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高静水压下β-乳球蛋白溶液pH变化的原位测量。

In situ measurements of pH changes in beta-lactoglobulin solutions under high hydrostatic pressure.

作者信息

Orlien Vibeke, Olsen Karsten, Skibsted Leif H

机构信息

Food Chemistry, Department of Food Science, Faculty of Life Sciences, Copenhagen University, Rolighedsvej 30, DK-1958 Frederiksberg C, Denmark.

出版信息

J Agric Food Chem. 2007 May 30;55(11):4422-8. doi: 10.1021/jf062840o. Epub 2007 Apr 27.

DOI:10.1021/jf062840o
PMID:17461592
Abstract

A novel in situ method, in which the spectral changes of aqueous solutions under pressure are measured using optical pH indicators in a high-pressure spectrophotometer, has been developed in order to provide a quantitative description of the pressure dependence of acid/base equilibria of proteins. The self-consistent method, insensitive to compressibility, was developed for measurement of changes in pH with pressure based on alpha-naphthyl red and neutral red as these indicators were found to have pressure insensitive pKa values. The method was validated for up to 500 MPa by measurement of the pressure-dependence of the weak acid buffers acetic acid/acetate and imidazolium/imidazole from which volumes of dissociation of DeltaV degrees = -11.2 and 3.7 mL/mol, respectively, were established. Succinic acid/hydrogensuccinate was surprisingly insensitive to pressure with DeltaV degrees = -0.9 mL/mol. For beta-lactoglobulin B in an unbuffered aqueous solution with ionic strength of 0.05 M and pH 4, pressure up to 300 MPa increased pH up to 1.5 units depending on concentration (up to 5 mg/mL investigated), followed by a decrease to the initial pH 4 for pressure up to 500 MPa. The surprising increase in pH at pressure up to 300 MPa is suggested to be caused by an increase in the effective pKa values of aspartic acid and glutamic acid side chain in hydrophobic compartments of the protein created by pressure denaturation, leading to a binding of water protons and an increase in free hydroxide ions. For higher pressure the carboxylic side chains in the fully denatured protein again becomes exposed to the solvent, and pH decreases to the initial pH of the aqueous system.

摘要

为了定量描述蛋白质酸碱平衡的压力依赖性,已开发出一种新颖的原位方法,该方法使用高压分光光度计中的光学pH指示剂来测量压力下水溶液的光谱变化。基于α-萘基红和中性红开发了一种对压缩性不敏感的自洽方法,用于测量pH随压力的变化,因为发现这些指示剂的pKa值对压力不敏感。通过测量弱酸缓冲液乙酸/乙酸盐和咪唑鎓/咪唑的压力依赖性,验证了该方法在高达500 MPa的压力下的有效性,由此确定了ΔV°分别为-11.2和3.7 mL/mol的解离体积。琥珀酸/氢琥珀酸盐对压力出奇地不敏感,ΔV° = -0.9 mL/mol。对于离子强度为0.05 M、pH为4的无缓冲水溶液中的β-乳球蛋白B,高达300 MPa的压力会使pH根据浓度(最高研究浓度为5 mg/mL)升高至1.5个单位,随后在高达500 MPa的压力下又降至初始pH 4。高达300 MPa压力下pH的惊人升高被认为是由于压力变性导致蛋白质疏水区域中天冬氨酸和谷氨酸侧链的有效pKa值增加,从而导致水质子结合和游离氢氧根离子增加。对于更高的压力,完全变性蛋白质中的羧基侧链再次暴露于溶剂中,pH降至水体系的初始pH。

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