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Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis

In Schizosaccharomyces pombe, over 90% of transcription factor genes are nonessential. Moreover, the majority do not exhibit significant growth defects under optimal conditions when deleted, complicating their functional characterization and target gene identification. Here, we systematically overex...

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Autores principales: Vachon, Lianne, Wood, Justin, Kwon, Eun-Joo Gina, Laderoute, Amy, Chatfield-Reed, Kate, Karagiannis, Jim, Chua, Gordon
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Genetics Society of America 2013
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3730917/
https://www.ncbi.nlm.nih.gov/pubmed/23695302
http://dx.doi.org/10.1534/genetics.113.150870
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author Vachon, Lianne
Wood, Justin
Kwon, Eun-Joo Gina
Laderoute, Amy
Chatfield-Reed, Kate
Karagiannis, Jim
Chua, Gordon
author_facet Vachon, Lianne
Wood, Justin
Kwon, Eun-Joo Gina
Laderoute, Amy
Chatfield-Reed, Kate
Karagiannis, Jim
Chua, Gordon
author_sort Vachon, Lianne
collection PubMed
description In Schizosaccharomyces pombe, over 90% of transcription factor genes are nonessential. Moreover, the majority do not exhibit significant growth defects under optimal conditions when deleted, complicating their functional characterization and target gene identification. Here, we systematically overexpressed 99 transcription factor genes with the nmt1 promoter and found that 64 transcription factor genes exhibited reduced fitness when ectopically expressed. Cell cycle defects were also often observed. We further investigated three uncharacterized transcription factor genes (toe1(+)–toe3(+)) that displayed cell elongation when overexpressed. Ectopic expression of toe1(+) resulted in a G1 delay while toe2(+) and toe3(+) overexpression produced an accumulation of septated cells with abnormalities in septum formation and nuclear segregation, respectively. Transcriptome profiling and ChIP-chip analysis of the transcription factor overexpression strains indicated that Toe1 activates target genes of the pyrimidine-salvage pathway, while Toe3 regulates target genes involved in polyamine synthesis. We also found that ectopic expression of the putative target genes SPBC3H7.05c, and dad5(+) and SPAC11D3.06 could recapitulate the cell cycle phenotypes of toe2(+) and toe3(+) overexpression, respectively. Furthermore, single deletions of the putative target genes urg2(+) and SPAC1399.04c, and SPBC3H7.05c, SPACUNK4.15, and rds1(+), could suppress the phenotypes of toe1(+) and toe2(+) overexpression, respectively. This study implicates new transcription factors and metabolism genes in cell cycle regulation and demonstrates the potential of systematic overexpression analysis to elucidate the function and target genes of transcription factors in S. pombe.
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spelling pubmed-37309172013-08-01 Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis Vachon, Lianne Wood, Justin Kwon, Eun-Joo Gina Laderoute, Amy Chatfield-Reed, Kate Karagiannis, Jim Chua, Gordon Genetics Investigations In Schizosaccharomyces pombe, over 90% of transcription factor genes are nonessential. Moreover, the majority do not exhibit significant growth defects under optimal conditions when deleted, complicating their functional characterization and target gene identification. Here, we systematically overexpressed 99 transcription factor genes with the nmt1 promoter and found that 64 transcription factor genes exhibited reduced fitness when ectopically expressed. Cell cycle defects were also often observed. We further investigated three uncharacterized transcription factor genes (toe1(+)–toe3(+)) that displayed cell elongation when overexpressed. Ectopic expression of toe1(+) resulted in a G1 delay while toe2(+) and toe3(+) overexpression produced an accumulation of septated cells with abnormalities in septum formation and nuclear segregation, respectively. Transcriptome profiling and ChIP-chip analysis of the transcription factor overexpression strains indicated that Toe1 activates target genes of the pyrimidine-salvage pathway, while Toe3 regulates target genes involved in polyamine synthesis. We also found that ectopic expression of the putative target genes SPBC3H7.05c, and dad5(+) and SPAC11D3.06 could recapitulate the cell cycle phenotypes of toe2(+) and toe3(+) overexpression, respectively. Furthermore, single deletions of the putative target genes urg2(+) and SPAC1399.04c, and SPBC3H7.05c, SPACUNK4.15, and rds1(+), could suppress the phenotypes of toe1(+) and toe2(+) overexpression, respectively. This study implicates new transcription factors and metabolism genes in cell cycle regulation and demonstrates the potential of systematic overexpression analysis to elucidate the function and target genes of transcription factors in S. pombe. Genetics Society of America 2013-08 /pmc/articles/PMC3730917/ /pubmed/23695302 http://dx.doi.org/10.1534/genetics.113.150870 Text en Copyright © 2013 by the Genetics Society of America Available freely online through the author-supported open access option.
spellingShingle Investigations
Vachon, Lianne
Wood, Justin
Kwon, Eun-Joo Gina
Laderoute, Amy
Chatfield-Reed, Kate
Karagiannis, Jim
Chua, Gordon
Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis
title Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis
title_full Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis
title_fullStr Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis
title_full_unstemmed Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis
title_short Functional Characterization of Fission Yeast Transcription Factors by Overexpression Analysis
title_sort functional characterization of fission yeast transcription factors by overexpression analysis
topic Investigations
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3730917/
https://www.ncbi.nlm.nih.gov/pubmed/23695302
http://dx.doi.org/10.1534/genetics.113.150870
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