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来自牛晶状体的网蛋白。化学性质、结构分析及相互作用伙伴的初步鉴定。

Plectin from bovine lenses. Chemical properties, structural analysis and initial identification of interaction partners.

作者信息

Weitzer G, Wiche G

机构信息

Institute of Biochemistry, University of Vienna, Austria.

出版信息

Eur J Biochem. 1987 Nov 16;169(1):41-52. doi: 10.1111/j.1432-1033.1987.tb13578.x.

Abstract

Plectin was purified to near homogeneity from epithelial and cortical cell layers of bovine lenses using a simple and fast purification scheme that included as last step, gel permeation chromatography in the presence of 0.25% sodium N-lauroyl sarcosinate. Lens cell plectin showed extensive structural homology to plectin from cultured cells as revealed by immunoblotting experiments and amino acid analysis. Further characterization included solubility in various buffer solutions, codistribution with vimentin in repeated rounds of intermediate filament disassembly and assembly, and hydrodynamic behaviour in high-performance gel permeation chromatography. Electron microscopy of negatively stained and rotary shadowed plectin molecules revealed a dumb-bell-like structure with an estimated relative molecular mass of 1.16 X 10(6). Specific head-to-head self-interaction of plectin molecules at low salt concentrations and formation of large aggregates under high-salt and physiological conditions was also demonstrated. Isolation, as well as reconstitution of soluble protein complexes containing plectin, vimentin and other cytoskeletal and membrane skeleton proteins, provided first hints to plectin's role as an interlinking component of the cytoskeleton and the membrane skeleton of lens tissue.

摘要

使用一种简单快速的纯化方案从牛晶状体的上皮细胞层和皮质细胞层中纯化出接近均一的网蛋白,该方案的最后一步是在0.25%的N-月桂酰肌氨酸钠存在下进行凝胶渗透色谱。免疫印迹实验和氨基酸分析表明,晶状体细胞网蛋白与培养细胞中的网蛋白具有广泛的结构同源性。进一步的特性分析包括在各种缓冲溶液中的溶解度、在中间丝反复解聚和组装过程中与波形蛋白的共分布,以及在高效凝胶渗透色谱中的流体动力学行为。对经负染色和旋转阴影处理的网蛋白分子进行电子显微镜观察,发现其呈哑铃状结构,估计相对分子质量为1.16×10⁶。还证明了网蛋白分子在低盐浓度下特异性的头对头自相互作用,以及在高盐和生理条件下形成大聚集体。包含网蛋白、波形蛋白以及其他细胞骨架和膜骨架蛋白的可溶性蛋白复合物的分离和重组,首次揭示了网蛋白作为晶状体组织细胞骨架和膜骨架的连接成分的作用。

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