中性粒细胞裂解物中肌动蛋白丝的带刺末端封端活性：封端蛋白β2的作用。

Actin filament barbed-end capping activity in neutrophil lysates: the role of capping protein-beta 2.

作者信息

DiNubile M J, Cassimeris L, Joyce M, Zigmond S H

机构信息

Department of Medicine, Cooper Hospital/University Medical Center, UMDNJ/Robert Wood Johnson Medical School, Camden, USA.

出版信息

Mol Biol Cell. 1995 Dec;6(12):1659-71. doi: 10.1091/mbc.6.12.1659.

DOI:10.1091/mbc.6.12.1659

PMID:8590796

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC301323/

Abstract

A barbed-end capping activity was found in high speed supernates of neutrophils lysed in submicromolar calcium. In dilute supernate (> or = 100-fold dilution of cytoplasm), this activity accounted for most of the inhibition of barbed-end elongation of pyrenyl-G-actin from spectrin-F-actin seeds. Pointed-end elongation from gelsolin-capped F-actin seeds was not inhibited at comparable concentrations of supernate, thus excluding actin monomer sequestration as a cause of the observed inhibition. Most of the capping activity was due to capping protein-beta 2 (a homologue of cap Z). Thus, while immunoadsorption of > or = 95% of the gelsolin in the supernate did not decrease capping activity, immunoadsorption of capping protein-beta 2 reduced capping activity proportionally to the amount of capping protein-beta 2 adsorbed. Depletion of > 90% of capping protein-beta 2 from the supernate removed 90% of its capping activity. The functional properties of the capping activity were defined. The dissociation constant for binding to barbed ends (determined by steady state and kinetic analyses) was approximately 1-2 nM; the on-rate of capping was between 7 x 10(5) and 5 x 10(6) M-1 s-1; and the off-rate was approximately 2 x 10(-3) s-1. The concentration of capper free in the intact cell (determined by adsorption of supernate with spectrin-actin seeds) was estimated to be approximately 1-2 microM. Thus, there appeared to be enough high affinity capper to cap all the barbed ends in vivo. Nevertheless, immediately after lysis with detergent, neutrophils contained sites that nucleate barbed-end elongation of pyrenyl-G-actin. These barbed ends subsequently become capped with a time course and concentration dependence similar to that of spectrin-F-actin seeds in high speed supernates. These observations suggest that, despite the excess of high affinity capper, some ends either are not capped in vivo or are transiently uncapped upon lysis and dilution.

摘要

在亚微摩尔钙浓度下裂解的中性粒细胞的高速上清液中发现了一种带刺末端封端活性。在稀释的上清液中（细胞质稀释100倍或更高），这种活性占了对血影蛋白-F-肌动蛋白种子上的芘基-G-肌动蛋白带刺末端伸长抑制作用的大部分。在相当浓度的上清液中，凝溶胶蛋白封端的F-肌动蛋白种子的尖端伸长未受抑制，因此排除了肌动蛋白单体隔离是观察到的抑制作用的原因。大部分封端活性归因于封端蛋白-β2（帽Z的同源物）。因此，虽然上清液中95%或更多的凝溶胶蛋白进行免疫吸附并没有降低封端活性，但封端蛋白-β2的免疫吸附会使封端活性与吸附的封端蛋白-β2量成比例降低。从上清液中去除90%以上的封端蛋白-β2会消除其90%的封端活性。确定了封端活性的功能特性。与带刺末端结合的解离常数（通过稳态和动力学分析确定）约为1-2 nM；封端的结合速率在7×10⁵至5×10⁶ M⁻¹ s⁻¹之间；解离速率约为2×10⁻³ s⁻¹。完整细胞中游离封端剂的浓度（通过用血影蛋白-肌动蛋白种子吸附上清液确定）估计约为1-2 μM。因此，似乎有足够的高亲和力封端剂在体内封端所有带刺末端。然而，在用去污剂裂解后，中性粒细胞立即含有能使芘基-G-肌动蛋白带刺末端伸长成核的位点。这些带刺末端随后会被封端，其时间进程和浓度依赖性与高速上清液中的血影蛋白-F-肌动蛋白种子相似。这些观察结果表明，尽管有过量的高亲和力封端剂，但一些末端要么在体内未被封端，要么在裂解和稀释时短暂地未被封端。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9893/301323/5df37ffa024e/mbc00081-0063-a.jpg

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Actin filament barbed-end capping activity in neutrophil lysates: the role of capping protein-beta 2.中性粒细胞裂解物中肌动蛋白丝的带刺末端封端活性：封端蛋白β2的作用。

Mol Biol Cell. 1995 Dec;6(12):1659-71. doi: 10.1091/mbc.6.12.1659.

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中性粒细胞裂解物中肌动蛋白丝的带刺末端封端活性：封端蛋白β2的作用。

Actin filament barbed-end capping activity in neutrophil lysates: the role of capping protein-beta 2.

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