Beta cap73: a novel beta actin-specific binding protein.

C B Shuster, A Y Lin, R Nayak, I M Herman
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引用次数: 55

Abstract

Whereas actin-binding proteins (ABPs) regulate network formation during the cell cycle, it is not known whether ABPs also function to sequester or target isoactins to specific subcellular compartments. Recently, we have shown that ezrin indirectly associates with beta, but not alpha actin filaments in a calcium- and cytochalasin-sensitive manner [Shuster and Herman, 1995: J. Cell Biol. 128:837-848]. To identify the beta actin-specific binding protein that fosters ezrin-beta actin interactions, we developed an isoactin affinity fractionation and F-isoactin overlay/Western blotting technique. Results reveal that a 73 kd polypeptide that co-precipitates with ezrin and beta actin [Shuster and Herman, 1995: J. Cell Biol. 128:837-848] can also binds directly to filaments of beta, but not alpha actin by isoactin overlay. In an effort to establish whether p73 plays a role in regulating beta actin dynamics in cells, we produced monoclonal antibodies by immunizing BALB/c mice with p73-containing lamellar lysates or high salt elutions from beta actin affinity columns. Two monoclonal antibodies were cloned that react with p73 present in fractions released from beta actin Sepharose-4B or purified to homogeneity by DEAE chromatography. Anti-p73 Western blots reveal that there is a 16-fold difference in p73 binding to beta actin vs. alpha actin affinity columns when experiments are performed in physiological salts. To characterize p73-beta actin binding in vitro and establish whether p73 binds along the lengths or at the barbed end of the beta actin filament, we asked whether cytochalasin D (CD) could displace p73 pre-bound to beta actin-Sepharose 4B. Anti-p73 Western blotting reveals that nanomolar concentrations of CD are capable of selectively eluting p73 and ezrin from beta actin Sepharose 4B, indicating that p73 binds beta actin via the barbed end. Simultaneous double antibody localization studies using anti-beta actin IgG and anti-p73 IgM reveal that p73 and beta actin are co-localized in the forward aspects of motile cytoplasmic domains, in close proximity to the plasma membrane. Because of its isoform-specific interactions with the barbed end of beta actin filaments, we have named this molecule beta cap73. These results indicate that isoform-specific actin-binding proteins can be identified from cortical cytoplasm, and suggest that beta cap73 may not only act to spatially regulate the intracellular distribution of isoactins, but may also facilitate forward protrusion formation through the regulated release of free filament ends during cell motility.

β cap73:一种新的β肌动蛋白特异性结合蛋白。
虽然肌动蛋白结合蛋白(ABPs)在细胞周期中调节网络的形成,但目前尚不清楚ABPs是否也具有隔离或靶向等肌动蛋白到特定亚细胞区室的功能。最近,我们发现ezrin间接地与β肌动蛋白丝结合,而不是以钙和细胞松弛素敏感的方式与α肌动蛋白丝结合[Shuster和Herman, 1995: J.细胞生物学杂志,128:837-848]。为了鉴定促进ezrin- β肌动蛋白相互作用的β肌动蛋白特异性结合蛋白,我们开发了一种等肌动蛋白亲和分离和f -等肌动蛋白覆盖/Western印迹技术。结果表明,与ezrin和β肌动蛋白共沉淀的73 kd多肽[Shuster and Herman, 1995: J. Cell Biol. 128:837-848]也可以直接与β肌动蛋白结合,但不能通过等肌动蛋白覆盖与α肌动蛋白结合。为了确定p73是否在细胞中调节-肌动蛋白动力学中起作用,我们用含有p73的层状裂解物或β -肌动蛋白亲和柱的高盐洗脱液免疫BALB/c小鼠,制备了单克隆抗体。克隆了两种单克隆抗体,它们与β actin Sepharose-4B释放的p73反应,或通过DEAE层析纯化至均质。抗p73 Western blots显示,在生理盐中进行实验时,p73与β肌动蛋白的结合与α肌动蛋白亲和柱的结合差异为16倍。为了在体外表征p73- β肌动蛋白结合,并确定p73是沿着长度结合还是在β肌动蛋白丝的刺端结合,我们询问细胞松弛素D (CD)是否可以取代p73预结合到β肌动蛋白- sepharose 4B。抗p73 Western blotting显示,纳米摩尔浓度的CD能够选择性地从-肌动蛋白Sepharose 4B中洗脱p73和ezrin,表明p73通过倒刺端与-肌动蛋白结合。利用抗-肌动蛋白IgG和抗p73 IgM同时进行的双抗体定位研究表明,p73和-肌动蛋白在运动细胞质结构域的前侧共定位,靠近质膜。由于它与-肌动蛋白丝的带刺末端具有同型特异性相互作用,我们将这种分子命名为- cap73。这些结果表明,可以从皮质细胞质中鉴定出同种异构体特异性肌动蛋白结合蛋白,并提示β - cap73可能不仅在空间上调节异动蛋白在细胞内的分布,还可能在细胞运动过程中通过调节游离丝末端的释放来促进前突的形成。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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