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二维核磁共振作为结构相似性的一种探测手段应用于细胞色素c的突变体。

Two-dimensional NMR as a probe of structural similarity applied to mutants of cytochrome c.

作者信息

Pielak G J, Atkinson R A, Boyd J, Williams R J

机构信息

Inorganic Chemistry Laboratory, University of Oxford, England.

出版信息

Eur J Biochem. 1988 Oct 15;177(1):179-85. doi: 10.1111/j.1432-1033.1988.tb14360.x.

Abstract

Using site-directed mutagenesis, it is possible to prepare many mutants of a protein in a short time, and to uncover differences in function. To understand the changes in function, it is essential to understand the effect(s) of the mutation in terms of structural and dynamic changes. It is particularly important to establish a rapid method for comparing the structure of the mutants with that of the wild-type protein. We propose that a combination of overlayed and difference two-dimensional NOE spectra between the wild-type and mutant protein provide a rapid method for determination of structural similarity. The observation of differences other than those due directly to the field effects of the exchanged side chain allow both local and distant conformational changes to be assessed. Here we compare NOESY spectra from a mutant of yeast iso-1-ferrocytochrome c in which the invariant residue Phe-82 has been changed to a Tyr. We conclude that NMR can show subtle changes in protein structure. Specifically, we show the change must involve the reorientation of the side chain of Leu-85 which is proximal to the mutation. The dynamics of the aromatic side chain at position 82 are shown not to give rise to measurable differences between the wild-type and mutant protein. Structural changes are not propagated to a measurable degree in other parts of the protein.

摘要

利用定点诱变技术,能够在短时间内制备出一种蛋白质的多个突变体,并揭示其功能差异。为了理解功能变化,从结构和动力学变化的角度理解突变的影响至关重要。建立一种快速方法来比较突变体与野生型蛋白质的结构尤为重要。我们提出,野生型和突变型蛋白质之间叠加的二维核欧沃豪斯效应(NOE)谱和差值二维NOE谱相结合,为确定结构相似性提供了一种快速方法。观察到的并非直接由交换侧链的场效应导致的差异,使得局部和远距离的构象变化都能够得到评估。在此,我们比较了酵母同工酶-1-亚铁细胞色素c的一个突变体的核欧沃豪斯效应相关光谱(NOESY谱),该突变体中不变残基苯丙氨酸-82已被替换为酪氨酸。我们得出结论,核磁共振(NMR)能够显示蛋白质结构中的细微变化。具体而言,我们表明这种变化必定涉及到靠近突变位点的亮氨酸-85侧链的重新定向。位置82处芳香族侧链的动力学变化并未在野生型和突变型蛋白质之间产生可测量的差异。结构变化在蛋白质的其他部分并未传播到可测量的程度。

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