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微管与垂体分泌颗粒及分泌颗粒膜的结合。

Binding of microtubules to pituitary secretory granules and secretory granule membranes.

作者信息

Sherline P, Lee Y C, Jacobs L S

出版信息

J Cell Biol. 1977 Feb;72(2):380-9. doi: 10.1083/jcb.72.2.380.

Abstract

Microtubules assembled in vitro were bound to purified porcine pituitary secretory granules and to isolated granule membranes. The interaction between microtubules and whole secretory granules was demonstrated by alteration in the sedimentation properties of the microtubules. Incubation of secretory granules with microtubules resulted in pelleting of microtubules which increased as a function of the number of granules added. Binding was quantitated by measurement of the tubulin remaining in the supernate after centrifugation. The interaction of secretory granules and microtubules was inhibited by nucleoside triphosphates and augmented by adenosine 5'-monophosphate and adenosine. When depolymerized protein from microtubules was incubated with secretory granules, the granules did not appear to bind the soluble tubulin dimer present in these preparations. However, the high molecular weight protein associated with microtubules was adsorbed by secretory granules during the binding process. Incubation of isolated secretory granule membranes with microtubules followed by centrifugation to density equilibrium in a discontinuous sucrose density gradient caused pelleting of the membranes, which otherwise banded higher in the gradient. The visible alteration in membrane sedimentation was confirmed by measurements of the membrane-associated magnesium-ATPase activity and by a shift in radioactivity in iodinated membrane preparations. Our data suggest a role for microtubules in the intracellular movement of secretory granules; this movement is perhaps brought about by dynein-like cross bridges which link the tubulin backbone and granule surface.

摘要

在体外组装的微管与纯化的猪垂体分泌颗粒及分离的颗粒膜相结合。微管沉降特性的改变证明了微管与整个分泌颗粒之间的相互作用。分泌颗粒与微管一起温育导致微管沉淀,沉淀量随添加颗粒数量的增加而增加。通过测量离心后上清液中剩余的微管蛋白来定量结合。核苷三磷酸抑制分泌颗粒与微管的相互作用,而5'-单磷酸腺苷和腺苷增强这种相互作用。当将来自微管的解聚蛋白与分泌颗粒一起温育时,颗粒似乎不结合这些制剂中存在的可溶性微管蛋白二聚体。然而,与微管相关的高分子量蛋白在结合过程中被分泌颗粒吸附。将分离的分泌颗粒膜与微管一起温育,然后在不连续蔗糖密度梯度中离心至密度平衡,导致膜沉淀,否则膜在梯度中会位于更高位置。通过测量与膜相关的镁 - ATP酶活性以及碘化膜制剂中放射性的变化,证实了膜沉降的明显改变。我们的数据表明微管在分泌颗粒的细胞内移动中起作用;这种移动可能是由类似动力蛋白的跨桥引起的,这些跨桥连接微管蛋白骨架和颗粒表面。

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