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纯化的天然微管相关蛋白MAP1A:微管组装动力学及MAP1A/微管蛋白化学计量比

Purified native microtubule associated protein MAP1A: kinetics of microtubule assembly and MAP1A/tubulin stoichiometry.

作者信息

Pedrotti B, Islam K

机构信息

Department of Biology, University of Milan, Italy.

出版信息

Biochemistry. 1994 Oct 18;33(41):12463-70. doi: 10.1021/bi00207a013.

Abstract

In a recent study, we have shown that sulfonate buffers affect microtubule assembly and alter microtubule protein composition (Pedrotti et al., 1993). In particular, we noted that PIPES buffer leads to removal of MAP1 from the microtubule surface without affecting the association of MAP2 with microtubules. This observation has been exploited to develop a simple purification procedure for MAP1A using twice-cycled microtubule protein prepared from whole bovine brain. A single chromatographic step on an ion-exchange column results in > 90% pure MAP1A. Using purified MAP1A, we now show that MAP1A (a) binds in a dose-dependent manner to unpolymerized tubulin and assembled microtubules, (b) binds 13-15 mol of tubulin dimers in assembled microtubules, (c) promotes both nucleation and elongation of tubulin, and (d) promotes incorporation of tubulin dimers at low GTP concentrations and of tubulin dimers and oligomers at high GTP concentrations. MAP1A lowers the critical concentration for assembly, and MAP1A-promoted incorporation of dimers has an association rate constant (K+1) of 39.3 x 10(6) M-1s-1 and a dissociation rate constant (K-1) of 15 s-1; both constants are about 2-3-fold higher compared with MAP2.

摘要

在最近的一项研究中,我们已经表明磺酸盐缓冲液会影响微管组装并改变微管蛋白组成(佩德罗蒂等人,1993年)。特别地,我们注意到PIPES缓冲液会导致微管相关蛋白1(MAP1)从微管表面去除,而不影响微管相关蛋白2(MAP2)与微管的结合。这一观察结果已被用于开发一种简单的纯化程序,用于从全牛脑中制备的经过两次循环的微管蛋白来纯化微管相关蛋白1A(MAP1A)。在离子交换柱上进行单一色谱步骤可得到纯度大于90%的MAP1A。使用纯化的MAP1A,我们现在表明MAP1A:(a)以剂量依赖的方式与未聚合的微管蛋白和组装好的微管结合;(b)在组装好的微管中结合13 - 15摩尔的微管蛋白二聚体;(c)促进微管蛋白的成核和延长;(d)在低鸟苷三磷酸(GTP)浓度下促进微管蛋白二聚体的掺入,在高GTP浓度下促进微管蛋白二聚体和寡聚体的掺入。MAP1A降低了组装的临界浓度,并且MAP1A促进的二聚体掺入的缔合速率常数(K+1)为39.3×10⁶ M⁻¹s⁻¹,解离速率常数(K-1)为15 s⁻¹;与MAP2相比,这两个常数都高出约2 - 3倍。

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