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血影蛋白与脑微管的关联。

Association of fodrin with brain microtubules.

作者信息

Fach B L, Graham S F, Keates R A

出版信息

Can J Biochem Cell Biol. 1985 May;63(5):372-81. doi: 10.1139/o85-054.

Abstract

We have compared the polypeptide composition of microtubules isolated from bovine brain by the conventional in vitro reassembly method with those obtained by direct isolation of brain microtubules into a stabilizing buffer. The stabilizing buffer included 6.7 M glycerol to limit the rate of subunit exchange between assembled and unassembled states. The microtubule-associated proteins normally found by in vitro reassembly are also found in the stabilized preparation, but in smaller proportions. Fodrin, a brain membrane-associated protein believed to be homologous to spectrin, was found to be the most abundant component after tubulin in the stabilized microtubules. The ratio of tubulin to fodrin, 16:1 by mass, was almost constant at each stage of the preparation. Some actin was initially present in the stabilized microtubules, but was gradually lost during purification. When stabilized microtubules were diluted into cold aqueous buffer, they depolymerized and the recovered microtubule protein could then be purified by in vitro reassembly. The composition after this treatment resembled that of microtubules prepared initially by reassembly in vitro. The missing fodrin was found to be removed in the preliminary centrifugation and was unavailable for incorporation into growing microtubules during the in vitro assembly step. This suggests that the standard in vitro reassembly procedure for purification of microtubules may distort the composition of microtubule-associated proteins.

摘要

我们已将通过传统体外重装配方法从牛脑中分离得到的微管的多肽组成,与通过将脑微管直接分离到稳定缓冲液中得到的微管的多肽组成进行了比较。该稳定缓冲液包含6.7 M甘油,以限制组装态和未组装态之间亚基交换的速率。通常通过体外重装配发现的微管相关蛋白在稳定制剂中也能找到,但比例较小。血影蛋白是一种与脑细胞膜相关的蛋白,被认为与血影蛋白同源,它是稳定微管中仅次于微管蛋白的最丰富成分。微管蛋白与血影蛋白的质量比为16:1,在制备的每个阶段几乎恒定。一些肌动蛋白最初存在于稳定的微管中,但在纯化过程中逐渐丢失。当将稳定的微管稀释到冰冷的水性缓冲液中时,它们会解聚,然后回收的微管蛋白可通过体外重装配进行纯化。这种处理后的组成类似于最初通过体外重装配制备的微管的组成。发现缺失的血影蛋白在初步离心过程中被去除,并且在体外组装步骤中无法掺入生长的微管中。这表明用于纯化微管的标准体外重装配程序可能会扭曲微管相关蛋白的组成。

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