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体外神经胶质细胞引导的颗粒神经元迁移:一项高分辨率延时视频显微镜研究。

Glial-guided granule neuron migration in vitro: a high-resolution time-lapse video microscopic study.

作者信息

Edmondson J C, Hatten M E

出版信息

J Neurosci. 1987 Jun;7(6):1928-34. doi: 10.1523/JNEUROSCI.07-06-01928.1987.

DOI:10.1523/JNEUROSCI.07-06-01928.1987
PMID:3598656
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6568879/
Abstract

To study neuronal migration, migrating granule neurons in microcultures prepared from early postnatal cerebellum have been analyzed with time-lapse, video-enhanced differential interference contrast microscopy. The morphology of migrating neurons resembles the elongated forms of migrating neurons described both in vivo and in vitro (Rakic, 1971; Hatten et al., 1984). The neuron closely apposes its soma along the glial fiber and extends a thickened leading process in the direction of migration. This leading tip is highly motile, with several filopodial extensions. Intracellular vesicular structures extend from the nucleus into the leading process of migrating neurons in vitro. Quantitation of the motions of migrating neurons revealed a saltatory pattern of advance along the glial fiber. Periods of cell soma movement at the rate of 56 +/- 26 micron/hr along the glial fiber are punctuated by periods during which the cell soma slows to a complete stop. The overall rate of migration is 33 +/- 20 micron/hr. The growing tip of the leading process rapidly extends and retracts, resulting in a net advance along the glial fiber. However, the periods of the extension and retraction of the leading process growing tip are not synchronized with the motions of the cell soma.

摘要

为了研究神经元迁移,利用延时、视频增强微分干涉相差显微镜对出生后早期小脑制备的微培养物中迁移的颗粒神经元进行了分析。迁移神经元的形态类似于体内和体外描述的迁移神经元的细长形态(拉基奇,1971年;哈滕等人,1984年)。神经元的胞体沿着胶质纤维紧密贴附,并在迁移方向上延伸出一个增厚的前端突起。这个前端非常活跃,有几个丝状伪足延伸。在体外,细胞内囊泡结构从细胞核延伸到迁移神经元的前端突起。对迁移神经元运动的定量分析揭示了沿着胶质纤维的跳跃式前进模式。细胞胞体以56±26微米/小时的速度沿着胶质纤维移动的时期,被细胞胞体减慢至完全停止的时期所打断。总体迁移速度为33±20微米/小时。前端突起的生长尖端迅速伸展和回缩,导致沿着胶质纤维的净前进。然而,前端突起生长尖端的伸展和回缩时期与细胞胞体的运动并不同步。