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糖化酶的亚位点结构与配体结合机制

Subsite structure and ligand binding mechanism of glucoamylase.

作者信息

Hiromi K, Ohnishi M, Tanaka A

出版信息

Mol Cell Biochem. 1983;51(1):79-95. doi: 10.1007/BF00215589.

Abstract
  1. The basic concept and outline of the subsite theory were described, which correlates quantitatively the subsite structure (the arrangement of subsite affinities) to the action pattern of amylases in a unified manner. 2. The subsite structures of several amylases including glucoamylase were summarized. 3. In parallel with the theoretical prediction obtained therefrom, the binding subsites of glucose, gluconolactone and linear substrates to Rhizopus glucoamylase were investigated experimentally, by using steady-state inhibition kinetics, difference absorption spectrophotometry, and fluorometric titration. 4. From several lines of evidence, it was concluded that gluconolactone, a transition state analogue, is bound at Subsite 1 (nonreducing end side) where a tryptophan residue is located. 5. The stopped-flow kinetic studies have revealed that all the ligand bindings studied consist of two-step mechanism in which a bimolecular association between the enzyme and a ligand to form a loosely bound complex (EL) followed by the unimolecular isomerization process in which EL converts to the final firmly bound EL complex. For substrates the EL may be the productive complex and the fluorescence of the tryptophan located at Subsite 1 is quenched in their isomerization process, most probably a relocation of ligand to occupy this subsite.
摘要
  1. 描述了亚位点理论的基本概念和概要,该理论以统一的方式将亚位点结构(亚位点亲和力的排列)与淀粉酶的作用模式进行了定量关联。2. 总结了包括葡糖淀粉酶在内的几种淀粉酶的亚位点结构。3. 与由此获得的理论预测并行,通过稳态抑制动力学、差示吸收分光光度法和荧光滴定法,对葡萄糖、葡糖酸内酯和线性底物与米根霉葡糖淀粉酶的结合亚位点进行了实验研究。4. 从多方面证据得出结论,过渡态类似物葡糖酸内酯结合在1号亚位点(非还原端侧),该位点有一个色氨酸残基。5. 停流动力学研究表明,所有研究的配体结合均由两步机制组成,其中酶与配体之间的双分子缔合形成松散结合的复合物(EL),随后是单分子异构化过程,其中EL转化为最终牢固结合的EL复合物。对于底物,EL可能是有活性的复合物,位于1号亚位点的色氨酸的荧光在其异构化过程中被淬灭,很可能是配体重新定位以占据该亚位点。

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