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Probing carbohydrate product expulsion from a processive cellulase with multiple absolute binding free energy methods.采用多种绝对结合自由能方法探测持续型纤维素酶的碳水化合物产物排出。
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Applications of computational science for understanding enzymatic deconstruction of cellulose.计算科学在理解纤维素酶解中的应用。
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The O-glycosylated linker from the Trichoderma reesei Family 7 cellulase is a flexible, disordered protein.里氏木霉家族 7 号纤维素酶的 O-糖基化连接子是一种灵活的无规卷曲蛋白质。
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Mechanism of initial rapid rate retardation in cellobiohydrolase catalyzed cellulose hydrolysis.纤维素水解过程中纤维二糖水解酶初始快速速率降低的机制。
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产物结合在延伸性和非延伸性纤维素酶之间有显著差异。

Product binding varies dramatically between processive and nonprocessive cellulase enzymes.

机构信息

National Bioenergy Center, National Renewable Energy Laboratory, Golden, Colorado 80401, USA.

出版信息

J Biol Chem. 2012 Jul 13;287(29):24807-13. doi: 10.1074/jbc.M112.365510. Epub 2012 May 30.

DOI:10.1074/jbc.M112.365510
PMID:22648408
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3397907/
Abstract

Cellulases hydrolyze β-1,4 glycosidic linkages in cellulose, which are among the most prevalent and stable bonds in Nature. Cellulases comprise many glycoside hydrolase families and exist as processive or nonprocessive enzymes. Product inhibition negatively impacts cellulase action, but experimental measurements of product-binding constants vary significantly, and there is little consensus on the importance of this phenomenon. To provide molecular level insights into cellulase product inhibition, we examine the impact of product binding on processive and nonprocessive cellulases by calculating the binding free energy of cellobiose to the product sites of catalytic domains of processive and nonprocessive enzymes from glycoside hydrolase families 6 and 7. The results suggest that cellobiose binds to processive cellulases much more strongly than nonprocessive cellulases. We also predict that the presence of a cellodextrin bound in the reactant site of the catalytic domain, which is present during enzymatic catalysis, has no effect on product binding in nonprocessive cellulases, whereas it significantly increases product binding to processive cellulases. This difference in product binding correlates with hydrogen bonding between the substrate-side ligand and the cellobiose product in processive cellulase tunnels and the additional stabilization from the longer tunnel-forming loops. The hydrogen bonds between the substrate- and product-side ligands are disrupted by water in nonprocessive cellulase clefts, and the lack of long tunnel-forming loops results in lower affinity of the product ligand. These findings provide new insights into the large discrepancies reported for binding constants for cellulases and suggest that product inhibition will vary significantly based on the amount of productive binding for processive cellulases on cellulose.

摘要

纤维素酶水解纤维素中的β-1,4 糖苷键,而β-1,4 糖苷键是自然界中最普遍和稳定的键之一。纤维素酶包含许多糖苷水解酶家族,并且作为连续的或非连续的酶存在。产物抑制对纤维素酶的作用产生负面影响,但产物结合常数的实验测量差异很大,并且对于这种现象的重要性几乎没有共识。为了从分子水平上了解纤维素酶产物抑制,我们通过计算β-1,4 糖苷键与来自糖苷水解酶家族 6 和 7 的连续和非连续酶的催化结构域的产物结合部位的结合自由能,来检查产物结合对连续和非连续纤维素酶的影响。结果表明,纤维二糖与连续纤维素酶的结合强度远远大于非连续纤维素酶。我们还预测,在酶催化过程中存在于催化结构域的反应物结合部位的纤维二糖的存在对非连续纤维素酶的产物结合没有影响,而它显著增加了对连续纤维素酶的产物结合。这种产物结合的差异与底物侧配体与连续纤维素酶隧道中的纤维二糖产物之间的氢键以及较长的隧道形成环的额外稳定作用有关。非连续纤维素酶裂隙中底物和产物侧配体之间的氢键被水破坏,而缺乏长的隧道形成环导致产物配体的亲和力降低。这些发现为报道的纤维素酶结合常数的巨大差异提供了新的见解,并表明产物抑制将根据纤维素上连续纤维素酶的生产性结合量而有很大差异。