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通过动态核极化实现RNA-蛋白质界面的特异性信号增强

Specific Signal Enhancement on an RNA-Protein Interface by Dynamic Nuclear Polarization.

作者信息

Aladin Victoria, Sreemantula Arun K, Biedenbänder Thomas, Marchanka Alexander, Corzilius Björn

机构信息

Institute of Chemistry, University of Rostock, Albert-Einstein-Str. 27, 18059, Rostock, Germany.

Department Life, Light & Matter, University of Rostock, Albert-Einstein-Str. 25, 18059, Rostock, Germany.

出版信息

Chemistry. 2023 Mar 16;29(16):e202203443. doi: 10.1002/chem.202203443. Epub 2023 Feb 7.

Abstract

Sensitivity and specificity are both crucial for the efficient solid-state NMR structure determination of large biomolecules. We present an approach that features both advantages by site-specific enhancement of NMR spectroscopic signals from the protein-RNA binding site within a ribonucleoprotein (RNP) by dynamic nuclear polarization (DNP). This approach uses modern biochemical techniques for sparse isotope labeling and exploits the molecular dynamics of C-labeled methyl groups exclusively present in the protein. These dynamics drive heteronuclear cross relaxation and thus allow specific hyperpolarization transfer across the biomolecular complex's interface. For the example of the L7Ae protein in complex with a 26mer guide RNA minimal construct from the box C/D complex in archaea, we demonstrate that a single methyl-nucleotide contact is responsible for most of the polarization transfer to the RNA, and that this specific transfer can be used to boost both NMR spectral sensitivity and specificity by DNP.

摘要

灵敏度和特异性对于高效确定大型生物分子的固态核磁共振结构都至关重要。我们提出了一种方法,该方法通过动态核极化(DNP)对核糖核蛋白(RNP)中蛋白质-RNA结合位点的核磁共振光谱信号进行位点特异性增强,兼具两者优势。此方法采用现代生化技术进行稀疏同位素标记,并利用仅存在于蛋白质中的碳标记甲基基团的分子动力学。这些动力学驱动异核交叉弛豫,从而允许在生物分子复合物界面进行特定的超极化转移。以古细菌中与来自盒C/D复合物的26聚体引导RNA最小构建体形成复合物的L7Ae蛋白为例,我们证明单个甲基-核苷酸接触是大部分极化转移至RNA的原因,并且这种特异性转移可用于通过DNP提高核磁共振光谱的灵敏度和特异性。

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