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大鼠神经元中免疫特性不同的驱动蛋白重链的轴突运输与分布

Axonal transport and distribution of immunologically distinct kinesin heavy chains in rat neurons.

作者信息

Li J Y, Pfister K K, Brady S, Dahlström A

机构信息

Department of Anatomy and Cell Biology, Göteborg University, Göteborg, Sweden.

出版信息

J Neurosci Res. 1999 Oct 15;58(2):226-41.

PMID:10502279
Abstract

The functional significance of biochemical and immunochemical heterogeneity in neuronal kinesin remains uncertain. Confocal laser scanning microscopy, cytofluorimetric scanning, and immunoblots were used for quantitative analyses of axonal transport and cellular distribution of immunochemically distinct kinesin heavy chain isoforms (H1 and H2) in rat peripheral nerve and spinal cord. H1 and H2 immunoreactivities (IR) were observed in axons proximal to a crush as early as 1 hr after the crush operation and increased linearly with time, consistent with fast axonal transport of both. Only approximately 10% of the proximal accumulations of H1-IR and H2-IR accumulated distal to the crush, in contrast to synaptophysin-IR (approximately 70%). H2-IR was widely present in peripheral nervous system and virtually colocalized with synaptic vesicle proteins synaptophysin, synaptobrevin I, and SNAP-25 and two neuropeptides [calcitonin gene-related peptide (CGRP) and substance P (SP)], although H2-IR was weaker in spinal cord terminals. In contrast, H1-IR appeared preferentially enriched in large axons, probably motor and large sensory neurons, which contained synaptophysin-IR, synaptobrevin I-IR, SNAP-25-IR, and CGRP-IR. However, H1-IR was weak or absent from SP-containing thin and medium-sized axons. In addition, H1-IR appeared to be absent from spinal cord nerve terminals. H1- and H2-IR kinesins are both transported with fast axonal transport, and comparatively small amounts of kinesins are retrogradely transported. H2 was widely distributed in motor, sensory, and sympathetic neurons, whereas H1 was enriched in large motor and sensory neurons.

摘要

神经元驱动蛋白中生化和免疫化学异质性的功能意义仍不确定。共聚焦激光扫描显微镜、细胞荧光扫描和免疫印迹法用于定量分析大鼠外周神经和脊髓中免疫化学上不同的驱动蛋白重链亚型(H1和H2)的轴突运输和细胞分布。早在挤压手术后1小时,就在挤压近端的轴突中观察到H1和H2免疫反应性(IR),并且随时间呈线性增加,这与两者的快速轴突运输一致。与突触素-IR(约70%)相比,只有约10%的H1-IR和H2-IR近端积累物在挤压远端积累。H2-IR广泛存在于外周神经系统中,实际上与突触小泡蛋白突触素、突触结合蛋白I和SNAP-25以及两种神经肽[降钙素基因相关肽(CGRP)和P物质(SP)]共定位,尽管H2-IR在脊髓终末中较弱。相比之下,H1-IR似乎优先富集于大轴突中,可能是运动神经元和大感觉神经元,这些神经元含有突触素-IR、突触结合蛋白I-IR、SNAP-25-IR和CGRP-IR。然而,含SP的细和中等大小轴突中H1-IR较弱或缺失。此外,脊髓神经终末似乎不存在H1-IR。H1-IR和H2-IR驱动蛋白均通过快速轴突运输进行运输,且相对少量的驱动蛋白进行逆行运输。H2广泛分布于运动、感觉和交感神经元中,而H1富集于大运动和感觉神经元中。

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