Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA

DNA-binding proteins (DBPs), such as transcription factors, constitute about 10% of the protein-coding genes in eukaryotic genomes and play pivotal roles in the regulation of chromatin structure and gene expression by binding to short stretches of DNA. Despite their number and importance, only for a...

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Autores principales: Brand, Luise H., Henneges, Carsten, Schüssler, Axel, Kolukisaoglu, H. Üner, Koch, Grit, Wallmeroth, Niklas, Hecker, Andreas, Thurow, Kerstin, Zell, Andreas, Harter, Klaus, Wanke, Dierk
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2013
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3795721/
https://www.ncbi.nlm.nih.gov/pubmed/24146751
http://dx.doi.org/10.1371/journal.pone.0075177
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author Brand, Luise H.
Henneges, Carsten
Schüssler, Axel
Kolukisaoglu, H. Üner
Koch, Grit
Wallmeroth, Niklas
Hecker, Andreas
Thurow, Kerstin
Zell, Andreas
Harter, Klaus
Wanke, Dierk
author_facet Brand, Luise H.
Henneges, Carsten
Schüssler, Axel
Kolukisaoglu, H. Üner
Koch, Grit
Wallmeroth, Niklas
Hecker, Andreas
Thurow, Kerstin
Zell, Andreas
Harter, Klaus
Wanke, Dierk
author_sort Brand, Luise H.
collection PubMed
description DNA-binding proteins (DBPs), such as transcription factors, constitute about 10% of the protein-coding genes in eukaryotic genomes and play pivotal roles in the regulation of chromatin structure and gene expression by binding to short stretches of DNA. Despite their number and importance, only for a minor portion of DBPs the binding sequence had been disclosed. Methods that allow the de novo identification of DNA-binding motifs of known DBPs, such as protein binding microarray technology or SELEX, are not yet suited for high-throughput and automation. To close this gap, we report an automatable DNA-protein-interaction (DPI)-ELISA screen of an optimized double-stranded DNA (dsDNA) probe library that allows the high-throughput identification of hexanucleotide DNA-binding motifs. In contrast to other methods, this DPI-ELISA screen can be performed manually or with standard laboratory automation. Furthermore, output evaluation does not require extensive computational analysis to derive a binding consensus. We could show that the DPI-ELISA screen disclosed the full spectrum of binding preferences for a given DBP. As an example, AtWRKY11 was used to demonstrate that the automated DPI-ELISA screen revealed the entire range of in vitro binding preferences. In addition, protein extracts of AtbZIP63 and the DNA-binding domain of AtWRKY33 were analyzed, which led to a refinement of their known DNA-binding consensi. Finally, we performed a DPI-ELISA screen to disclose the DNA-binding consensus of a yet uncharacterized putative DBP, AtTIFY1. A palindromic TGATCA-consensus was uncovered and we could show that the GATC-core is compulsory for AtTIFY1 binding. This specific interaction between AtTIFY1 and its DNA-binding motif was confirmed by in vivo plant one-hybrid assays in protoplasts. Thus, the value and applicability of the DPI-ELISA screen for de novo binding site identification of DBPs, also under automatized conditions, is a promising approach for a deeper understanding of gene regulation in any organism of choice.
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spelling pubmed-37957212013-10-21 Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA Brand, Luise H. Henneges, Carsten Schüssler, Axel Kolukisaoglu, H. Üner Koch, Grit Wallmeroth, Niklas Hecker, Andreas Thurow, Kerstin Zell, Andreas Harter, Klaus Wanke, Dierk PLoS One Research Article DNA-binding proteins (DBPs), such as transcription factors, constitute about 10% of the protein-coding genes in eukaryotic genomes and play pivotal roles in the regulation of chromatin structure and gene expression by binding to short stretches of DNA. Despite their number and importance, only for a minor portion of DBPs the binding sequence had been disclosed. Methods that allow the de novo identification of DNA-binding motifs of known DBPs, such as protein binding microarray technology or SELEX, are not yet suited for high-throughput and automation. To close this gap, we report an automatable DNA-protein-interaction (DPI)-ELISA screen of an optimized double-stranded DNA (dsDNA) probe library that allows the high-throughput identification of hexanucleotide DNA-binding motifs. In contrast to other methods, this DPI-ELISA screen can be performed manually or with standard laboratory automation. Furthermore, output evaluation does not require extensive computational analysis to derive a binding consensus. We could show that the DPI-ELISA screen disclosed the full spectrum of binding preferences for a given DBP. As an example, AtWRKY11 was used to demonstrate that the automated DPI-ELISA screen revealed the entire range of in vitro binding preferences. In addition, protein extracts of AtbZIP63 and the DNA-binding domain of AtWRKY33 were analyzed, which led to a refinement of their known DNA-binding consensi. Finally, we performed a DPI-ELISA screen to disclose the DNA-binding consensus of a yet uncharacterized putative DBP, AtTIFY1. A palindromic TGATCA-consensus was uncovered and we could show that the GATC-core is compulsory for AtTIFY1 binding. This specific interaction between AtTIFY1 and its DNA-binding motif was confirmed by in vivo plant one-hybrid assays in protoplasts. Thus, the value and applicability of the DPI-ELISA screen for de novo binding site identification of DBPs, also under automatized conditions, is a promising approach for a deeper understanding of gene regulation in any organism of choice. Public Library of Science 2013-10-11 /pmc/articles/PMC3795721/ /pubmed/24146751 http://dx.doi.org/10.1371/journal.pone.0075177 Text en © 2013 Brand et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Brand, Luise H.
Henneges, Carsten
Schüssler, Axel
Kolukisaoglu, H. Üner
Koch, Grit
Wallmeroth, Niklas
Hecker, Andreas
Thurow, Kerstin
Zell, Andreas
Harter, Klaus
Wanke, Dierk
Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA
title Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA
title_full Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA
title_fullStr Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA
title_full_unstemmed Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA
title_short Screening for Protein-DNA Interactions by Automatable DNA-Protein Interaction ELISA
title_sort screening for protein-dna interactions by automatable dna-protein interaction elisa
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3795721/
https://www.ncbi.nlm.nih.gov/pubmed/24146751
http://dx.doi.org/10.1371/journal.pone.0075177
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