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高碘酸盐氧化对葡萄糖氧化酶结构和性质的影响。

Effect of periodate oxidation on the structure and properties of glucose oxidase.

作者信息

Nakamura S, Hayashi S, Koga K

出版信息

Biochim Biophys Acta. 1976 Sep 14;445(2):294-308. doi: 10.1016/0005-2744(76)90084-x.

DOI:10.1016/0005-2744(76)90084-x
PMID:182278
Abstract

In order to elucidate the molecular structure of glucose oxidase (beta-D-glucose: oxygen 1-oxidoreductase, EC 1.1.3.4) and the roles of its carbohydrate moiety, chemical, physiochemical and immunological experiments were performed with enzyme samples before and after periodate oxidation. Hydrodynamic parameters indicated that the native enzyme was a globular protein with values of 1.21 for the frictional ratio and 43 A for the Stokes radius. The enzyme contained about 12% carbohydrate by weight, of which the main component was mannose. The periodate treatment decreased the carbohydrate content to about 40% of its original value. Slight modifications were detected in the absorbance spectrum and the content of arginyl residue. However, no significant alteration was brought about by this treatment in the catalytic parameters, immunological reactivities of the gross structure, not in the secondary and quaternary structures of the protein moity. Thermal denaturation temperature (about 72.5 degrees C) and the enthalpy of denaturation (about 450 kcal/mol) were common to the native and the periodate-oxodozed enzymes. The native was found to be quite resistant to sodium dodecyl sulfate and fairly stable to urea and heating. The periodate-oxidized enzyme was also stable to heat treatment, but it showed a diminished stability when denaturing agents were present. Kinetic analyses of the thermal inactivation processes showed that the entropy of activation was greatly decreased by the denaturing agents, especially in the case of the periodate-oxidized enzyme. It is concluded that the carbohydrate moiety of the enzyme plays a role in increasing the stability of the protein moiety, but does not directly participate in the catalytic activity, the immunological reactivity, or in maintaining the conformation of the enzyme protein.

摘要

为了阐明葡萄糖氧化酶(β-D-葡萄糖:氧1-氧化还原酶,EC 1.1.3.4)的分子结构及其碳水化合物部分的作用,对高碘酸盐氧化前后的酶样品进行了化学、物理化学和免疫学实验。流体动力学参数表明,天然酶是一种球状蛋白质,摩擦系数为1.21,斯托克斯半径为43埃。该酶含约12%(重量)的碳水化合物,其主要成分是甘露糖。高碘酸盐处理使碳水化合物含量降至其原始值的约40%。在吸收光谱和精氨酰残基含量方面检测到轻微变化。然而,这种处理在催化参数、整体结构的免疫反应性方面未引起显著改变,在蛋白质部分的二级和四级结构方面也未引起显著改变。天然酶和高碘酸盐氧化酶的热变性温度(约72.5℃)和变性焓(约450千卡/摩尔)相同。发现天然酶对十二烷基硫酸钠相当耐受,对尿素和加热相当稳定。高碘酸盐氧化酶对热处理也稳定,但在有变性剂存在时稳定性降低。热失活过程的动力学分析表明,变性剂极大地降低了活化熵,尤其是在高碘酸盐氧化酶的情况下。得出的结论是,该酶的碳水化合物部分在增加蛋白质部分的稳定性方面起作用,但不直接参与催化活性、免疫反应性或维持酶蛋白的构象。

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