Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing

BACKGROUND: Short-read high-throughput DNA sequencing technologies provide new tools to answer biological questions. However, high cost and low throughput limit their widespread use, particularly in organisms with smaller genomes such as S. cerevisiae. Although ChIP-Seq in mammalian cell lines is re...

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Autores principales: Lefrançois, Philippe, Euskirchen, Ghia M, Auerbach, Raymond K, Rozowsky, Joel, Gibson, Theodore, Yellman, Christopher M, Gerstein, Mark, Snyder, Michael
Formato: Texto
Lenguaje:English
Publicado: BioMed Central 2009
Materias:
Methodology Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2656530/
https://www.ncbi.nlm.nih.gov/pubmed/19159457
http://dx.doi.org/10.1186/1471-2164-10-37
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author Lefrançois, Philippe
Euskirchen, Ghia M
Auerbach, Raymond K
Rozowsky, Joel
Gibson, Theodore
Yellman, Christopher M
Gerstein, Mark
Snyder, Michael
author_facet Lefrançois, Philippe
Euskirchen, Ghia M
Auerbach, Raymond K
Rozowsky, Joel
Gibson, Theodore
Yellman, Christopher M
Gerstein, Mark
Snyder, Michael
author_sort Lefrançois, Philippe
collection PubMed
description BACKGROUND: Short-read high-throughput DNA sequencing technologies provide new tools to answer biological questions. However, high cost and low throughput limit their widespread use, particularly in organisms with smaller genomes such as S. cerevisiae. Although ChIP-Seq in mammalian cell lines is replacing array-based ChIP-chip as the standard for transcription factor binding studies, ChIP-Seq in yeast is still underutilized compared to ChIP-chip. We developed a multiplex barcoding system that allows simultaneous sequencing and analysis of multiple samples using Illumina's platform. We applied this method to analyze the chromosomal distributions of three yeast DNA binding proteins (Ste12, Cse4 and RNA PolII) and a reference sample (input DNA) in a single experiment and demonstrate its utility for rapid and accurate results at reduced costs. RESULTS: We developed a barcoding ChIP-Seq method for the concurrent analysis of transcription factor binding sites in yeast. Our multiplex strategy generated high quality data that was indistinguishable from data obtained with non-barcoded libraries. None of the barcoded adapters induced differences relative to a non-barcoded adapter when applied to the same DNA sample. We used this method to map the binding sites for Cse4, Ste12 and Pol II throughout the yeast genome and we found 148 binding targets for Cse4, 823 targets for Ste12 and 2508 targets for PolII. Cse4 was strongly bound to all yeast centromeres as expected and the remaining non-centromeric targets correspond to highly expressed genes in rich media. The presence of Cse4 non-centromeric binding sites was not reported previously. CONCLUSION: We designed a multiplex short-read DNA sequencing method to perform efficient ChIP-Seq in yeast and other small genome model organisms. This method produces accurate results with higher throughput and reduced cost. Given constant improvements in high-throughput sequencing technologies, increasing multiplexing will be possible to further decrease costs per sample and to accelerate the completion of large consortium projects such as modENCODE.
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spelling pubmed-26565302009-03-17 Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing Lefrançois, Philippe Euskirchen, Ghia M Auerbach, Raymond K Rozowsky, Joel Gibson, Theodore Yellman, Christopher M Gerstein, Mark Snyder, Michael BMC Genomics Methodology Article BACKGROUND: Short-read high-throughput DNA sequencing technologies provide new tools to answer biological questions. However, high cost and low throughput limit their widespread use, particularly in organisms with smaller genomes such as S. cerevisiae. Although ChIP-Seq in mammalian cell lines is replacing array-based ChIP-chip as the standard for transcription factor binding studies, ChIP-Seq in yeast is still underutilized compared to ChIP-chip. We developed a multiplex barcoding system that allows simultaneous sequencing and analysis of multiple samples using Illumina's platform. We applied this method to analyze the chromosomal distributions of three yeast DNA binding proteins (Ste12, Cse4 and RNA PolII) and a reference sample (input DNA) in a single experiment and demonstrate its utility for rapid and accurate results at reduced costs. RESULTS: We developed a barcoding ChIP-Seq method for the concurrent analysis of transcription factor binding sites in yeast. Our multiplex strategy generated high quality data that was indistinguishable from data obtained with non-barcoded libraries. None of the barcoded adapters induced differences relative to a non-barcoded adapter when applied to the same DNA sample. We used this method to map the binding sites for Cse4, Ste12 and Pol II throughout the yeast genome and we found 148 binding targets for Cse4, 823 targets for Ste12 and 2508 targets for PolII. Cse4 was strongly bound to all yeast centromeres as expected and the remaining non-centromeric targets correspond to highly expressed genes in rich media. The presence of Cse4 non-centromeric binding sites was not reported previously. CONCLUSION: We designed a multiplex short-read DNA sequencing method to perform efficient ChIP-Seq in yeast and other small genome model organisms. This method produces accurate results with higher throughput and reduced cost. Given constant improvements in high-throughput sequencing technologies, increasing multiplexing will be possible to further decrease costs per sample and to accelerate the completion of large consortium projects such as modENCODE. BioMed Central 2009-01-21 /pmc/articles/PMC2656530/ /pubmed/19159457 http://dx.doi.org/10.1186/1471-2164-10-37 Text en Copyright © 2009 Lefrançois et al; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License ( (http://creativecommons.org/licenses/by/2.0) ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.
spellingShingle Methodology Article
Lefrançois, Philippe
Euskirchen, Ghia M
Auerbach, Raymond K
Rozowsky, Joel
Gibson, Theodore
Yellman, Christopher M
Gerstein, Mark
Snyder, Michael
Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing
title Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing
title_full Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing
title_fullStr Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing
title_full_unstemmed Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing
title_short Efficient yeast ChIP-Seq using multiplex short-read DNA sequencing
title_sort efficient yeast chip-seq using multiplex short-read dna sequencing
topic Methodology Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2656530/
https://www.ncbi.nlm.nih.gov/pubmed/19159457
http://dx.doi.org/10.1186/1471-2164-10-37
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