4.7 Article

The impact of hydrogen peroxide supply on LPMO activity and overall saccharification efficiency of a commercial cellulase cocktail

Journal

BIOTECHNOLOGY FOR BIOFUELS
Volume 11, Issue -, Pages -

Publisher

BMC
DOI: 10.1186/s13068-018-1199-4

Keywords

Cellulase; Lignocellulose; Lytic polysaccharide monooxygenase; LPMO; Hydrogen peroxide; Oxygen; Biofuel

Funding

  1. Research Council of Norway [226247, 221568, 256766, 257622]
  2. Norwegian University of Life Sciences
  3. EU in the framework of the Marie-Curie FP7 COFUND People Programme, through the award of an AgreenSkills fellowship [267196]
  4. French Institut National de la Recherche Agronomique (INRA)

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Background: The discovery of enzymes named lytic polysaccharide monooxygenases (LPMOs) has had a major impact on the efficiency of current commercial cellulase cocktails for saccharification of lignocellulosic biomass. However, the notion that LPMOs use molecular oxygen as a co-substrate and require two externally delivered electrons per catalytic cycle poses a challenge in the development of efficient large-scale industrial processes. Building on the recent discovery that H2O2, rather than O-2, is the co-substrate of LPMOs, we show here how cellulose degradation by the LPMO-containing commercial cellulase cocktail-Cellic (R) CTec2 can be controlled and boosted by supplying the reaction with H2O2. Results: The controlled supply of anaerobic hydrolysis reactions with H2O2 and sub-stoichiometric amounts of reductant increased apparent LPMO activity by almost two orders of magnitude compared to standard aerobic reactions utilizing O-2 and stoichiometric amounts of reductant. Improved LPMO activity was correlated with enhanced saccharification rates and yields for a model cellulosic substrate (Avicel) as well as industrial lignocellulosic substrates (sulfite-pulped Norway spruce and steam-exploded birch), although the magnitude of the effects was substrate dependent. Improvements in lignocellulose conversions were achieved at low H2O2 feeding rates (in the range of 90-600 mu M h(-1)). Tight control of LPMO reactions by controlled supply of H2O2 under anaerobic conditions was possible. Conclusion: We report saccharification rates and yields for a model substrate (Avicel) and industrial lignocellulosic substrates that, at low H2O2 feeding rates, are higher than those seen under standard aerobic conditions. In an industrial setting, controlling and supplying molecular oxygen and stoichiometric amounts of reductant are challenging. The present report shows that the use of small amounts of a liquid bulk chemical, H2O2, provides an alternative to the currently available processes, which likely is cheaper and more easy to control, while giving higher product yields.

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