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中间丝中卷曲螺旋结构域和亚基组装的实时观察

Real-time observation of coiled-coil domains and subunit assembly in intermediate filaments.

作者信息

Hess John F, Voss John C, FitzGerald Paul G

机构信息

Department of Cell Biology and Human Anatomy, University of California, School of Medicine, Davis, California 95616, USA.

出版信息

J Biol Chem. 2002 Sep 20;277(38):35516-22. doi: 10.1074/jbc.M206500200. Epub 2002 Jul 16.

Abstract

We have utilized electron paramagnetic resonance spectroscopy to study secondary structure, subunit interaction, and molecular orientation of vimentin molecules within intact intermediate filaments and assembly intermediates. Spectroscopy data prove alpha-helical coiled-coil structures at individual amino acids 316-336 located in rod 2B. Analysis of positions 305, 309, and 312 identify this region as conforming to the helical pattern identified within 316-336 and thus demonstrates that, contrary to some previous predictions, this region is in an alpha-helical conformation. We show that by varying the position of the spin label, we can identify both intra- and inter-dimer interactions. With a label attached to the outside of the alpha-helix, we have been able to measure interactions between positions 348 of separate dimers as they align together in intact filaments, identifying the exact point of overlap. By mixing different spin-labeled proteins, we demonstrate that the interaction at position 348 is the result of an anti-parallel arrangement of dimers. This approach provides high resolution structural information (<2 nm resolution), can be used to identify molecular arrangements between subunits in an intact intermediate filament, and should be applicable to other noncrystallizable filamentous systems as well as to the study of protein fibrils.

摘要

我们利用电子顺磁共振光谱研究了完整中间丝和组装中间体中波形蛋白分子的二级结构、亚基相互作用及分子取向。光谱数据证明位于杆状区2B的单个氨基酸316 - 336处存在α-螺旋卷曲螺旋结构。对305、309和312位的分析表明该区域符合316 - 336内确定的螺旋模式,因此表明,与之前的一些预测相反,该区域处于α-螺旋构象。我们表明,通过改变自旋标记的位置,我们可以识别二聚体内和二聚体间的相互作用。在α-螺旋外部附着一个标记后,我们能够测量完整丝中单独二聚体的348位之间的相互作用,当它们对齐时可确定精确的重叠点。通过混合不同的自旋标记蛋白,我们证明348位的相互作用是二聚体反平行排列的结果。这种方法提供了高分辨率的结构信息(分辨率<2 nm),可用于识别完整中间丝中亚基之间的分子排列,并且应该适用于其他不可结晶的丝状系统以及蛋白质原纤维的研究。

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