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基于残基特异性的实时核磁共振扩散实验确定了蛋白质折叠过程中的缔合状态。

Residue-specific real-time NMR diffusion experiments define the association states of proteins during folding.

作者信息

Buevich Alexei V, Baum Jean

机构信息

Department of Chemistry, Rutgers University, Piscataway, New Jersey 08854, USA.

出版信息

J Am Chem Soc. 2002 Jun 19;124(24):7156-62. doi: 10.1021/ja012699u.

DOI:10.1021/ja012699u
PMID:12059241
Abstract

Characterizing the association states of proteins during folding is critical for understanding the nature of protein-folding intermediates and protein-folding pathways, protein aggregation, and disease-related aggregation. To study the association states of unfolded, folded, and intermediate species during protein folding, we have introduced a novel residue-specific real-time NMR diffusion experiment. This experiment, a combination of NMR real-time folding experiments and 3D heteronuclear pulsed field gradient NMR diffusion experiments (LED-HSQC), measures hydrodynamic properties, or molecular sizes, of kinetic species directly during the folding process. Application of the residue-specific real-time NMR diffusion experiments to characterize the folding of the collagen triple helix motif shows that this experiment can be used to determine the association states of unfolded, folded, and kinetic intermediates with transient lifetimes simultaneously. The ratio of the apparent translational diffusion coefficients of the unfolded to the folded form of the triple helix is 0.59, which correlates very well with a theoretical ratio for monomer to linear trimer. The apparent diffusion coefficients of the kinetic intermediates formed during triple helix folding indicate the formation of trimer-like associates which is consistent with previously published kinetic and relaxation data. The residue-specific time dependence of apparent diffusion coefficients of monomer and trimer peaks also illustrates the ability to use diffusion data to probe the directionality of triple helix formation. NMR diffusion experiments provide a new strategy for the investigation of protein-folding mechanisms, both to understand the role of kinetic intermediates and to determine the time-dependent aggregation processes in human diseases.

摘要

表征蛋白质折叠过程中的缔合状态对于理解蛋白质折叠中间体的性质、蛋白质折叠途径、蛋白质聚集以及与疾病相关的聚集至关重要。为了研究蛋白质折叠过程中未折叠、折叠和中间体物种的缔合状态,我们引入了一种新型的基于残基特异性的实时核磁共振扩散实验。该实验结合了核磁共振实时折叠实验和三维异核脉冲场梯度核磁共振扩散实验(LED-HSQC),可在折叠过程中直接测量动力学物种的流体动力学性质或分子大小。将基于残基特异性的实时核磁共振扩散实验应用于表征胶原蛋白三螺旋基序的折叠,结果表明该实验可用于同时确定未折叠、折叠和具有短暂寿命的动力学中间体的缔合状态。三螺旋未折叠形式与折叠形式的表观平移扩散系数之比为0.59,这与单体与线性三聚体的理论比值非常吻合。三螺旋折叠过程中形成的动力学中间体的表观扩散系数表明形成了三聚体样缔合体,这与先前发表的动力学和弛豫数据一致。单体和三聚体峰的表观扩散系数基于残基特异性的时间依赖性也说明了利用扩散数据探测三螺旋形成方向性的能力。核磁共振扩散实验为研究蛋白质折叠机制提供了一种新策略,既有助于理解动力学中间体的作用,也有助于确定人类疾病中随时间变化的聚集过程。

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