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蛋白质中的缓慢内部动力学:核磁共振弛豫分散光谱在T4溶菌酶腔突变体甲基基团中的应用。

Slow internal dynamics in proteins: application of NMR relaxation dispersion spectroscopy to methyl groups in a cavity mutant of T4 lysozyme.

作者信息

Mulder Frans A A, Hon Bin, Mittermaier Anthony, Dahlquist Frederick W, Kay Lewis E

机构信息

Protein Engineering Network Centres of Excellence and Department of Medical Genetics, University of Toronto, Toronto M5S 1A8, Canada.

出版信息

J Am Chem Soc. 2002 Feb 20;124(7):1443-51. doi: 10.1021/ja0119806.

Abstract

Recently developed carbon transverse relaxation dispersion experiments (Skrynnikov, N. R.; et al. J. Am. Chem. Soc. 2001, 123, 4556-4566) were applied to the study of millisecond to microsecond time scale motions in a cavity mutant of T4 lysozyme (L99A) using methyl groups as probes of dynamics. Protein expressed in E. coli cells with (13)CH(3)-pyruvate as the sole carbon source contained high levels of (13)C enrichment at a total of 80 Val gamma, Leu delta, Ile gamma (2), Ala beta, and Met epsilon methyl positions with little extraneous incorporation. Data for 72 methyl groups were available for analysis. Dispersion profiles with large amplitudes were measured for many of these residues and were well fit to a two-state exchange model. The interconversion rates and populations of the states, obtained from fitting relaxation dispersion profiles of each individual probe, were remarkably homogeneous and data for nearly all methyl groups in the protein could be collectively fit to a single cooperative conformational transition. The present study demonstrates the general applicability of methyl relaxation dispersion measurements for the investigation of millisecond time scale protein motions at a large number of side-chain positions. Potential artifacts associated with the experiments are described and methods to minimize their effects presented. These experiments should be particularly well suited for probing dynamics in high molecular weight systems due to the favorable NMR spectroscopic properties of methyl groups.

摘要

最近开发的碳横向弛豫色散实验(Skrynnikov,N. R.;等人,《美国化学会志》,2001年,123卷,4556 - 4566页)被应用于研究T4溶菌酶(L99A)的一个腔突变体中毫秒到微秒时间尺度的运动,使用甲基作为动力学探针。在以(13)CH(3)-丙酮酸作为唯一碳源的大肠杆菌细胞中表达的蛋白质,在总共80个缬氨酸γ、亮氨酸δ、异亮氨酸γ(2个)、丙氨酸β和甲硫氨酸ε甲基位置含有高水平的(13)C富集,且几乎没有外来掺入。有72个甲基的数据可用于分析。对许多这些残基测量了具有大振幅的色散曲线,并很好地拟合了双态交换模型。从拟合每个单独探针的弛豫色散曲线获得的状态间转换速率和种群非常均匀,并且蛋白质中几乎所有甲基的数据都可以共同拟合到一个单一的协同构象转变。本研究证明了甲基弛豫色散测量对于研究大量侧链位置的毫秒时间尺度蛋白质运动的普遍适用性。描述了与实验相关的潜在假象,并提出了最小化其影响的方法。由于甲基有利的核磁共振光谱性质,这些实验应该特别适合于探测高分子量系统中的动力学。

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