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通过硫 K 边荧光 X 射线近边结构光谱法探测朊病毒 Ure2p 在蛋白质原纤维中的堆积情况。

Packing of the prion Ure2p in protein fibrils probed by fluorescence X-ray near-edge structure spectroscopy at sulfur K-edge.

作者信息

Fayard Barbara, Fay Nicolas, David Gabriel, Doucet J, Melki Ronald

机构信息

Laboratoire de Physique des Solides, Université Paris-Sud, F-91405 Orsay cedex, France.

出版信息

J Mol Biol. 2006 Mar 3;356(4):843-9. doi: 10.1016/j.jmb.2005.12.011. Epub 2005 Dec 20.

Abstract

The soluble protein Ure2p from the yeast Saccharomyces cerevisiae assembles in vitro into straight and insoluble protein fibrils, through subtle changes of conformation. Whereas the structure of soluble Ure2p has been revealed by X-ray crystallography, further characterization of the structure of insoluble Ure2p fibrils is needed. We performed X-ray absorption near-edge spectroscopy (XANES) at the sulfur K-edge to probe the state of Cys221 in the fibrillar form of Ure2pC221 and provide structural information on the structure of Ure2p within fibrils. Although the Ure2p dimer dissociation into its constituent monomers has proven to be a prerequisite for assembly into fibrils, we showed the ability of every Ure2pC221 monomer to establish disulfide bonds upon incubation of the fibrils under oxidizing conditions. Our result indicates either that the constituent unit of the fibrillar form of the protein is a dimeric Ure2p or that the fibrils are made of protofilaments assembled in such a way that the residue C221 from a Ure2p molecule in one protofilament is located in the vicinity of a C221 residue from another molecule belonging to a neighbor protofilament.

摘要

来自酿酒酵母的可溶性蛋白Ure2p在体外通过构象的细微变化组装成直的不溶性蛋白纤维。虽然可溶性Ure2p的结构已通过X射线晶体学揭示,但仍需要对不溶性Ure2p纤维的结构进行进一步表征。我们在硫K边进行了X射线吸收近边光谱(XANES),以探测Ure2pC221纤维状形式中Cys221的状态,并提供关于纤维中Ure2p结构的结构信息。尽管已证明Ure2p二聚体解离成其组成单体是组装成纤维的前提条件,但我们展示了在氧化条件下孵育纤维时每个Ure2pC221单体建立二硫键的能力。我们的结果表明,该蛋白质纤维状形式的组成单元要么是二聚体Ure2p,要么是由原丝组装而成的纤维,其中一条原丝中Ure2p分子的C221残基位于属于相邻原丝的另一个分子的C221残基附近。

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