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构建辐条:鞭毛辐条蛋白3(RSP3)是一种二聚体。

Building a radial spoke: flagellar radial spoke protein 3 (RSP3) is a dimer.

作者信息

Wirschell Maureen, Zhao Feifei, Yang Chun, Yang Pinfen, Diener Dennis, Gaillard Anne, Rosenbaum Joel L, Sale Winfield S

机构信息

Department of Cell Biology, Emory University School of Medicine, Atlanta, Georgia 30322, USA.

出版信息

Cell Motil Cytoskeleton. 2008 Mar;65(3):238-48. doi: 10.1002/cm.20257.

Abstract

Radial spokes are critical multisubunit structures required for normal ciliary and eukaryotic flagellar motility. Experimental evidence indicates the radial spokes are mechanochemical transducers that transmit signals from the central pair apparatus to the outer doublet microtubules for local control of dynein activity. Recently, progress has been made in identifying individual components of the radial spoke, yet little is known about how the radial spoke is assembled or how it performs in signal transduction. Here we focus on radial spoke protein 3 (RSP3), a highly conserved AKAP located at the base of the radial spoke stalk and required for radial spoke assembly on the doublet microtubules. Biochemical approaches were taken to further explore the functional role of RSP3 within the radial spoke structure and for control of motility. Chemical crosslinking, native gel electrophoresis, and epitope-tagged RSP3 proteins established that RSP3 forms a dimer. Analysis of truncated RSP3 proteins indicates the dimerization domain coincides with the previously characterized axoneme binding domain in the N-terminus. We propose a model in which each radial spoke structure is built on an RSP3 dimer, and indicating that each radial spoke can potentially localize multiple PKAs or AKAP-binding proteins in position to control dynein activity and flagellar motility.

摘要

辐条是正常纤毛和真核生物鞭毛运动所必需的关键多亚基结构。实验证据表明,辐条是机械化学换能器,可将信号从中央微管对传递到外部双联微管,以局部控制动力蛋白的活性。最近,在确定辐条的各个组成部分方面取得了进展,但对于辐条如何组装或其在信号转导中的作用知之甚少。在这里,我们聚焦于辐条蛋白3(RSP3),它是一种高度保守的A激酶锚定蛋白,位于辐条柄的基部,是双联微管上辐条组装所必需的。我们采用生化方法进一步探究RSP3在辐条结构中的功能作用以及对运动的控制。化学交联、非变性凝胶电泳和表位标记的RSP3蛋白证实RSP3形成二聚体。对截短的RSP3蛋白的分析表明,二聚化结构域与先前在N端鉴定的轴丝结合结构域一致。我们提出了一个模型,其中每个辐条结构都基于一个RSP3二聚体构建,这表明每个辐条都可能将多个蛋白激酶A或A激酶锚定蛋白结合蛋白定位在适当位置,以控制动力蛋白的活性和鞭毛运动。

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