Literature DB >> 24818689

Direct involvement of the CreA transcription factor in penicillin biosynthesis and expression of the pcbAB gene in Penicillium chrysogenum.

Cristina Cepeda-García1, Rebeca Domínguez-Santos, Ramón O García-Rico, Carlos García-Estrada, Angela Cajiao, Francisco Fierro, Juan Francisco Martín.   

Abstract

The transcription factor CreA is the main regulator responsible for carbon repression in filamentous fungi. CreA is a wide domain regulator that binds to regulatory elements in the promoters of target genes to repress their transcription. Penicillin biosynthesis and the expression of penicillin biosynthetic genes are subject to carbon repression. However, evidence of the participation of CreA in this regulation is still lacking, and previous studies on the promoter of the pcbC gene of Aspergillus nidulans indicated the lack of involvement of CreA in its regulation. Here we present clear evidence of the participation of CreA in carbon repression of penicillin biosynthesis and expression of the pcbAB gene, encoding the first enzyme of the pathway, in Penicillium chrysogenum. Mutations in cis of some of the putative CreA binding sites present in the pcbAB gene promoter fused to a reporter gene caused an important increase in the measured enzyme activity in glucose-containing medium, whereas activity in the medium with lactose was not affected. An RNAi strategy was used to attenuate the expression of the creA gene. Transformants expressing a small interfering RNA for creA showed higher penicillin production, and this increase was more evident when glucose was used as carbon source. These results confirm that CreA plays an important role in the regulation of penicillin biosynthesis in P. chrysogenum and opens the possibility of its utilization to improve the industrial production of this antibiotic.

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Year:  2014        PMID: 24818689     DOI: 10.1007/s00253-014-5760-1

Source DB:  PubMed          Journal:  Appl Microbiol Biotechnol        ISSN: 0175-7598            Impact factor:   4.813


  22 in total

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Review 3.  Key role of LaeA and velvet complex proteins on expression of β-lactam and PR-toxin genes in Penicillium chrysogenum: cross-talk regulation of secondary metabolite pathways.

Authors:  Juan F Martín
Journal:  J Ind Microbiol Biotechnol       Date:  2016-08-26       Impact factor: 3.346

Review 4.  Overview of carbon and nitrogen catabolite metabolism in the virulence of human pathogenic fungi.

Authors:  Laure Nicolas Annick Ries; Sarah Beattie; Robert A Cramer; Gustavo H Goldman
Journal:  Mol Microbiol       Date:  2017-12-29       Impact factor: 3.501

5.  Carbon regulation of environmental pH by secreted small molecules that modulate pathogenicity in phytopathogenic fungi.

Authors:  Fangcheng Bi; Shiri Barad; Dana Ment; Neta Luria; Amit Dubey; Virginia Casado; Nofar Glam; Jose Diaz Mínguez; Eduardo A Espeso; Robert Fluhr; Dov Prusky
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Review 6.  Penicillium chrysogenum, a Vintage Model with a Cutting-Edge Profile in Biotechnology.

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7.  Secondary metabolite gene clusters in the entomopathogen fungus Metarhizium anisopliae: genome identification and patterns of expression in a cuticle infection model.

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Journal:  BMC Genomics       Date:  2016-10-25       Impact factor: 3.969

8.  Proteomic analysis of the signaling pathway mediated by the heterotrimeric Gα protein Pga1 of Penicillium chrysogenum.

Authors:  Ulises Carrasco-Navarro; Rosario Vera-Estrella; Bronwyn J Barkla; Eduardo Zúñiga-León; Horacio Reyes-Vivas; Francisco J Fernández; Francisco Fierro
Journal:  Microb Cell Fact       Date:  2016-10-06       Impact factor: 5.328

9.  Filamentous fungal carbon catabolite repression supports metabolic plasticity and stress responses essential for disease progression.

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Journal:  PLoS Pathog       Date:  2017-04-19       Impact factor: 6.823

Review 10.  Regulators of plant biomass degradation in ascomycetous fungi.

Authors:  Tiziano Benocci; Maria Victoria Aguilar-Pontes; Miaomiao Zhou; Bernhard Seiboth; Ronald P de Vries
Journal:  Biotechnol Biofuels       Date:  2017-06-12       Impact factor: 6.040

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