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同型纯微管蛋白二聚体微管组装的体外分析。在缺乏微管相关蛋白的情况下,αβII、αβIII和αβIV微管蛋白二聚体组装特性的内在差异。

In vitro analysis of microtubule assembly of isotypically pure tubulin dimers. Intrinsic differences in the assembly properties of alpha beta II, alpha beta III, and alpha beta IV tubulin dimers in the absence of microtubule-associated proteins.

作者信息

Lu Q, Luduena R F

机构信息

Department of Biochemistry, University of Texas Health Science Center, San Antonio 78284-7760.

出版信息

J Biol Chem. 1994 Jan 21;269(3):2041-7.

PMID:8294455
Abstract

Microtubule assembly of different beta tubulin isotypes in the presence of 4 M glycerol and 6 mM magnesium ion demonstrates significantly different characteristics. alpha beta II and alpha beta IV assembled faster and to a greater extent than did unfractionated phosphocellulose-purified tubulin (PC-tubulin). Microtubule assembly from alpha beta III showed a distinctive delay in nucleation, proceeded at a slower rate than those of the other beta tubulin isotypes, and had the highest critical concentration. However, treatment of beta tubulin isotypes with subtilisin to remove the C-terminal domain of the tubulin dimer abolished these differences in microtubule assembly pattern and enhanced self-assembly. The kinetic analysis of microtubule elongation of different beta tubulin isotypes also showed significant differences. Elongation of alpha beta III from microtubule seeds had a lower apparent K alpha and a lower apparent Kd than did alpha beta II and alpha beta IV. The dynamic behaviors of different beta tubulin isotypes were qualitatively similar to each other and fit the dynamic instability model. However, microtubules formed from alpha beta III appeared to be less dynamic than microtubules formed from other beta tubulin isotypes. Our results suggest that the beta III isotype might have a different conformation than do the other beta tubulin isotypes. The distinctive nucleation and elongation behaviors of the alpha beta III dimers demonstrated in vitro may have a significant influence on microtubule functions in vivo.

摘要

在存在4M甘油和6mM镁离子的情况下,不同β微管蛋白同种型的微管组装表现出显著不同的特征。αβII和αβIV的组装速度更快,程度也比未分级的磷酸纤维素纯化微管蛋白(PC-微管蛋白)更高。来自αβIII的微管组装在成核过程中表现出明显的延迟,其组装速度比其他β微管蛋白同种型慢,并且具有最高的临界浓度。然而,用枯草杆菌蛋白酶处理β微管蛋白同种型以去除微管蛋白二聚体的C末端结构域,消除了微管组装模式上的这些差异并增强了自组装。不同β微管蛋白同种型的微管伸长动力学分析也显示出显著差异。与αβII和αβIV相比,由微管种子产生的αβIII的伸长具有更低的表观Kα和更低的表观Kd。不同β微管蛋白同种型的动态行为在定性上彼此相似,并且符合动态不稳定性模型。然而,由αβIII形成的微管似乎比由其他β微管蛋白同种型形成的微管动态性更低。我们的结果表明,βIII同种型可能具有与其他β微管蛋白同种型不同的构象。体外显示的αβIII二聚体独特的成核和伸长行为可能对体内微管功能有重大影响。

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