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微管相关蛋白与肌动蛋白丝的相互作用。运用荧光光漂白恢复技术的研究。

Interaction of microtubule-associated proteins with actin filaments. Studies using the fluorescence-photobleaching recovery technique.

作者信息

Arakawa T, Frieden C

出版信息

J Biol Chem. 1984 Oct 10;259(19):11730-4.

PMID:6480581
Abstract

The interaction of microtubule-associated proteins with actin filaments has been investigated by measuring the diffusion coefficient of either the filament or the microtubule-associated proteins. Experiments were performed using the technique of fluorescence photobleaching recovery with actin labeled with iodoacetamidotetramethyl rhodamine or microtubule-associated proteins labeled with iodoacetamidofluorescein. Actin filaments composed of pure rhodamine-labeled actin are not immobilized under a variety of conditions (Tait, J. F., and Frieden, C. (1982c) Biochemistry 21, 6046-6053). We find that addition of microtubule-associated proteins to rhodamine-labeled actin in a ratio as low as 1:1000 can cause immobilization, presumably cross-linking actin into a network of nondiffusible filaments. Immobilization occurs after polymerization is complete, suggesting either a length redistribution of actin filaments, a redistribution of the cross-links between filaments, or the slow addition of actin filaments to other filaments via the microtubule-associated protein. Experiments using fluorescein-labeled microtubule-associated proteins show that these proteins are bound to actin filaments as they are formed and that binding depended on actin concentration, indicating that there are a number of binding sites on the actin filaments. However, while the actin filaments become completely immobilized, the microtubule-associated proteins become only partially immobilized suggesting at least two different classes of binding affinities. The large peptide obtained from trypsin-treated fluorescein-labeled microtubule-associated proteins is not able to immobilize actin filaments since it does not bind to the filaments.

摘要

通过测量肌动蛋白丝或微管相关蛋白的扩散系数,对微管相关蛋白与肌动蛋白丝之间的相互作用进行了研究。实验采用荧光光漂白恢复技术,用碘乙酰胺基四甲基罗丹明标记肌动蛋白或用碘乙酰胺基荧光素标记微管相关蛋白。由纯罗丹明标记的肌动蛋白组成的肌动蛋白丝在各种条件下都不会固定(泰特,J.F.,和弗里登,C.(1982c)《生物化学》21,6046 - 6053)。我们发现,以低至1:1000的比例向罗丹明标记的肌动蛋白中添加微管相关蛋白会导致固定,推测是将肌动蛋白交联成不可扩散的丝网络。固定在聚合完成后发生,这表明要么是肌动蛋白丝的长度重新分布,要么是丝之间交联的重新分布,要么是通过微管相关蛋白将肌动蛋白丝缓慢添加到其他丝上。使用荧光素标记的微管相关蛋白进行的实验表明,这些蛋白在肌动蛋白丝形成时就与之结合,并且结合取决于肌动蛋白浓度,这表明肌动蛋白丝上有许多结合位点。然而,虽然肌动蛋白丝完全固定,但微管相关蛋白只是部分固定,这表明至少有两类不同的结合亲和力。从经胰蛋白酶处理的荧光素标记的微管相关蛋白中获得的大肽不能固定肌动蛋白丝,因为它不与丝结合。

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