PT  - JOURNAL ARTICLE
AU  - Felipe Calzado
AU  - Mariane P. Zubieta
AU  - Gabriela F. Persinoti
AU  - Cesar Rafael Fanchini Terrasan
AU  - Marcelo V. Rubio
AU  - Fabiano J. Contesini
AU  - Fabio M. Squina
AU  - André Damasio
TI  - Comparative RNA-seq based transcriptomic analysis of &lt;em&gt;Aspergillus nidulans&lt;/em&gt; recombinant strains overproducing heterologous glycoside hydrolases
AID  - 10.1101/241273
DP  - 2018 Jan 01
TA  - bioRxiv
PG  - 241273
4099  - http://biorxiv.org/content/early/2018/08/02/241273.short
4100  - http://biorxiv.org/content/early/2018/08/02/241273.full
AB  - Filamentous fungi are important cellular factories for the production and secretion of homologous and heterologous enzymes such as carbohydrate-active enzymes. However, the regulation of protein secretion in these microorganisms requires more profound studies since the enzyme levels produced are usually below the levels required by industry for profitable processes. Genomic and transcriptomic approaches have been used to understand the overexpression and production of heterologous enzymes and their capacity to induce different cellular biological processes. To investigate this regulation, Aspergillus nidulans recombinant strains were analyzed by transcriptomics. We designed three A. nidulans recombinant strains producing the following heterologous proteins: alpha-arabinofuranosidase (AbfA), beta-glucosidase (BglC) and thermophilic mannanase (Tp-Man5). The heterologous genes abfA and bglC were highly expressed, while tp-man5 mRNA levels were low and similar to those of a reference gene. There was an indirect relationship between mRNA and protein secretion levels, suggesting that transcription is not a bottleneck for target gene expression in this system. Despite the distinct features of the recombinant proteins, 30 differentially expressed genes were common to all the recombinant strains, suggesting that these genes represent a general response to the expression of heterologous genes. We also showed that the early activation of the canonical unfolded protein response (UPR) pathway by hacA alternative splicing was normalized after 8h, except in the strain expressing BglC, suggesting either no accumulation of the BglC misfolded form or the presence of an alternative endoplasmic reticulum (ER) stress and UPR pathway. Finally, to focus our analysis on the secretion pathway, a set of 374 genes was further evaluated. Seventeen genes were common to all the recombinant strains, suggesting again that these genes represent a general response of A. nidulans cells to the overexpression of recombinant genes, even thermophilic genes. Additionally, we reported the possible genetic interactions of these 17 genes based on coexpression network calculations. Interestingly, protein improvements are nongeneric, and improvements in the production of one target protein are not necessarily transferable to another one. Thus, this study may provide genetic and cellular background and targets for genetic manipulation to improve protein secretion by A. nidulans.