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一种类似Sfi1p的中心蛋白结合蛋白介导了四膜虫中基于中心蛋白的Ca2+依赖性收缩。

An Sfi1p-like centrin-binding protein mediates centrin-based Ca2+ -dependent contractility in Paramecium tetraurelia.

作者信息

Gogendeau Delphine, Beisson Janine, de Loubresse Nicole Garreau, Le Caer Jean-Pierre, Ruiz Françoise, Cohen Jean, Sperling Linda, Koll France, Klotz Catherine

机构信息

Centre de Génétique Moléculaire, UPR 2167, Centre National de la Recherche Scientifique, 91198 Gif-sur-Yvette, France.

出版信息

Eukaryot Cell. 2007 Nov;6(11):1992-2000. doi: 10.1128/EC.00197-07. Epub 2007 Aug 3.

Abstract

The previous characterization and structural analyses of Sfi1p, a Saccharomyces cerevisiae centrin-binding protein essential for spindle pole body duplication, have suggested molecular models to account for centrin-mediated, Ca2+-dependent contractility processes (S. Li, A. M. Sandercock, P. Conduit, C. V. Robinson, R. L. Williams, and J. V. Kilmartin, J. Cell Biol. 173:867-877, 2006). Such processes can be analyzed by using Paramecium tetraurelia, which harbors a large Ca2+ -dependent contractile cytoskeletal network, the infraciliary lattice (ICL). Previous biochemical and genetic studies have shown that the ICL is composed of diverse centrin isoforms and a high-molecular-mass centrin-associated protein, whose reduced size in the démaillé (dem1) mutant correlates with defective organization of the ICL. Using sequences derived from the high-molecular-mass protein to probe the Paramecium genome sequence, we characterized the PtCenBP1 gene, which encodes a 460-kDa protein. PtCenBP1p displays six almost perfect repeats of ca. 427 amino acids (aa) and harbors 89 potential centrin-binding sites with the consensus motif LLX11F/LX2WK/R, similar to the centrin-binding sites of ScSfi1p. The smaller (260-kDa) protein encoded by the dem1 mutant PtCenBP1 allele comprises only two repeats of 427 aa and 46 centrin-binding sites. By using RNA interference and green fluorescent protein fusion experiments, we showed that PtCenBP1p forms the backbone of the ICL and plays an essential role in its assembly and contractility. This study provides the first in vivo demonstration of the role of Sfi1p-like proteins in centrin-mediated Ca2+-dependent contractile processes.

摘要

Sfi1p是酿酒酵母中一种对纺锤极体复制至关重要的中心蛋白结合蛋白,之前对其进行的特性鉴定和结构分析提出了分子模型,以解释中心蛋白介导的、Ca2+依赖的收缩过程(S. Li、A. M. Sandercock、P. Conduit、C. V. Robinson、R. L. Williams和J. V. Kilmartin,《细胞生物学杂志》173:867 - 877,2006年)。可以通过利用四膜虫来分析此类过程,四膜虫拥有一个大型的Ca2+依赖收缩细胞骨架网络,即纤毛下晶格(ICL)。之前的生化和遗传学研究表明,ICL由多种中心蛋白亚型和一种高分子量中心蛋白相关蛋白组成,在démaillé(dem1)突变体中其尺寸减小与ICL的组织缺陷相关。利用来自高分子量蛋白的序列探测四膜虫基因组序列,我们鉴定了PtCenBP1基因,该基因编码一种460 kDa的蛋白。PtCenBP1p显示出约427个氨基酸(aa)的六个几乎完美的重复序列,并拥有89个潜在的中心蛋白结合位点,其共有基序为LLX11F/LX2WK/R,类似于ScSfi1p的中心蛋白结合位点。由dem1突变体PtCenBP1等位基因编码的较小(260 kDa)蛋白仅包含两个427 aa的重复序列和46个中心蛋白结合位点。通过RNA干扰和绿色荧光蛋白融合实验,我们表明PtCenBP1p形成了ICL的骨架,并在其组装和收缩中起关键作用。这项研究首次在体内证明了结蛋白样蛋白在中心蛋白介导的Ca2+依赖收缩过程中的作用。

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