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从牛脑中分离出具有微管播种活性的超稳定微管子群体。

Isolation from bovine brain of a superstable microtubule subpopulation with microtubule seeding activity.

作者信息

Job D, Margolis R L

出版信息

Biochemistry. 1984 Jun 19;23(13):3025-31. doi: 10.1021/bi00308a028.

DOI:10.1021/bi00308a028
PMID:6466629
Abstract

Cold-stable microtubule protein isolated from beef brain is capable of seeding microtubule assembly under conditions that prevent the initiation of self-assembly of cold-labile microtubules. We have developed a quantitative assay for the determination of seeding activity. Using this assay, we find that seeding activity is apparently due to microtubule fragments that resist -80 degrees C, a condition that causes the depolymerization of cold-stable microtubules ("cold stability" is defined as resistance to 0 degree C disassembly), but rapidly depolymerize when exposed to 3.0 mM free calcium, to micromolar Ca2+-calmodulin, or to 0.2 M NaCl at 4 degrees C. After salt treatment, seeding activity is permanently lost although microtubule cold stability is retained through further assembly cycles. Similarly, after sedimentation of microtubule seeds the supernatant protein assembles into cold-stable microtubules, which are permanently devoid of seeding activity. By contrast, seeding activity can be recovered by recycling of supernatant protein from preparations exposed to 3.0 mM calcium or to Ca2+-calmodulin prior to centrifugation, indicating the solubilization of an active component (designated "preseeds") under these conditions. Polyacrylamide gels show some differences in polypeptides between seeding and non-seeding cold-stable microtubule preparations. Approximately 35% of the microtubule population assembled from beef brain crude extract is cold stable, while approximately 2% constitutes -80 degrees C resistant seeds. The formation of seeds from seed-forming subunits (preseeds) occurs rapidly, is apparently a cooperative phenomenon, and occurs on preexisting microtubules under either assembly initiating or steady-state conditions.

摘要

从牛脑中分离出的冷稳定微管蛋白能够在阻止冷不稳定微管自我组装起始的条件下引发微管组装。我们开发了一种用于测定引发活性的定量分析方法。使用该分析方法,我们发现引发活性显然归因于能抵抗 -80℃的微管片段,这种条件会导致冷稳定微管解聚(“冷稳定性”定义为对0℃解聚的抗性),但当暴露于3.0 mM游离钙、微摩尔浓度的Ca2 + -钙调蛋白或4℃下的0.2 M NaCl时会迅速解聚。盐处理后,尽管通过进一步的组装循环微管冷稳定性得以保留,但引发活性会永久丧失。同样,微管种子沉降后,上清液中的蛋白质组装成冷稳定微管,这些微管永久失去引发活性。相比之下,通过在离心前回收暴露于3.0 mM钙或Ca2 + -钙调蛋白的制剂中的上清液蛋白质,可以恢复引发活性,这表明在这些条件下一种活性成分(称为“前体种子”)被溶解。聚丙烯酰胺凝胶显示,引发和非引发的冷稳定微管制剂之间的多肽存在一些差异。从牛脑粗提物组装的微管群体中约35%是冷稳定的,而约2%构成抗 -80℃的种子。由种子形成亚基(前体种子)形成种子的过程迅速,显然是一种协同现象,并且在组装起始或稳态条件下在预先存在的微管上发生。

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