High Activity CAZyme Cassette for Improving Biomass Degradation in Thermophiles

Overview

Journal Biotechnol Biofuels

Publisher Biomed Central

Specialty Biotechnology

Date 2018 Feb 14

PMID 29434665

Citations 18

Authors

Roman Brunecky

Daehwan Chung

Nicholas S Sarai

Neal Hengge

Jordan F Russell

Jenna Young

Ashutosh Mittal

Patthra Pason

Todd Vander Wall

William Michener

Todd Shollenberger

Janet Westpheling

Michael E Himmel

Yannick J Bomble

Affiliations

Soon will be listed here.

Abstract

Background: Thermophilic microorganisms and their enzymes offer several advantages for industrial application over their mesophilic counterparts. For example, a hyperthermophilic anaerobe, , was recently isolated from hot springs in Kamchatka, Siberia, and shown to have very high cellulolytic activity. Additionally, it is one of a few microorganisms being considered as viable candidates for consolidated bioprocessing applications. Moreover, is capable of deconstructing plant biomass without enzymatic or chemical pretreatment. This ability is accomplished by the production and secretion of free, multi-modular and multi-functional enzymes, one of which, Cel9A/Cel48A also known as CelA, is able to outperform enzymes found in commercial enzyme preparations. Furthermore, the complete exoproteome is extremely thermostable and highly active at elevated temperatures, unlike commercial fungal cellulases. Therefore, understanding the functional diversity of enzymes in the exoproteome and how inter-molecular synergy between them confers with its high cellulolytic activity is an important endeavor to enable the production of more efficient biomass degrading enzyme formulations and in turn, better cellulolytic industrial microorganisms.

Results: To advance the understanding of the exoproteome we have expressed, purified, and tested four of the primary enzymes found in the exoproteome and we have found that the combination of three or four of the most highly expressed enzymes exhibit synergistic activity. We also demonstrated that discrete combinations of these enzymes mimic and even improve upon the activity of the whole exoproteome, even though some of the enzymes lack significant activity on their own.

Conclusions: We have demonstrated that it is possible to replicate the cellulolytic activity of the native exoproteome utilizing a minimal gene set, and that these minimal gene sets are more active than the whole exoproteome. In the future, this may lead to more simplified and efficient cellulolytic enzyme preparations or yield improvements when these enzymes are expressed in microorganisms engineered for consolidated bioprocessing.

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