Real-time imaging reveals that lytic polysaccharide monooxygenase promotes cellulase activity by increasing cellulose accessibility

Bo Song; Bingyao Li; Xiaoyan Wang; Wei Shen; Sungjin Park; Cynthia Collings; Anran Feng; Steve J Smith; Jonathan D Walton; Shi-You Ding

doi:10.1186/s13068-018-1023-1

Real-time imaging reveals that lytic polysaccharide monooxygenase promotes cellulase activity by increasing cellulose accessibility

Biotechnol Biofuels. 2018 Feb 15:11:41. doi: 10.1186/s13068-018-1023-1. eCollection 2018.

Authors

Bo Song^#¹, Bingyao Li^#^{1

2

3}, Xiaoyan Wang¹, Wei Shen^{1

3}, Sungjin Park¹, Cynthia Collings^{1

3}, Anran Feng¹, Steve J Smith⁴, Jonathan D Walton^{1

2

3}, Shi-You Ding^{1

3}

Affiliations

¹ 1Department of Plant Biology, Michigan State University, East Lansing, MI 48824 USA.
² 2MSU-DOE Plant Research Laboratory, Michigan State University, East Lansing, MI 48824 USA.
³ 3DOE Great Lakes Bioenergy Research Center, Michigan State University, East Lansing, MI 48824 USA.
⁴ 4Nanoscience and Nanoengineering Program, South Dakota School of Mines and Technology, Rapid City, SD 57701 USA.

^# Contributed equally.

Abstract

Background: The high cost of enzymes is one of the key technical barriers that must be overcome to realize the economical production of biofuels and biomaterials from biomass. Supplementation of enzyme cocktails with lytic polysaccharide monooxygenase (LPMO) can increase the efficiency of these cellulase mixtures for biomass conversion. The previous studies have revealed that LPMOs cleave polysaccharide chains by oxidization of the C1 and/or C4 carbons of the monomeric units. However, how LPMOs enhance enzymatic degradation of lignocellulose is still poorly understood.

Results: In this study, we combined enzymatic assays and real-time imaging using atomic force microscopy (AFM) to study the molecular interactions of an LPMO [TrAA9A, formerly known as TrCel61A) from Trichoderma reesei] and a cellobiohydrolase I (TlCel7A from T. longibrachiatum) with bacterial microcrystalline cellulose (BMCC) as a substrate. Cellulose conversion by TlCel7A alone was enhanced from 46 to 54% by the addition of TrAA9A. Conversion by a mixture of TlCel7A, endoglucanase, and β-glucosidase was increased from 79 to 87% using pretreated BMCC with TrAA9A for 72 h. AFM imaging demonstrated that individual TrAA9A molecules exhibited intermittent random movement along, across, and penetrating into the ribbon-like microfibril structure of BMCC, which was concomitant with the release of a small amount of oxidized sugars and the splitting of large cellulose ribbons into fibrils with smaller diameters. The dividing effect of the cellulose microfibril occurred more rapidly when TrAA9A and TlCel7A were added together compared to TrAA9A alone; TlCel7A alone caused no separation.

Conclusions: TrAA9A increases the accessible surface area of BMCC by separating large cellulose ribbons, and thereby enhances cellulose hydrolysis yield. By providing the first direct observation of LPMO action on a cellulosic substrate, this study sheds new light on the mechanisms by which LPMO enhances biomass conversion.

Keywords: AFM; Biomass; Biorefinery; CBH I; Cellulose; LPMO; Lignocellulose.