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在亚秒级时间分辨率下对蛋白质超极化进行残基分辨监测。

Residue-resolved monitoring of protein hyperpolarization at sub-second time resolution.

作者信息

Negroni Mattia, Kurzbach Dennis

机构信息

Faculty of Chemistry, Institute of Biological Chemistry, University Vienna, Währinger Str. 38, 1090, Vienna, Austria.

出版信息

Commun Chem. 2021 Oct 22;4(1):147. doi: 10.1038/s42004-021-00587-y.

Abstract

Signal-enhancement techniques for NMR spectroscopy are important to amplify the weak resonances provided by nuclear spins. Recently, 'hyperpolarization' techniques have been intensively investigated. These provide nuclear spin states far from equilibrium yielding strong signal boosts up to four orders of magnitude. Here we propose a method for real-time NMR of 'hyperpolarized' proteins at residue resolution. The approach is based on dissolution dynamic nuclear polarization (d-DNP), which enables the use of hyperpolarized buffers that selectively boost NMR signals of solvent-exposed protein residues. The resulting spectral sparseness and signal enhancements enable recording of residue-resolved spectra at a 2 Hz sampling rate. Thus, we monitor the hyperpolarization level of different protein residues simultaneously under near-physiological conditions. We aim to address two points: 1) NMR experiments are often performed under conditions that increase sensitivity but are physiologically irrelevant; 2) long signal accumulation impedes fast real-time monitoring. Both limitations are of fundamental relevance to ascertain pharmacological relevance and study protein kinetics.

摘要

核磁共振波谱的信号增强技术对于放大核自旋提供的微弱共振非常重要。最近,“超极化”技术受到了深入研究。这些技术能产生远离平衡态的核自旋态,使信号增强多达四个数量级。在此,我们提出一种在残基分辨率下对“超极化”蛋白质进行实时核磁共振的方法。该方法基于溶解动态核极化(d-DNP),它能使用超极化缓冲液,选择性地增强溶剂暴露的蛋白质残基的核磁共振信号。由此产生的光谱稀疏性和信号增强使得能够以2赫兹的采样率记录残基分辨光谱。因此,我们能在近生理条件下同时监测不同蛋白质残基的超极化水平。我们旨在解决两点:1)核磁共振实验通常在提高灵敏度但与生理无关的条件下进行;2)长时间的信号积累阻碍了快速实时监测。这两个限制对于确定药理学相关性和研究蛋白质动力学都具有根本意义。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/92b3/9814832/4120d186d5f1/42004_2021_587_Fig1_HTML.jpg

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