Genomics

Dataset Information

0

Transcriptomic insights into the roles of the transcription factors Clr1, Clr2 and Clr4 in lignocellulose degradation of the thermophilic fungal platform Thermothelomyces thermophilus

ABSTRACT: Thermothelomyces thermophilus, formerly known as Myceliophthora thermophila, is used in industry to produce lignocellulolytic enzymes and heterologous proteins. However, the transcriptional network driving the expression of these proteins remains elusive. As a first step to systematically uncover this network, we investigated growth, protein secretion, and transcriptomic fingerprints of strains deficient in the cellulolytic transcriptional regulators Clr1, Clr2, and Clr4, respectively. The genes encoding Clr1, Clr2, and Clr4 were individually deleted using split marker or the CRISPR/Cas12a technology and the resulting strains as well as the parental strain were cultivated in bioreactors under chemostat conditions using glucose as carbon source. During steady state conditions, cellulose was added instead of glucose to study the genetic and cellular responses in all four strains to the shift in carbon source availability. Notably, the clr1 and clr2 deletion strains were unable to continue to grow on cellulose, demonstrating a key role of both regulators in cellulose catabolism. Their transcriptomic fingerprints uncovered not only a lack of cellulase gene expression but also reduced expression of genes predicted to encode hemicellulases, pectinases, and esterases. In contrast, the growth of the clr4 deletion strain was very similar compared to the parental strain. However, a much stronger expression of cellulases, hemicellulases, pectinases, and esterases was observed. The data gained in this study suggest that both transcriptional regulators Clr1 and Clr2 activate the expression of genes predicted to encode cellulases as well as hemicellulases, pectinases, and esterases. They further suggest that Clr1 controls the basal expression of cellulases and initiates the main lignocellulolytic response to cellulose via induction of clr2 expression. In contrast, Clr4 seems to act as a repressor of the lignocellulolytic response presumably via controlling clr2 expression. Comparative transcriptomics in all four strains revealed potentially new regulators in carbohydrate catabolism and lignocellulolytic enzyme expression that define a candidate gene list for future analyses.

ORGANISM(S): Thermothelomyces thermophilus

PROVIDER: GSE183387 | GEO | 2021/12/15

REPOSITORIES: GEO

Json Xml

Similar Datasets

Transcriptomics Transcriptomic analysis of cellulolytic fungus Penicillium decumbens strains in response to different carbon sources
2013-01-18 | GSE34288 | GEO
Transcriptomics Transcriptomes of Aspergillus fumigatus Z5 induced by different carbon sources
2015-11-22 | GSE55086 | GEO
Transcriptomics Transcriptomes of Aspergillus fumigatus Z5 induced by different carbon sources
2015-11-22 | E-GEOD-55086 | biostudies-arrayexpress
Transcriptomics Transcriptional landscape of XYR1 in Trichoderma reesei during the degradation of cellulosic material
2017-02-09 | GSE66982 | GEO
Transcriptomics Decoding the black box of cellulase formation in Hypocrea jecorina by RNA-Seq analysis
2014-04-01 | GSE53629 | GEO
Proteomics Cellulose and hemicellulose decomposition by forest soil bacteria proceeds by the action of structurally variable enzymatic systems
2016-05-02 | PXD003844 | Pride
Transcriptomics Growth, enzymatic, and transcriptomic analysis of xyr1 deletion reveals a major regulator of plant biomass-degrading enzymes in Trichoderma harzianum
2023-12-26 | GSE252008 | GEO
Proteomics Insight into enzymatic degradation of corn, wheat, and soybean cell wall cellulose using quantitative secretome analysis of Aspergillus fumigatus
2016-09-29 | PXD004670 | Pride
Genomics ArrayCGH of Trichoderma reesei strains QM9123, QM9414, NG14 and RutC-30
2010-11-26 | GSE19606 | GEO
Transcriptomics Aspergillus niger : Control (fructose) vs. xylose + arabinose (XA)
2012-05-07 | GSE37760 | GEO