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一种提高 N-NMR 弛豫测量中 NH₃⁺基团灵敏度的独特而简单的方法:在蛋白质-DNA 复合物中的应用。

A Unique and Simple Approach to Improve Sensitivity in N-NMR Relaxation Measurements for NH₃⁺ Groups: Application to a Protein-DNA Complex.

机构信息

Department of Biochemistry and Molecular Biology, Sealy Center for Structural Biology and Molecular Biophysics, University of Texas Medical Branch, Galveston, TX 77555, USA.

McGovern Medical School, Brown Foundation Institute of Molecular Medicine for the Prevention of Human Diseases, University of Texas Health Science Center, Houston, TX 77030, USA.

出版信息

Molecules. 2017 Aug 15;22(8):1355. doi: 10.3390/molecules22081355.

Abstract

NMR spectroscopy is a powerful tool for research on protein dynamics. In the past decade, there has been significant progress in the development of NMR methods for studying charged side chains. In particular, NMR methods for lysine side-chain NH₃⁺ groups have been proven to be powerful for investigating the dynamics of hydrogen bonds or ion pairs that play important roles in biological processes. However, relatively low sensitivity has been a major practical issue in NMR experiments on NH₃⁺ groups. In this paper, we present a unique and simple approach to improve sensitivity in N relaxation measurements for NH₃⁺ groups. In this approach, the efficiency of coherence transfers for the desired components are maximized, whereas undesired anti-phase or multi-spin order components are purged through pulse schemes and rapid relaxation. For lysine side-chain NH₃⁺ groups of a protein-DNA complex, we compared the data obtained with the previous and new pulse sequences under the same conditions and confirmed that the N relaxation parameters were consistent for these datasets. While retaining accuracy in measuring N relaxation, our new pulse sequences for NH₃⁺ groups allowed an 82% increase in detection sensitivity of N longitudinal and transverse relaxation measurements.

摘要

NMR 光谱学是研究蛋白质动力学的有力工具。在过去的十年中,用于研究带电侧链的 NMR 方法取得了重大进展。特别是,用于赖氨酸侧链 NH₃⁺基团的 NMR 方法已被证明对于研究在生物过程中起重要作用的氢键或离子对的动力学非常有效。然而,在 NH₃⁺基团的 NMR 实验中,相对较低的灵敏度一直是一个主要的实际问题。在本文中,我们提出了一种独特而简单的方法来提高 NH₃⁺基团的 N 弛豫测量灵敏度。在这种方法中,通过脉冲方案和快速弛豫来最大化所需组件的相干转移效率,同时清除不需要的反相或多自旋顺序组件。对于蛋白质-DNA 复合物中的赖氨酸侧链 NH₃⁺基团,我们在相同条件下比较了使用先前和新脉冲序列获得的数据,并确认这些数据集的 N 弛豫参数是一致的。在保留测量 N 弛豫准确性的同时,我们用于 NH₃⁺基团的新脉冲序列允许 N 纵向和横向弛豫测量的检测灵敏度提高 82%。

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