Levorin Leonardo, Becker Nina, Uluca-Yazgi Boran, Gardon Luis, Kraus Mirko, Sevenich Marc, Apostolidis Athina, Schmitz Kai, Rüter Neomi, Apanasenko Irina, Willbold Dieter, Hoyer Wolfgang, Neudecker Philipp, Gremer Lothar, Heise Henrike
Institute of Physical Biology, Heinrich-Heine-Universität Düsseldorf, Düsseldorf 40225, Germany.
Institute of Biological Information Processing (IBI-7: Structural Biochemistry), Forschungszentrum Jülich, Jülich 52425, Germany.
J Am Chem Soc. 2025 May 7;147(18):15867-15879. doi: 10.1021/jacs.5c04159. Epub 2025 Apr 26.
Conformations of protein side chains are closely linked to protein function. DNP-enhanced solid-state NMR (ssNMR), which operates at cryogenic temperatures (<110 K), can be used to freeze-trap protein conformations, including the side chains. In the present study, we employed two-dimensional DNP-enhanced ssNMR to get detailed insights into backbone and side chain conformations of isoleucine. We used different amino acid selectively labeled model proteins for intrinsically disordered proteins (IDPs), denatured and well-folded proteins, and amyloid fibrils. C chemical shifts are closely correlated with secondary structure elements and χ and χ angles in isoleucine side chains. Thus, line shape analysis by integration of representative peak areas in 2D spectra provides an accurate overview of the distribution of backbone and side chain conformations. For the well-folded proteins GABARAP and bovine PI3-kinase (PI3K) SH3 domain, most Ile chemical shifts in frozen solution are well resolved and similar to those observed in solution. However, line widths of individual Ile residues are directly linked to residual mobility, and line broadening or even signal splitting appears for those Ile residues, which are not part of well-defined secondary structure elements. For unfolded PI3K SH3 and the IDP α-synuclein (α-syn), all Ile side chains have full conformational freedom, and as a consequence, inhomogeneous line broadening dominates the cryogenic spectra. Moreover, we demonstrate that conformational ensembles of proteins strongly depend on solvent and buffer conditions. This allowed different unfolded structures for chemical and acidic pH denaturation of the PI3K SH3 domain to be distinguished. In amyloid fibrils of α-syn and PI3K SH3, chemical shifts typical for β-strand like secondary structure dominate the spectra, whereas Ile residues belonging to the fuzzy coat still add the IDP-type line shapes. Hence, DNP-enhanced ssNMR is a useful tool for investigating side chain facilitated protein functions and interactions.
蛋白质侧链的构象与蛋白质功能密切相关。动态核极化增强固态核磁共振(ssNMR)在低温(<110 K)下运行,可用于冷冻捕获蛋白质构象,包括侧链构象。在本研究中,我们采用二维动态核极化增强ssNMR来深入了解异亮氨酸的主链和侧链构象。我们使用了不同的氨基酸选择性标记模型蛋白,用于内在无序蛋白(IDP)、变性和折叠良好的蛋白以及淀粉样纤维。碳化学位移与二级结构元件以及异亮氨酸侧链中的χ和χ角密切相关。因此,通过对二维谱中代表性峰面积进行积分的线形分析,可以准确概述主链和侧链构象的分布情况。对于折叠良好的蛋白GABARAP和牛PI3激酶(PI3K)的SH3结构域,冷冻溶液中大多数异亮氨酸的化学位移得到了很好的解析,并且与溶液中观察到的化学位移相似。然而,单个异亮氨酸残基的线宽与残余流动性直接相关,对于那些不属于明确二级结构元件的异亮氨酸残基,会出现线宽变宽甚至信号分裂的现象。对于未折叠的PI3K SH3和内在无序蛋白α-突触核蛋白(α-syn),所有异亮氨酸侧链都具有完全的构象自由度,因此,不均匀线宽展宽主导了低温谱。此外,我们证明了蛋白质的构象集合强烈依赖于溶剂和缓冲条件。这使得能够区分PI3K SH3结构域在化学和酸性pH变性时的不同未折叠结构。在α-syn和PI3K SH3的淀粉样纤维中,类似β-链二级结构的典型化学位移主导了光谱,而属于模糊外层的异亮氨酸残基仍然呈现出内在无序蛋白类型的线形。因此,动态核极化增强ssNMR是研究侧链促进蛋白质功能和相互作用的有用工具。
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