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一种用于内在无序蛋白质中明确归属的降维核磁共振脉冲序列及高效方案。

A reduced dimensionality NMR pulse sequence and an efficient protocol for unambiguous assignment in intrinsically disordered proteins.

作者信息

Reddy Jithender G, Hosur Ramakrishna V

机构信息

Department of Chemical Sciences, Tata Institute of Fundamental Research (TIFR), 1, Homi Bhabha Road, Colaba, 400005, Mumbai, India.

出版信息

J Biomol NMR. 2014 Jul;59(3):199-210. doi: 10.1007/s10858-014-9839-x. Epub 2014 May 23.

Abstract

Resonance assignment in intrinsically disordered proteins poses a great challenge because of poor chemical shift dispersion in most of the nuclei that are commonly monitored. Reduced dimensionality (RD) experiments where more than one nuclei are co-evolved simultaneously along one of the time axes of a multi-dimensional NMR experiment help to resolve this problem partially, and one can conceive of different combinations of nuclei for co-evolution depending upon the magnetization transfer pathways and the desired information content in the spectrum. Here, we present a RD experiment, (4,3)D-hNCOCAnH, which uses a combination of CO and CA chemical shifts along one of the axes of the 3-dimensional spectrum, to improve spectral dispersion on one hand, and provide information on four backbone atoms of every residue-HN, N, CA and CO chemical shifts-from a single experiment, on the other. The experiment provides multiple unidirectional sequential (i → i - 1) amide (1)H correlations along different planes of the spectrum enabling easy assignment of most nuclei along the protein backbone. Occasional ambiguities that may arise due to degeneracy of amide proton chemical shifts are proposed to be resolved using the HNN experiment described previously (Panchal et al. in J Biomol NMR 20:135-147, 2001). Applications of the experiment and the assignment protocol have been demonstrated using intrinsically disordered α-synuclein (140 aa) protein.

摘要

由于在大多数常用监测核中化学位移分散性较差,内在无序蛋白质中的共振归属面临巨大挑战。在多维核磁共振实验的一个时间轴上同时使多个核共同演化的降维(RD)实验有助于部分解决这个问题,并且根据磁化转移途径和谱图中所需的信息内容,可以设想不同的核共同演化组合。在此,我们展示了一个RD实验,即(4,3)D-hNCOCAnH,它在三维谱图的一个轴上结合了CO和CA化学位移,一方面改善谱图分散性,另一方面从单个实验中提供每个残基的四个主链原子(-HN、N、CA和CO化学位移)的信息。该实验沿着谱图的不同平面提供多个单向顺序(i → i - 1)酰胺(1)H相关性,从而便于沿着蛋白质主链对大多数核进行归属。有人提出,由于酰胺质子化学位移简并可能产生的偶尔模糊性,可以使用先前描述的HNN实验(Panchal等人,《生物分子核磁共振杂志》20:135 - 147,2001年)来解决。使用内在无序的α-突触核蛋白(140个氨基酸)蛋白证明了该实验和归属方案的应用。

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