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电离辐射损伤后室管膜下再填充的长期损害。

Long-term impairment of subependymal repopulation following damage by ionizing irradiation.

作者信息

Tada E, Yang C, Gobbel G T, Lamborn K R, Fike J R

机构信息

Department of Neurological Surgery, School of Medicine, University of California, San Francisco 94143-0520, USA.

出版信息

Exp Neurol. 1999 Nov;160(1):66-77. doi: 10.1006/exnr.1999.7172.

Abstract

In the mammalian brain, the subependyma (SE) contains stem cells capable of producing neurons and glia. In normal brain these stem cells are responsible, in part, for maintaining the morphologic and functional integrity of the SE; what role the cells of the SE play in brain injury has not yet been elucidated. The present study was designed to determine the long-term regenerative potential of the rat SE after significant depletion of stem cells. Ionizing irradiation was used to deplete cells of the SE and subsequent cellular responses were quantified using immunohistochemical analyses on formalin-fixed, paraffin-embedded tissues. A histomorphometric approach was used to quantify total cell number, number of proliferating cells, number of immature neurons, astrocytes, and undifferentiated components of the SE. Because there are no markers specific for stem cells, we used a repopulation assay as an indirect measure of stem cell response after injury. Our data showed clear radiation dose-dependencies in our quantitative endpoints, implying that there was progressively more stem cell damage with increasing radiation dose. Repopulation of the SE in terms of total cell number, number of proliferating cells and numbers of immature neurons was impaired in a dose-dependent fashion up to 180 days after treatment. These data suggest that after irradiation, surviving stem cells are unable to regenerate the SE. This inability to regenerate after stem cell damage/depletion could have important implications with respect to the normal function of the SE and the function of the SE after brain injury.

摘要

在哺乳动物大脑中,室管膜下区(SE)含有能够产生神经元和神经胶质细胞的干细胞。在正常大脑中,这些干细胞部分负责维持SE的形态和功能完整性;然而,SE细胞在脑损伤中所起的作用尚未阐明。本研究旨在确定大鼠SE在干细胞大量耗竭后的长期再生潜力。采用电离辐射来耗尽SE细胞,并使用免疫组织化学分析对福尔马林固定、石蜡包埋的组织进行后续细胞反应的定量分析。采用组织形态计量学方法来量化SE的总细胞数、增殖细胞数、未成熟神经元数、星形胶质细胞数以及未分化成分。由于没有针对干细胞的特异性标志物,我们使用再增殖试验作为损伤后干细胞反应的间接测量方法。我们的数据在定量终点显示出明显的辐射剂量依赖性,这意味着随着辐射剂量的增加,干细胞损伤逐渐加重。在治疗后的180天内,SE在总细胞数、增殖细胞数和未成熟神经元数方面的再增殖以剂量依赖的方式受到损害。这些数据表明,照射后存活的干细胞无法使SE再生。干细胞损伤/耗竭后无法再生可能对SE的正常功能以及脑损伤后SE的功能具有重要意义。

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