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Titlebook: Computational Biology of Transcription Factor Binding; Istvan Ladunga Book 2010 Springer Science+Business Media, LLC 2010 Annotation.ChIP-

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2.1.1.3.2 Symmetry of a surface layer, with specific DNA motifs in the control regions of the genes that they regulate. Upon binding to DNA, and through specific protein–protein interactions, these regulatory proteins convey signals to the basal transcriptional machinery, containing the respective RNA polymerases, resulting in particula
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2.1.1.3.2 Symmetry of a surface layer,ory elements, on the DNA are footprints for the .-acting proteins involved in transcription, either for the positioning of the basic transcriptional machinery or for the regulation – in simple terms turn on or turn off – thereof. The basic transcriptional machinery is DNA-dependent RNA polymerase (R
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2.1.1.3.2 Symmetry of a surface layer, expression patterns, cell specificity and development. This chapter describes the advanced approaches to identify promoters in animal, plant and bacterial sequences. Also, we discuss an approach to identify statistically significant regulatory motifs in genomic sequences.
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X-Ray and Neutron Instrumentationffer from each other by pursuing different objectives and by taking into account different sources of information. For methods based on statistical approaches, these programs differ at an elementary level from each other by the statistical models used for individual binding sites and flanking sequen
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https://doi.org/10.1007/978-1-4757-6624-0e genome-wide transcription factor binding site and chromatin modification data produced by ChIP-seq provide invaluable information for studying gene regulation. This chapter reviews basic characteristics of ChIP-seq data and introduces a computational procedure to identify protein–DNA interactions
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Structural Studies of Inorganic Materialsatin immunoprecipitation combined by next-generation sequencing (ChIP-seq) but also in advanced statistical analyses. A fundamental issue, however, is the alarming number of false positive predictions. This problem can be remedied by improved peak calling methods of twin peaks, one at each strand of
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L. A. Feigin,D. I. Svergun,George W. Taylorf the sequences of the identified regions allows binding to be localized at a higher resolution than can be achieved by current high-throughput experiments without sequence analysis and may provide important insight into the regulatory programs enacted by the protein of interest. In this chapter we
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