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果糖基转移酶在弱阴离子交换树脂上的吸附平衡

Adsorption equilibrium of fructosyltransferase on a weak anion-exchange resin.

作者信息

Vanková Katarína, Antosová Monika, Polakovic Milan

机构信息

Department of Chemical and Biochemical Engineering, Institute of Chemical and Environmental Engineering, Faculty of Chemical and Food Technology, Slovak University of Technology, Radlinského 9, 81237 Bratislava, Slovakia.

出版信息

J Chromatogr A. 2007 Aug 24;1162(1):56-61. doi: 10.1016/j.chroma.2007.05.031. Epub 2007 May 16.

Abstract

The adsorption equilibrium of a glycoprotein, fructosyltransferase from Aureobasidium pullulans, on an anion-exchange resin, Sepabeads FP-DA activated with 0.1M NaOH, was investigated. The adsorption isotherms were determined at 20 degrees C in a phosphate-citrate buffer with pH 6.0 using the static method. Sodium chloride was used to adjust the ionic strength in the range from 0.0215 to 0.1215 mol dm(-3) which provided conditions varying from a weak effect of salt concentration on protein binding to its strong suppression. The equilibrium data were very well fitted by means of the steric mass-action model when the ion-exchange capacity of 290 mmol dm(-3) was obtained from independent frontal column experiments. The model fit provided the protein characteristic charge equal to 1.9, equilibrium constant 0.326, and steric factor 1.095 x 10(5).

摘要

研究了来自出芽短梗霉的糖蛋白果糖基转移酶在经0.1M NaOH活化的阴离子交换树脂Sepabeads FP - DA上的吸附平衡。采用静态法在20℃、pH 6.0的磷酸盐 - 柠檬酸盐缓冲液中测定吸附等温线。使用氯化钠将离子强度调节至0.0215至0.1215 mol dm(-3)的范围,该范围提供了从盐浓度对蛋白质结合的弱影响到强抑制的不同条件。当通过独立的前沿柱实验获得290 mmol dm(-3)的离子交换容量时,平衡数据通过空间位阻质量作用模型得到了很好的拟合。该模型拟合得出蛋白质特征电荷等于1.9、平衡常数0.326和空间位阻因子1.095×10(5)。

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