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一种描述纤维素酶在气液界面失活的实验和建模方法。

An experimental and modeling approach to describe the deactivation of cellulases at the air-liquid interface.

机构信息

IFP Energies nouvelles, Solaize, France.

IFP Energies nouvelles, Rueil-Malmaison, France.

出版信息

Biotechnol Bioeng. 2024 Jun;121(6):1927-1936. doi: 10.1002/bit.28698. Epub 2024 Mar 19.

DOI:10.1002/bit.28698
PMID:38501733
Abstract

Understanding the reaction mechanisms involved in the enzymatic hydrolysis of cellulose is important because it is kinetically the most limiting step of the bioethanol production process. The present work focuses on the enzymatic deactivation at the air-liquid interface, which is one of the aspects contributing to this global deactivation. This phenomenon has already been experimentally proven, but this is the first time that a model has been proposed to describe it. Experiments were performed by incubating Celluclast cocktail solutions on an orbital stirring system at different enzyme concentrations and different surface-to-volume ratios. A 5-day follow-up was carried out by measuring the global FPase activity of cellulases for each condition tested. The activity loss was proven to depend on both the air-liquid surface area and the enzyme concentration. Both observations suggest that the loss of activity takes place at the air-liquid surface, the total amount of enzymes varying with volume or enzyme concentration. Furthermore, tests performed using five individual enzymes purified from a Trichoderma reesei cocktail showed that the only cellulase that is deactivated at the air-liquid interface is cellobiohydrolase II. From the experimental data collected by varying the initial enzyme concentration and the ratio surface to volume, it was possible to develop, for the first time, a model that describes the loss of activity at the air-liquid interface for this configuration.

摘要

了解纤维素酶水解过程中涉及的反应机制很重要,因为它是生物乙醇生产过程中动力学上最受限制的步骤。本工作重点研究了在气液界面处的酶失活,这是导致这种整体失活的因素之一。这种现象已经在实验中得到证实,但这是首次提出模型来描述它。实验是通过在不同酶浓度和不同的表面积与体积比的轨道搅拌系统中孵育 Celluclast 酶混合物溶液来进行的。通过测量每种测试条件下的纤维素酶的整体 FPase 活性,进行了为期 5 天的跟踪。证明活性损失取决于气液表面积和酶浓度。这两个观察结果表明,活性损失发生在气液表面,随着体积或酶浓度的变化,酶的总量也随之变化。此外,使用从 Trichoderma reesei 酶混合物中纯化的五种单个酶进行的测试表明,唯一在气液界面失活的纤维素酶是纤维二糖水解酶 II。通过改变初始酶浓度和表面积与体积比收集的实验数据,首次为这种配置下描述气液界面处活性损失的模型提供了可能。

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