Abstract
BackgroundTranscription factor (TF) binding to regulatory DNA sites is a key determinant of cell identity within multi-cellular organisms and has been studied extensively in relation to site affinity and chromatin modifications. There has been a strong focus on the inference of TF-gene regulatory networks and TF-TF physical interaction networks. Here, we present a third type of TF network, the spatial network of co-localized TF binding sites within the three-dimensional genome.ResultsUsing published canonical Hi-C data and single-cell genome structures, we assess the spatial proximity of a genome-wide array of potential TF-TF co-localizations in human and mouse cell lines. For individual TFs, the abundance of occupied binding sites shows a positive correspondence with their clustering in three dimensions, and this is especially apparent for weak TF binding sites and at enhancer regions. An analysis between different TF proteins identifies significantly proximal pairs, which are enriched in reported physical interactions. Furthermore, clustering of different TFs based on proximity enrichment identifies two partially segregated co-localization sub-networks, involving different TFs in different cell types. Using data from both human lymphoblastoid cells and mouse embryonic stem cells, we find that these sub-networks are enriched within, but not exclusive to, different chromosome sub-compartments that have been identified previously in Hi-C data.ConclusionsThis suggests that the association of TFs within spatial networks is closely coupled to gene regulatory networks. This applies to both differentiated and undifferentiated cells and is a potential causal link between lineage-specific TF binding and chromosome sub-compartment segregation.
Highlights
Transcription factor (TF) binding to regulatory DNA sites is a key determinant of cell identity within multi-cellular organisms and has been studied extensively in relation to site affinity and chromatin modifications
ChIP-seq profiles for a total of 37 transcription factors in human lymphoblastoid cells (GM12878) and 22 transcription factors in mouse embryonic stem cells were obtained from either ENCODE [10] or publications listed in Additional file 1: Table S1a
Hi-C contact maps and single-cell Hi-C structures show two interaction groups of heterotypic TFs While initial analyses mainly focused on the co-localization of binding sites for individual TFs, we investigated whether there was any notable co-localization between binding sites of different TFs and whether these may be attributable to particular TF-TF interactions
Summary
Transcription factor (TF) binding to regulatory DNA sites is a key determinant of cell identity within multi-cellular organisms and has been studied extensively in relation to site affinity and chromatin modifications. Sequence-specific transcription factors (TFs) are regulatory proteins that bind DNA sequence motifs to activate or repress target genes [1,2,3,4,5,6]. In multi-cellular organisms, while there are many universal TFs that act within a wide variety of cell types, others are only active in a subset. This is especially important for the establishment and maintenance of linage-specific gene expression patterns and for defining cell identity [5, 6].
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