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蒸汽预处理玉米秸秆水解过程中特定里氏木霉纤维素酶/木聚糖酶成分的吸附和酶活性谱。

The adsorption and enzyme activity profiles of specific Trichoderma reesei cellulase/xylanase components when hydrolyzing steam pretreated corn stover.

机构信息

Forest Products Biotechnology/Bioenergy Group, University of British Columbia, 2424 Main Mall, Vancouver, British Columbia, Canada V6T1Z4.

出版信息

Enzyme Microb Technol. 2012 Mar 10;50(3):195-203. doi: 10.1016/j.enzmictec.2011.12.004. Epub 2011 Dec 26.

DOI:10.1016/j.enzmictec.2011.12.004
PMID:22305175
Abstract

Recycling of enzymes during biomass conversion is one potential strategy to reduce the cost of the hydrolysis step of cellulosic ethanol production. Devising an efficient enzyme recycling strategy requires a good understanding of how the enzymes adsorb, distribute, and interact with the substrate during hydrolysis. We investigated the interaction of individual Trichoderma reesei enzymes present in a commercial cellulase mixture during the hydrolysis of steam-pretreated corn stover (SPCS). The enzyme profiles were followed using zymograms, gel electrophoresis, enzyme activity assays and mass spectrometry. The adsorption and activity profiles of 6 specific enzymes Cel7A (CBH I), Cel7B (EG I), Cel5A (EG II), Xyn 10 (endo-1,4-β-xylanase III), Xyn 11 (endo-xylanase II), and β-glucosidase were characterized. Initially, each of the enzymes rapidly adsorbed onto the SPCS. However, this was followed by partial desorption to an adsorption equilibrium where the Cel7A, Cel7B, Xyn 10, and β-glucosidase were partially adsorbed to the SPCS and also found free in solution throughout the course of hydrolysis. In contrast, the Cel5A and Xyn 11 components remained primarily free in the supernatant. The Cel7A component also exhibited a partial desorption when the rate of hydrolysis leveled off as evidenced by MUC zymogram and SDS-PAGE. Those cellulase components that did not bind to the substrate were generally less stable and lost their activities within the first 24h when compared to enzymes that were distributed in both the liquid and solid phases. Therefore, to ensure maximum enzyme activity recovery, enzyme recycling seems to be most effective when short-term rounds of hydrolysis are combined with the recovery of enzymes from both the liquid and the solid phases and potentially enzyme supplementation to replenish lost activity.

摘要

在生物质转化过程中回收酶是降低纤维素乙醇生产中水解步骤成本的一种潜在策略。设计有效的酶回收策略需要很好地了解酶在水解过程中如何吸附、分布和与底物相互作用。我们研究了存在于商业纤维素酶混合物中的单个里氏木霉酶在蒸汽预处理玉米秸秆(SPCS)水解过程中的相互作用。使用酶谱、凝胶电泳、酶活性测定和质谱法跟踪酶谱。 6 种特定酶 Cel7A(CBH I)、Cel7B(EG I)、Cel5A(EG II)、Xyn 10(内切-1,4-β-木聚糖酶 III)、Xyn 11(内切木聚糖酶 II)和β-葡萄糖苷酶的吸附和活性谱进行了表征。最初,每种酶都迅速吸附到 SPCS 上。然而,随后部分解吸到吸附平衡,其中 Cel7A、Cel7B、Xyn 10 和β-葡萄糖苷酶部分吸附到 SPCS 上,并在水解过程中始终发现游离在溶液中。相比之下,Cel5A 和 Xyn 11 成分主要仍留在上清液中。当水解速率达到平衡时,Cel7A 成分也表现出部分解吸,这一点可以从 MUC 酶谱和 SDS-PAGE 得到证明。与分布在液相和固相中的酶相比,那些没有与底物结合的纤维素酶成分通常不太稳定,并且在最初的 24 小时内失去活性。因此,为了确保最大的酶活性回收,当结合回收液相和固相中的酶以及潜在的酶补充以补充失去的活性进行短期水解循环时,酶回收似乎最为有效。

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