An algorithm for finding protein–DNA binding sites with applications to chromatin- immunoprecipitati...
An algorithm for finding protein–DNA binding sites with applications to chromatin- immunoprecipitation microarray experiments
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London: Nature Publishing Group UK
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English
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London: Nature Publishing Group UK
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Chromatin immunoprecipitation followed by cDNA microarray hybridization (ChIP–array) has become a popular procedure for studying genome-wide protein–DNA interactions and transcription regulation. However, it can only map the probable protein–DNA interaction loci within 1–2 kilobases resolution. To pinpoint interaction sites down to the base-pair level, we introduce a computational method, Motif Discovery scan (MDscan), that examines the ChIP–array-selected sequences and searches for DNA sequence motifs representing the protein–DNA interaction sites. MDscan combines the advantages of two widely adopted motif search strategies, word enumeration
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and position-specific weight matrix updating
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, and incorporates the ChIP–array ranking information to accelerate searches and enhance their success rates. MDscan correctly identified all the experimentally verified motifs from published ChIP–array experiments in yeast
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(STE12, GAL4, RAP1, SCB, MCB, MCM1, SFF, and SWI5), and predicted two motif patterns for the differential binding of Rap1 protein in telomere regions. In our studies, the method was faster and more accurate than several established motif-finding algorithms
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. MDscan can be used to find DNA motifs not only in ChIP–array experiments but also in other experiments in which a subgroup of the sequences can be inferred to contain relatively abundant motif sites. The MDscan web server can be accessed at
http://BioProspector.stanford.edu/MDscan/
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An algorithm for finding protein–DNA binding sites with applications to chromatin- immunoprecipitation microarray experiments
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TN_cdi_proquest_miscellaneous_71960618
Permalink
https://devfeature-collection.sl.nsw.gov.au/record/TN_cdi_proquest_miscellaneous_71960618
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ISSN
1087-0156
E-ISSN
1546-1696
DOI
10.1038/nbt717