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亚基解离前压力对寡聚蛋白结构的影响。

Pressure effects on the structure of oligomeric proteins prior to subunit dissociation.

作者信息

Cioni P, Strambini G B

机构信息

C.N.R.-Istituto di Biofisica, Pisa, Italy.

出版信息

J Mol Biol. 1996 Nov 15;263(5):789-99. doi: 10.1006/jmbi.1996.0616.

DOI:10.1006/jmbi.1996.0616
PMID:8947576
Abstract

In studies of pressure-induced subunit dissociation of protein aggregates, now widely used to evaluate the association free energy, entropy and enthalpy of very stable complexes, it is assumed that high pressure does not influence their structure/thermodynamic parameters and that some peculiarities of these equilibria, such as the decrease in subunit affinity at larger degrees of dissociation (alpha) and hysteresis in alpha/pressure diagrams are imputable to the slow conformational drift of isolated subunits. To test this premise, the conformation of dimeric alcohol dehydrogenase from horse liver and alkaline phosphatase from Escherichia coli was monitored as a function of pressure (up to 3 kbar) and temperature (0 to 50 degrees C) by means of the intrinsic Trp fluorescence and phosphorescence emission and binding of the 1-anilinonaphatalene-8-sulphonic acid (ANS) fluorophore. The results show a distinct influence of high pressure on the native dimers whose changes in conformation may, depending on whether or not these alterations are promptly reversed, be distinguished in elastic and inelastic changes. Elastic changes are ubiquitous and refer to pronounced modulations of the phosphorescence lifetime which is a monitor of the internal flexibility of the macromolecules. They attest to a tightening of the globular structure in the lower pressure range (below 1.5 kbar) as opposed to an increased fluidity in the higher range. The trend is similar between the two proteins and the tightening/loosening effect is fully consistent with the role that internal cavities and hydration of polypeptide is expected to play in determining the compressibility of these biopolymers. Inelastic perturbations reveal a more profound loosening of the globular fold and were observed only with alcohol dehydrogenase under conditions (low temperature (t < 10 degrees C) and high pressure (p > 2.5 kbar)) that favour protein hydration. They involve slow consecutive reactions that produce drastic reductions in phosphorescence lifetime, spectral red shifts, quenching of fluorescence and phosphorescence emission and modulation of ANS binding. Judging from the full protection afforded by glycerol as cosolvent, or the remarkable enhancement caused by modest concentrations of urea, the driving force of these perturbations appears to be pressure-induced hydration of the protein. Inelastic conformational changes are accompanied by a slow and often incomplete recovery of enzymatic activity. The characteristic times of these processes, their pressure dependence and the slow, thermally activated, reversibility are discussed in the light of hysteresis phenomena and changes of subunit affinity in dissociation equilibria.

摘要

在蛋白质聚集体压力诱导亚基解离的研究中,目前该方法被广泛用于评估非常稳定复合物的缔合自由能、熵和焓。研究假定高压不会影响其结构/热力学参数,并且这些平衡的一些特性,例如在较大解离度(α)下亚基亲和力的降低以及α/压力图中的滞后现象,可归因于分离亚基的缓慢构象漂移。为了验证这一前提,通过内在色氨酸荧光、磷光发射以及1-苯胺基萘-8-磺酸(ANS)荧光团的结合,监测了来自马肝的二聚体乙醇脱氢酶和来自大肠杆菌的碱性磷酸酶的构象随压力(高达3千巴)和温度(0至50摄氏度)的变化。结果表明高压对天然二聚体有明显影响,其构象变化根据这些改变是否能迅速逆转,可分为弹性变化和非弹性变化。弹性变化普遍存在,指的是磷光寿命的显著调制,而磷光寿命是大分子内部柔韧性的一种监测指标。它们证明在较低压力范围(低于1.5千巴)球状结构收紧,而在较高压力范围流动性增加。两种蛋白质之间的趋势相似,收紧/松弛效应与多肽的内部空腔和水合作用在决定这些生物聚合物可压缩性方面所起的作用完全一致。非弹性扰动揭示了球状折叠更深刻的松弛,并且仅在有利于蛋白质水合的条件下(低温(t < 10摄氏度)和高压(p > 2.5千巴))对乙醇脱氢酶观察到这种情况。它们涉及缓慢的连续反应,这些反应会导致磷光寿命急剧缩短、光谱红移、荧光和磷光发射猝灭以及ANS结合的调制。从甘油作为共溶剂提供的完全保护,或适度浓度尿素引起的显著增强来看,这些扰动的驱动力似乎是压力诱导的蛋白质水合作用。非弹性构象变化伴随着酶活性缓慢且往往不完全的恢复。根据滞后现象和解离平衡中亚基亲和力的变化,讨论了这些过程的特征时间、它们的压力依赖性以及缓慢的、热激活的可逆性。

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