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Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi

The Phaffia rhodozyma UCD 67-385 genome harbors a 7873 bp cluster containing DDGS, OMT, and ATPG, encoding 2-desmethy-4-deoxygadusol synthase, O-methyl transferase, and ATP-grasp ligase, respectively, of the mycosporine glutaminol (MG) biosynthesis pathway. Homozygous deletion mutants of the entire...

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Autores principales: Sepúlveda, Dionisia, Campusano, Sebastián, Moliné, Martín, Barahona, Salvador, Baeza, Marcelo, Alcaíno, Jennifer, Colabella, Fernando, Urzúa, Blanca, Libkind, Diego, Cifuentes, Víctor
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2023
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Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10057719/
https://www.ncbi.nlm.nih.gov/pubmed/36983003
http://dx.doi.org/10.3390/ijms24065930
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author Sepúlveda, Dionisia
Campusano, Sebastián
Moliné, Martín
Barahona, Salvador
Baeza, Marcelo
Alcaíno, Jennifer
Colabella, Fernando
Urzúa, Blanca
Libkind, Diego
Cifuentes, Víctor
author_facet Sepúlveda, Dionisia
Campusano, Sebastián
Moliné, Martín
Barahona, Salvador
Baeza, Marcelo
Alcaíno, Jennifer
Colabella, Fernando
Urzúa, Blanca
Libkind, Diego
Cifuentes, Víctor
author_sort Sepúlveda, Dionisia
collection PubMed
description The Phaffia rhodozyma UCD 67-385 genome harbors a 7873 bp cluster containing DDGS, OMT, and ATPG, encoding 2-desmethy-4-deoxygadusol synthase, O-methyl transferase, and ATP-grasp ligase, respectively, of the mycosporine glutaminol (MG) biosynthesis pathway. Homozygous deletion mutants of the entire cluster, single-gene mutants, and the Δddgs(−/−);Δomt(−/−) and Δomt(−/−);Δatpg(−/−) double-gene mutants did not produce mycosporines. However, Δatpg(−/−) accumulated the intermediate 4-deoxygadusol. Heterologous expression of the DDGS and OMT or DDGS, OMT, and ATPG cDNAs in Saccharomyces cerevisiae led to 4-deoxygadusol or MG production, respectively. Genetic integration of the complete cluster into the genome of the non-mycosporine-producing CBS 6938 wild-type strain resulted in a transgenic strain (CBS 6938_MYC) that produced MG and mycosporine glutaminol glucoside. These results indicate the function of DDGS, OMT, and ATPG in the mycosporine biosynthesis pathway. The transcription factor gene mutants Δmig1(−/−), Δcyc8(−/−), and Δopi1(−/−) showed upregulation, Δrox1(−/−) and Δskn7(−/−) showed downregulation, and Δtup6(−/−) and Δyap6(−/−) showed no effect on mycosporinogenesis in glucose-containing medium. Finally, comparative analysis of the cluster sequences in several P. rhodozyma strains and the four newly described species of the genus showed the phylogenetic relationship of the P. rhodozyma strains and their differentiation from the other species of the genus Phaffia.
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spelling pubmed-100577192023-03-30 Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi Sepúlveda, Dionisia Campusano, Sebastián Moliné, Martín Barahona, Salvador Baeza, Marcelo Alcaíno, Jennifer Colabella, Fernando Urzúa, Blanca Libkind, Diego Cifuentes, Víctor Int J Mol Sci Article The Phaffia rhodozyma UCD 67-385 genome harbors a 7873 bp cluster containing DDGS, OMT, and ATPG, encoding 2-desmethy-4-deoxygadusol synthase, O-methyl transferase, and ATP-grasp ligase, respectively, of the mycosporine glutaminol (MG) biosynthesis pathway. Homozygous deletion mutants of the entire cluster, single-gene mutants, and the Δddgs(−/−);Δomt(−/−) and Δomt(−/−);Δatpg(−/−) double-gene mutants did not produce mycosporines. However, Δatpg(−/−) accumulated the intermediate 4-deoxygadusol. Heterologous expression of the DDGS and OMT or DDGS, OMT, and ATPG cDNAs in Saccharomyces cerevisiae led to 4-deoxygadusol or MG production, respectively. Genetic integration of the complete cluster into the genome of the non-mycosporine-producing CBS 6938 wild-type strain resulted in a transgenic strain (CBS 6938_MYC) that produced MG and mycosporine glutaminol glucoside. These results indicate the function of DDGS, OMT, and ATPG in the mycosporine biosynthesis pathway. The transcription factor gene mutants Δmig1(−/−), Δcyc8(−/−), and Δopi1(−/−) showed upregulation, Δrox1(−/−) and Δskn7(−/−) showed downregulation, and Δtup6(−/−) and Δyap6(−/−) showed no effect on mycosporinogenesis in glucose-containing medium. Finally, comparative analysis of the cluster sequences in several P. rhodozyma strains and the four newly described species of the genus showed the phylogenetic relationship of the P. rhodozyma strains and their differentiation from the other species of the genus Phaffia. MDPI 2023-03-21 /pmc/articles/PMC10057719/ /pubmed/36983003 http://dx.doi.org/10.3390/ijms24065930 Text en © 2023 by the authors. https://creativecommons.org/licenses/by/4.0/Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Sepúlveda, Dionisia
Campusano, Sebastián
Moliné, Martín
Barahona, Salvador
Baeza, Marcelo
Alcaíno, Jennifer
Colabella, Fernando
Urzúa, Blanca
Libkind, Diego
Cifuentes, Víctor
Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi
title Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi
title_full Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi
title_fullStr Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi
title_full_unstemmed Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi
title_short Unraveling the Molecular Basis of Mycosporine Biosynthesis in Fungi
title_sort unraveling the molecular basis of mycosporine biosynthesis in fungi
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10057719/
https://www.ncbi.nlm.nih.gov/pubmed/36983003
http://dx.doi.org/10.3390/ijms24065930
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