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在小鼠神经元分化过程中,微管锚定蛋白 ninein 从中心体向树突重新定位。

Relocalization of a microtubule-anchoring protein, ninein, from the centrosome to dendrites during differentiation of mouse neurons.

机构信息

Department of Materials and Life Sciences, Faculty of Science and Technology, Sophia University, 7-1 Kioicho, Chiyoda-ku, Tokyo, 102-8554, Japan.

出版信息

Histochem Cell Biol. 2009 Nov;132(5):515-24. doi: 10.1007/s00418-009-0631-z. Epub 2009 Aug 19.

DOI:10.1007/s00418-009-0631-z
PMID:19690882
Abstract

Microtubules in typical cells form radial arrays with their plus-ends pointing toward the cell periphery. In contrast, microtubules in dendrites of neurons are free from centrosomes and have a unique arrangement in which about half have a polarity with a minus-end distal orientation. Mechanisms for generation and maintenance of the microtubule arrangement in dendrites are not well understood. Here, we examined dendritic localization of a centrosomal protein, ninein, which has microtubule-anchoring and stabilizing functions. Immunohistochemical analysis of developing mouse cerebral and cerebellar cortices showed that ninein is localized at the centrosome in undifferentiated neural precursors. In contrast, ninein was barely detected in migrating neurons, such as those in the intermediate layer of the cerebral cortex and the internal granular layer of the cerebellar cortex. High expression was observed in thick dendrite-bearing neurons such as pyramidal neurons of the cerebral cortex and Purkinje neurons in the cerebellar cortex. Ninein was not detected at the centrosome of these cells, but was diffusely present in cell soma and dendrites. In cultured cortical neurons, ninein formed granular structures in soma and dendrites, being not associated with gamma-tubulin. About 60% of these structures showed resistance to detergent and association with microtubules. Our observations suggest that the minus-ends of microtubules may be anchored and stabilized by centrosomal proteins localized in dendrites.

摘要

典型细胞中的微管形成放射状排列,其正极指向细胞外周。相比之下,神经元树突中的微管没有中心体,排列独特,大约有一半具有远端负极端的极性。树突中微管排列的产生和维持机制尚不清楚。在这里,我们研究了中心体蛋白 ninein 的树突定位,它具有微管锚定和稳定功能。对发育中的小鼠大脑和小脑皮质的免疫组织化学分析表明,ninein 位于未分化神经前体细胞的中心体中。相比之下,在迁移神经元中几乎检测不到 ninein,如大脑皮质的中间层和小脑皮质的内颗粒层中的神经元。在具有厚树突的神经元中表达量较高,如大脑皮质的锥体细胞和小脑皮质的浦肯野神经元。在这些细胞的中心体中未检测到 ninein,但在细胞体和树突中广泛存在。在培养的皮质神经元中,ninein 在细胞体和树突中形成颗粒状结构,与γ微管蛋白无关。这些结构中约有 60%对去污剂有抗性,并与微管结合。我们的观察表明,微管的负端可能被定位在树突中的中心体蛋白锚定和稳定。

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