We describe the interaction of pure brain tubulin with purified membranes specialized in different cell functions, i.e., plasma membranes and mitochondrial membranes from liver and secretory granule membranes from adrenal medulla. We studied the tubulin-binding activity of cellular membranes using a radiolabeled ligand-receptor assay and an antibody retention assay. The tubulin-membrane interaction was time- and temperature-dependent, reversible, specific, and saturable. The binding of tubulin to membranes appears to be specific since acidic proteins such as serum albumin or actin did not interfere in the binding process. The apparent overall affinity constant of the tubulin- membrane interaction ranged between 1.5 and 3.0 X 10(7) M-1; similar values were obtained for the three types of membranes. Tubulin bound to membranes was not entrapped into vesicles since it reacted quantitatively with antitubulin antibodies. At saturation of the tubulin-binding sites, the amount of reversibly bound tubulin represents 5-10% by weight of membrane protein (0.4-0.9 nmol tubulin/mg membrane protein). The high tubulin-binding capacity of membranes seems to be inconsistent with a 1:1 stoichiometry between tubulin and a membrane component but could be relevant to a kind of tubulin assembly. Indeed, tubulin-membrane interaction had some properties in common with microtubule formation: (a) the association of tubulin to membranes increased with the temperature, whereas the dissociation of tubulin- membrane complexes increased by decreasing temperature; (b) the binding of tubulin to membranes was prevented by phosphate buffer. However, the tubulin-membrane interaction differed from tubulin polymerization in several aspects: (a) it occurred at concentrations far below the critical concentration for polymerization; (b) it was not inhibited at low ionic strength and (c) it was colchicine-insensitive. Plasma membranes, mitochondrial membranes, and secretory granule membranes contained tubulin as an integral component. This was demonstrated on intact membrane and on Nonidet P-40 solubilized membrane protein using antitubulin antibodies in antibody retention and radioimmune assays. Membrane tubulin content varied from 2.2 to 4.4 micrograms/mg protein. The involvement of membrane tubulin in tubulin-membrane interactions remains questionable since erythrocyte membranes devoid of membrane tubulin exhibited a low (one-tenth of that of rat liver plasma membranes) but significant tubulin-binding activity. These results show that membranes specialized in different cell functions possess high- affinity, large-capacity tubulin-binding sites...
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机译:我们描述了纯脑微管蛋白与纯化膜的相互作用,该膜专门用于不同的细胞功能,即肝的质膜和线粒体膜以及肾上腺髓质的分泌颗粒膜。我们使用放射性标记的配体受体测定法和抗体保留测定法研究了细胞膜的微管蛋白结合活性。微管蛋白-膜相互作用是时间和温度依赖性的,可逆的,特异性的和可饱和的。微管蛋白与膜的结合似乎是特异性的,因为酸性蛋白(例如血清白蛋白或肌动蛋白)不会干扰结合过程。微管蛋白-膜相互作用的表观总亲和常数在1.5和3.0 X 10(7)M-1之间;对于三种类型的膜获得了相似的值。与膜结合的微管蛋白没有与微管蛋白抗体发生定量反应,因此没有被囊泡包裹。在微管蛋白结合位点饱和时,可逆结合的微管蛋白的量占膜蛋白重量的5-10%(0.4-0.9nmol微管蛋白/ mg膜蛋白)。膜的高微管蛋白结合能力似乎与微管蛋白和膜成分之间的化学计量比为1:1不一致,但可能与一种微管蛋白组装有关。实际上,微管蛋白-膜相互作用与微管形成具有一些共同的特性:(a)微管蛋白与膜的缔合随温度升高而增加,而微管蛋白-膜复合物的离解因温度降低而增加; (b)磷酸盐缓冲液阻止了微管蛋白与膜的结合。然而,微管蛋白-膜相互作用在几个方面不同于微管蛋白聚合:(a)发生在远低于聚合临界浓度的浓度; (b)在低离子强度下不受抑制,(c)对秋水仙碱不敏感。质膜,线粒体膜和分泌性颗粒膜含有微管蛋白作为必不可少的成分。在抗体保留和放射免疫分析中,使用抗微管蛋白抗体在完整膜和Nonidet P-40增溶膜蛋白上证实了这一点。膜微管蛋白含量从2.2到4.4微克/毫克蛋白不等。膜微管蛋白在微管蛋白-膜相互作用中的参与仍然值得怀疑,因为缺乏膜微管蛋白的红细胞膜显示出低的(大鼠肝质膜的十分之一)但显着的微管蛋白结合活性。这些结果表明,专门从事不同细胞功能的膜具有高亲和力,大容量微管蛋白结合位点。
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