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里氏木霉纤维二糖水解酶Cel6A和Cel7A与纤维素在平衡状态及水解过程中的动态相互作用。

Dynamic interaction of Trichoderma reesei cellobiohydrolases Cel6A and Cel7A and cellulose at equilibrium and during hydrolysis.

作者信息

Palonen H, Tenkanen M, Linder M

机构信息

VTT Biotechnology and Food Research, FIN-02044 Espoo, Finland.

出版信息

Appl Environ Microbiol. 1999 Dec;65(12):5229-33. doi: 10.1128/AEM.65.12.5229-5233.1999.

Abstract

The binding of cellobiohydrolases to cellulose is a crucial initial step in cellulose hydrolysis. In the search for a detailed understanding of the function of cellobiohydrolases, much information concerning how the enzymes and their constituent catalytic and cellulose-binding domains interact with cellulose and with each other and how binding changes during hydrolysis is still needed. In this study we used tritium labeling by reductive methylation to monitor binding of the two Trichoderma reesei cellobiohydrolases, Cel6A and Cel7A (formerly CBHII and CBHI), and their catalytic domains. Measuring hydrolysis by high-performance liquid chromatography and measuring binding by scintillation counting allowed us to correlate activity and binding as a function of the extent of degradation. These experiments showed that the density of bound protein increased with both Cel6A and Cel7A as hydrolysis proceeded, in such a way that the adsorption points moved off the initial binding isotherms. We also compared the affinities of the cellulose-binding domains and the catalytic domains to the affinities of the intact proteins and found that in each case the affinity of the enzyme was determined by the linkage between the catalytic and cellulose-binding domains. Desorption of Cel6A by dilution of the sample showed hysteresis (60 to 70% reversible); in contrast, desorption of Cel7A did not show hysteresis and was more than 90% reversible. These findings showed that the two enzymes differ with respect to the reversibility of binding.

摘要

纤维二糖水解酶与纤维素的结合是纤维素水解过程中至关重要的起始步骤。在深入探究纤维二糖水解酶功能的过程中,仍需要大量关于这些酶及其组成的催化结构域和纤维素结合结构域如何与纤维素相互作用、如何彼此相互作用以及在水解过程中结合如何变化的信息。在本研究中,我们通过还原甲基化进行氚标记,以监测里氏木霉的两种纤维二糖水解酶Cel6A和Cel7A(以前称为CBHII和CBHI)及其催化结构域的结合情况。通过高效液相色谱法测定水解程度,通过闪烁计数法测定结合情况,使我们能够将活性和结合与降解程度关联起来。这些实验表明,随着水解的进行,Cel6A和Cel7A的结合蛋白密度均增加,吸附点偏离初始结合等温线。我们还比较了纤维素结合结构域和催化结构域的亲和力与完整蛋白的亲和力,发现每种情况下酶的亲和力均由催化结构域和纤维素结合结构域之间的连接决定。通过稀释样品对Cel6A进行解吸显示出滞后现象(60%至70%可逆);相比之下,Cel7A的解吸未显示滞后现象,且可逆性超过90%。这些发现表明,这两种酶在结合的可逆性方面存在差异。

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Widely different off rates of two closely related cellulose-binding domains from Trichoderma reesei.
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