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通过核磁共振快速评估蛋白质结构稳定性和折叠验证

Rapid assessment of protein structural stability and fold validation via NMR.

作者信息

Hoffmann Bernd, Eichmüller Christian, Steinhauser Othmar, Konrat Robert

机构信息

Institute of Theoretical Chemistry and Molecular Structural Biology, University of Vienna, Austria.

出版信息

Methods Enzymol. 2005;394:142-75. doi: 10.1016/S0076-6879(05)94006-8.

Abstract

In structural proteomics, it is necessary to efficiently screen in a high-throughput manner for the presence of stable structures in proteins that can be subjected to subsequent structure determination by X-ray or NMR spectroscopy. Here we illustrate that the (1)H chemical distribution in a protein as detected by (1)H NMR spectroscopy can be used to probe protein structural stability (e.g., the presence of stable protein structures) of proteins in solution. Based on experimental data obtained on well-structured proteins and proteins that exist in a molten globule state or a partially folded alpha-helical state, a well-defined threshold exists that can be used as a quantitative benchmark for protein structural stability (e.g., foldedness) in solution. Additionally, in this chapter we describe a largely automated strategy for rapid fold validation and structure-based backbone signal assignment. Our methodology is based on a limited number of NMR experiments (e.g., HNCA and 3D NOESY-HSQC) and performs a Monte Carlo-type optimization. The novel feature of the method is the opportunity to screen for structural fragments (e.g., template scanning). The performance of this new validation tool is demonstrated with applications to a diverse set of proteins.

摘要

在结构蛋白质组学中,有必要以高通量方式高效筛选蛋白质中稳定结构的存在情况,这些蛋白质随后可通过X射线或核磁共振光谱进行结构测定。在此我们表明,通过¹H核磁共振光谱检测到的蛋白质中¹H化学分布可用于探测溶液中蛋白质的结构稳定性(例如,稳定蛋白质结构的存在)。基于对结构良好的蛋白质以及处于熔球态或部分折叠α螺旋态的蛋白质所获得的实验数据,存在一个明确的阈值,可作为溶液中蛋白质结构稳定性(例如,折叠程度)的定量基准。此外,在本章中,我们描述了一种用于快速折叠验证和基于结构的主链信号归属的高度自动化策略。我们的方法基于有限数量的核磁共振实验(例如,HNCA和3D NOESY - HSQC)并进行蒙特卡洛类型的优化。该方法的新颖之处在于有机会筛选结构片段(例如,模板扫描)。通过将其应用于多种蛋白质展示了这种新验证工具的性能。

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