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来自原核生物类核的蛋白质:大肠杆菌DNA结合蛋白NS(HU)四级结构的核磁共振氢谱研究

Proteins from the prokaryotic nucleoid: 1H NMR study of the quaternary structure of Escherichia coli DNA binding protein NS (HU).

作者信息

Paci M, Gualerzi C

出版信息

Biochemistry. 1986 May 20;25(10):2765-9. doi: 10.1021/bi00358a004.

DOI:10.1021/bi00358a004
PMID:3521722
Abstract

The quaternary interactions of Escherichia coli DNA binding proteins NS1, NS2, and NS (NS1 + NS2) have been studied by 1H NMR spectroscopy at 400 MHz following the reversible spectral changes produced by temperature increases on the resonances (Phe ring and His C-2 protons) whose spectral characteristics reflect the formation and dissociation of either homologous or heterologous interactions. These changes include (a) a progressive intensity decrease of the Phe resonances shifted to high field by stacking interactions, (b) a progressive intensity increase of the resonances due to freely rotating Phe, and (c) splitting of the His C-2 proton resonance. The association constants and thermodynamic parameters for the homologous and heterologous interactions were calculated from the molar fractions of the relevant molecular species by assuming that the above effects are due to the existence of simple association equilibria. It was found that two (out of three) phenylalanine residues of each polypeptide chain are involved in quaternary interactions. Quantitative data concerning the internal mobility and mutual orientations in aggregates of these Phe rings were also obtained. From the calculated association constants, from comparison of these data with recent protein-protein cross-linking results [Losso, M. A., Pawlik, R. T., Canonaco, M. A., & Gualerzi, C. O. (1986) Eur. J. Biochem. 155, 27-32], and from other considerations, we suggest that even though stacking of the Phe rings occurs at the interface between monomers, the temperature-dependent alteration of the Phe spectrum monitors shifts of the dimer in equilibrium tetramer equilibrium whereas the splitting of the His C-2 proton resonance most likely monitors the equilibrium between tetramers and larger aggregates.

摘要

通过400 MHz的1H NMR光谱研究了大肠杆菌DNA结合蛋白NS1、NS2和NS(NS1 + NS2)的四级相互作用,研究是在温度升高引起共振(苯丙氨酸环和组氨酸C-2质子)的可逆光谱变化之后进行的,这些共振的光谱特征反映了同源或异源相互作用的形成和解离。这些变化包括:(a)通过堆积相互作用向高场移动的苯丙氨酸共振的强度逐渐降低;(b)由于自由旋转的苯丙氨酸引起的共振强度逐渐增加;(c)组氨酸C-2质子共振的分裂。通过假设上述效应是由于简单缔合平衡的存在,从相关分子物种的摩尔分数计算出同源和异源相互作用的缔合常数和热力学参数。发现每条多肽链的三个苯丙氨酸残基中有两个参与四级相互作用。还获得了有关这些苯丙氨酸环聚集体内部流动性和相互取向的定量数据。根据计算出的缔合常数,将这些数据与最近的蛋白质-蛋白质交联结果[Losso,M. A.,Pawlik,R. T.,Canonaco,M. A.,& Gualerzi,C. O.(1986)Eur. J. Biochem. 155,27 - 32]进行比较,并从其他方面考虑,我们认为即使苯丙氨酸环的堆积发生在单体之间的界面处,苯丙氨酸光谱随温度的变化监测二聚体在平衡四聚体平衡中的移动,而组氨酸C-2质子共振的分裂最有可能监测四聚体与更大聚集体之间的平衡。

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