-irradiation prior to demyelination, the number of NG2+ cells decreased to 48% of control levels by 3 days following the onset of demyelination and remained unchanged at 3 weeks. Since 40 Grays of x-irradiation kills dividing cells, these studies illustrate a responsive and nonresponsive NG2+ cell population following demyelination in the adult spinal cord and suggest that the responsive NG2+ cell population does not renew itself.

摘要

阐明少突胶质前体细胞群对成体中枢神经系统(CNS)脱髓鞘的反应,对于理解多发性硬化症中髓鞘再生失败的原因至关重要。我们使用抗NG2单克隆抗体来识别少突胶质前体细胞,记录了它们对成年大鼠脊髓背柱中抗体诱导的脱髓鞘的反应。脱髓鞘开始后的3天内,脱髓鞘病变附近的NG2+细胞数量增加了72%。NG2+细胞数量的增加并非反映反应性细胞的非特异性染色,因为在双重免疫染色的组织切片中,GFAP、OX-42和Rip抗体与NG2+细胞不共定位。脱髓鞘开始后48 - 72小时,NG2+细胞掺入了BrdU。髓鞘再生开始后(10 - 14天),NG2+细胞数量降至对照水平的46%,并在2个月内持续保持低水平。在脱髓鞘之前,当脊髓接受40格雷的x射线照射时,脱髓鞘开始后3天,NG2+细胞数量降至对照水平的48%,并在3周时保持不变。由于40格雷的x射线照射会杀死分裂细胞,这些研究表明成年脊髓脱髓鞘后存在反应性和无反应性的NG2+细胞群,并提示反应性NG2+细胞群不能自我更新。

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