4.8 Article

Biofilm disruption enhances growth rate and carbohydrate-active enzyme production in anaerobic fungi

Journal

BIORESOURCE TECHNOLOGY
Volume 358, Issue -, Pages -

Publisher

ELSEVIER SCI LTD
DOI: 10.1016/j.biortech.2022.127361

Keywords

Lignocellulose; Bioprocessing; Anaerobic fungi; Biofilms; Differential expression

Funding

  1. Army Research Office [W911NF-19-1-0010]
  2. California NanoSystems Institute (CNSI) Challenge Grant Program [DE-SC0020420]
  3. U.S. Department of Energy (DOE)
  4. U.S. Department of Energy (DOE) [DE-SC0020420] Funding Source: U.S. Department of Energy (DOE)

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This study compares the impact of different culture methods on gene expression, metabolic flux, growth rate, and xylan degradation rate of anaerobic gut fungi (AGF), providing insights for future industrial scale-up of AGF utilization. The results show that AGF grown in stirred culture exhibit faster biomass degradation, but negligible differences in primary metabolic flux, suggesting a potential way to accelerate AGF biomass valorization without altering fermentation product profile.
Anaerobic gut fungi (AGF) are lignocellulose degraders that naturally form biofilms in the rumen of large herbivores and in standard culture techniques. While biofilm formation enhances biomass degradation and carbohydrate-active enzyme (CAZyme) production in some bacteria and aerobic fungi, gene expression and metabolism in AGF biofilms have not been compared to non-biofilm cultures. Here, using the tunable morphology of the non-rhizoidal AGF, Caecomyces churrovis, the impacts of biofilm formation on AGF gene expression, metabolic flux, growth rate, and xylan degradation rate are quantified to inform future industrial scale-up efforts. Contrary to previous findings, C. churrovis upregulated catabolic CAZymes in stirred culture relative to biofilm culture. Using a de novo transcriptome, 197 new transcripts with predicted CAZyme function were identified. Stirred cultures grew and degraded xylan significantly faster than biofilm-forming cultures with negligible differences in primary metabolic flux, offering a way to accelerate AGF biomass valorization without altering the fermentation product profile. The rhizoidal AGF, Neocallimastix lanati, also grew faster with stirring on a solid plant substrate, suggesting that the advantages of stirred C. churrovis cultures may apply broadly to other AGF.

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