Purification by affinity chromatography of glutathione reductase (EC 1.6.4.2) from Escherichia coli and characterization of such enzyme.

A M Mata, M C Pinto, J López-Barea
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引用次数: 23

Abstract

The glutathione reductase from Escherichia coli strain S33 was purified to homogeneity by a simple and fast procedure consisting of two affinity chromatography steps. After 40-80% ammonium sulfate fractionation, the enzyme was adsorbed to an N6-2'.5'-ADP-Sepharose affinity column from which it was specifically eluted by a 0-10 mM NADP+ linear gradient. The enzyme was finally purified to homogeneity after a second affinity chromatography step in a C8-ATPR-Sepharose column, from which it was eluted by means of the same NADP+ gradient. Starting from 182 g of E. coli cells, 6.9 mg of pure enzyme was obtained after a 2632-fold purification, with a total yield of 63%. The pure enzyme showed a specific activity of 361 U/mg, and its absorption spectrum was characteristic of a flavoprotein, with an A272/A450 of 7.84. The enzyme was a dimer with a molecular weight 109 000 and 40 A hydrodynamic radius. The optimum pH were 7.5 and 4.5 with NADPH and NADH, respectively, as reductants. Apparent K'm values of 16, 377, and 66 microM were determined at pH 7.5 for NADPH, NADH, and GSSG, respectively. Upon storage the enzyme was stable at pH values ranging from 7.5 to 9.5, being additionally stabilized by FAD, NADP+, dithiothreitol, or glycerol. The pure enzyme was quite heat stable, denaturing significantly only after 10 min at 70 degrees C. A marked activity loss was observed however, even at 0 degrees C, in the presence of 20 microM NADPH. The enzyme was inactivated by low concentrations of para-hydroximercuribenzoate; the sensitivity towards such mercurial was greatly enhanced after reduction of the enzyme by NADPH.

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亲和层析法纯化大肠杆菌谷胱甘肽还原酶(EC 1.6.4.2)并进行酶学表征。
采用亲和层析两步法对大肠杆菌S33株谷胱甘肽还原酶进行了纯化。40-80%硫酸铵分馏后,酶被吸附在N6-2'上。5'-ADP-Sepharose亲和柱,通过0-10 mM NADP+线性梯度特异性洗脱。在C8-ATPR-Sepharose柱上进行第二次亲和层析后,酶最终被纯化到均匀性,并通过相同的NADP+梯度洗脱。从182 g大肠杆菌细胞开始,经过2632倍纯化,得到纯酶6.9 mg,总收率为63%。纯酶比活性为361 U/mg,吸收光谱为黄素蛋白,A272/A450为7.84。酶为二聚体,分子量109 000,水动力半径40 a。以NADPH和NADH为还原剂,最适pH为7.5和4.5。在pH 7.5条件下,NADPH、NADH和GSSG的表观K值分别为16、377和66微米。储存后,酶在7.5 - 9.5的pH值范围内是稳定的,另外可以用FAD、NADP+、二硫苏糖醇或甘油来稳定。纯酶具有相当的热稳定性,在70℃下仅10分钟就明显变性。然而,即使在0℃下,在20微米NADPH存在下,也观察到明显的活性丧失。低浓度的对羟基苯甲氧苄酯使酶失活;经NADPH还原后,该酶对汞的敏感性大大提高。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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