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非洲爪蟾卵母细胞和卵的细胞质提取物中的微管组装

Microtubule assembly in cytoplasmic extracts of Xenopus oocytes and eggs.

作者信息

Gard D L, Kirschner M W

机构信息

Department of Biochemistry and Biophysics, University of California, San Francisco School of Medicine 94143.

出版信息

J Cell Biol. 1987 Nov;105(5):2191-201. doi: 10.1083/jcb.105.5.2191.

Abstract

We have investigated the differences in microtubule assembly in cytoplasm from Xenopus oocytes and eggs in vitro. Extracts of activated eggs could be prepared that assembled extensive microtubule networks in vitro using Tetrahymena axonemes or mammalian centrosomes as nucleation centers. Assembly occurred predominantly from the plus-end of the microtubule with a rate constant of 2 microns.min-1.microM-1 (57 s-1.microM-1). At the in vivo tubulin concentration, this corresponds to the extraordinarily high rate of 40-50 microns.min-1. Microtubule disassembly rates in these extracts were -4.5 microns.min-1 (128 s-1) at the plus-end and -6.9 microns.min-1 (196 s-1) at the minus-end. The critical concentration for plus-end microtubule assembly was 0.4 microM. These extracts also promoted the plus-end assembly of microtubules from bovine brain tubulin, suggesting the presence of an assembly promoting factor in the egg. In contrast to activated eggs, assembly was never observed in extracts prepared from oocytes, even at tubulin concentrations as high as 20 microM. Addition of oocyte extract to egg extracts or to purified brain tubulin inhibited microtubule assembly. These results suggest that there is a plus-end-specific inhibitor of microtubule assembly in the oocyte and a plus-end-specific promoter of assembly in the eggs. These factors may serve to regulate microtubule assembly during early development in Xenopus.

摘要

我们研究了非洲爪蟾卵母细胞和卵子细胞质中微管体外组装的差异。可以制备活化卵子的提取物,这些提取物在体外使用四膜虫轴丝或哺乳动物中心体作为成核中心组装广泛的微管网络。组装主要从微管的正端发生,速率常数为2微米·分钟⁻¹·微摩尔⁻¹(57秒⁻¹·微摩尔⁻¹)。在体内微管蛋白浓度下,这相当于40 - 50微米·分钟⁻¹的极高速率。这些提取物中微管的解聚速率在正端为-4.5微米·分钟⁻¹(128秒⁻¹),在负端为-6.9微米·分钟⁻¹(196秒⁻¹)。正端微管组装的临界浓度为0.4微摩尔。这些提取物还促进了来自牛脑微管蛋白的微管正端组装,表明卵子中存在一种组装促进因子。与活化卵子相反,即使在微管蛋白浓度高达20微摩尔时,从卵母细胞制备的提取物中也从未观察到组装。将卵母细胞提取物添加到卵子提取物或纯化的脑微管蛋白中会抑制微管组装。这些结果表明,卵母细胞中存在微管组装的正端特异性抑制剂,而卵子中存在正端特异性组装促进剂。这些因子可能在非洲爪蟾早期发育过程中调节微管组装。

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