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伴随张力诱导的神经突起始的微管组装和组织研究。

Investigation of microtubule assembly and organization accompanying tension-induced neurite initiation.

作者信息

Zheng J, Buxbaum R E, Heidemann S R

机构信息

Department of Physiology, Michigan State University, East Lansing 48824-1101.

出版信息

J Cell Sci. 1993 Apr;104 ( Pt 4):1239-50. doi: 10.1242/jcs.104.4.1239.

DOI:10.1242/jcs.104.4.1239
PMID:8314903
Abstract

Pulling on the margin of embryonic chick sensory neurons induces neurite formation de novo. We find that these neurites contain microtubules within minutes after the application of tension and apparently normal microtubule arrays within 10-20 min. We wished to determine whether these microtubules reflected existing microtubules that were reorganized, e.g. pulled into the neurite by the applied forces, or whether they reflected primarily new assembly of tubulin. We investigated tension-induced neurite initiation in the presence of 4 nM vinblastine, a concentration that poisons net microtubule assembly but does not depolymerize extant polymers, thus separating new assembly from movements of existing microtubules. We find that vinblastine seriously compromises the ability of chick sensory neurons to initiate neurites in response to tension. The few poisoned neurites that did form were abnormal in several respects. In contrast to unpoisoned cells, poisoned neurites were prone to stretching and breaking while pulling, as though they lacked normal structural support. Indeed, poisoned neurites possessed only short microtubule fragments. We conclude that the microtubule array seen in tension-induced neurites reflects primarily new microtubule assembly, rather than existing microtubules that were reorganized to invade the neurite. This implies that tension applied to unpoisoned chick sensory neurons rapidly stimulates new microtubule assembly concomitant with neurite initiation. Examination of the tension-induced microtubules shows that both their spatial pattern and their acetylation are similar to that reported for normal growth cone-mediated neurites.

摘要

牵拉鸡胚感觉神经元的边缘会诱导神经突从头形成。我们发现,在施加张力后的几分钟内,这些神经突中就含有微管,在10 - 20分钟内含有明显正常的微管阵列。我们希望确定这些微管是反映了现有的、被重新组织(例如被施加的力拉入神经突)的微管,还是主要反映了微管蛋白的新组装。我们在存在4 nM长春花碱的情况下研究了张力诱导的神经突起始,该浓度会毒害微管的净组装,但不会使现存的聚合物解聚,从而将新组装与现有微管的运动区分开来。我们发现长春花碱严重损害了鸡胚感觉神经元响应张力起始神经突的能力。少数形成的中毒神经突在几个方面都不正常。与未中毒的细胞相比,中毒的神经突在牵拉时容易伸展和断裂,就好像它们缺乏正常的结构支撑。实际上,中毒的神经突只含有短的微管片段。我们得出结论,在张力诱导的神经突中看到的微管阵列主要反映了新的微管组装,而不是被重新组织以侵入神经突的现有微管。这意味着施加到未中毒的鸡胚感觉神经元上的张力会迅速刺激新的微管组装并伴随着神经突起始。对张力诱导的微管的检查表明,它们的空间模式和乙酰化与正常生长锥介导的神经突所报道的相似。

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