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Characterization of Folding Intermediates of a Domain-Swapped Protein by Solid-State NMR Spectroscopy

机译:固态核磁共振波谱法表征结构域交换蛋白的折叠中间体

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摘要

We have employed two-dimensional solid-state NMR to study structure and dynamics of insoluble folding states of the domain-swapped protein Crh. Starting from the protein precipitated at its pl, conformational changes due to a modest temperature increase were investigated at the level of individual residues and in real-time. As compared to the crystalline state, Crh pl-precipitates exhibited a higher degree of molecular mobility for several regions of the protein. A rigidly intact center was observed including a subset of residues of the hydrophobic core. Raising the temperature by 13 K to 282 K created a partially unfolded intermediate state that was converted into β-sheet-rich aggregates that are mostly of spherical character according to electron microscopy. Residue-by-residue analysis indicated that two out of three α-helices in aggregated Crh underwent major structural rearrangements while the third helix was preserved. Residues in the hinge region exhibited major chemical-shift changes, indicating that the domain swap was not conserved in the aggregated form. Our study provides direct evidence that protein aggregates of a domain-swapped protein retain a significant fraction of native secondary structure and demonstrates that solid-state NMR can be used to directly monitor slow molecular folding events.
机译:我们已使用二维固态NMR研究结构域交换蛋白Crh的不溶性折叠态的结构和动力学。从在p1处沉淀的蛋白质开始,实时研究了由于温和升高而引起的构象变化。与结晶状态相比,Crh pl沉淀物在蛋白质的多个区域均表现出更高的分子迁移率。观察到刚性完整的中心,包括疏水核的残基的子集。将温度提高13 K至282 K,产生了部分展开的中间状态,根据电子显微镜观察,该中间状态转换为富含β-折叠的聚集体,大部分具有球形特征。残基分析表明,聚集Crh中的三个α螺旋中有两个经历了主要的结构重排,而第三个螺旋被保留。铰链区的残基表现出主要的化学位移变化,表明结构域交换不是以聚集形式保守的。我们的研究提供了直接的证据,即域交换蛋白质的蛋白质聚集体保留了很大一部分的天然二级结构,并证明了固态NMR可用于直接监测慢速分子折叠事件。

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