Ocalize around the TSS of the Hsp70Aa gene in S2 cells that have not been heat shocked, consistent with a model in which they interact to establish pausing (Figure 5G). Spt5 is recruited 10781694 to RNAP II during the transition from initiation to early elongation [44] and is involved in all transcription irrespective of promoter proximal pausing, thus it is unlikely that Spt5 recruitment is directly dependent on Pho. Pho is a sequence specific DNA binding protein [12]. However, Pho is also found spread across actively transcribed genes, including hsp70, where it is involved with re-establishing polymerase pausing after heat shock [26]. It is possible that Spt5 recruits Pho to theGene Regulation by Spt5 and PleiohomeoticFigure 5. Meta-analysis of ChIP data for Pho [22], Spt5 [25], NELF [25,31] and GAF [31] binding across the genome of Drosophila S2 cells. Asterisks denote the NELF data from [31]. A) Venn diagram showing peaks the overlap of Pho binding with Spt5. B) Heat maps shows peaks of Spt5, NELF-B and Pho binding relative to the TSS (centre of each column) for all coding genes annotated in the genome from the Ensembl database (Release 5.48). Plots show 200 bp up and downstream of the TSS. SEQMINER was used to cluster and visualise the data using the default settings (the ‘Kmeans raw’ clustering normalization method with 10 expected clusters) [60]. C) Venn diagram showing overlap of Pho and Spt5 peaks with NELF-B binding. D) Overlap of Pho peaks with peaks derived from NELF-B* and NELF-E* datasets. E) Venn diagram showing the overlap between the NELF-B peaks from [25] and NELF-B* and NELF-E* datasets from [31]. Differences in the profiles of NELF binding between these two studies may be due to the use of different antibodies and/or experimental conditions to perform ChIP-chip. F) Overlap between Pho and GAF peaks in S2 cells. Note: the total number of peaks for an individual factor can vary due to the merging of several overlapping peaks into a single peak if multiple peaks of one factor overlap with a single peak of another. G) Overlap of ChIP peaks for Spt5 and Pho binding at the Hsp70Aa gene. Note: There are differences in the publicly available track format of Spt5 (bedgraph) and Pho (smoothed wig) data, and differences in the tiling array used for the ChIP-chip experiments (Spt5: Nimblegen Henikoff_Dmel_r52_ChIP tiling design, mean probe length = 53 bp, mean Lixisenatide chemical information distance between probes = 12 bp; Pho: Affymetrix Drosophila v2.0R tiling array, probe length = 25 bp, mean distance between probes = 38 bp). doi:10.1371/journal.pone.0070184.gGene Regulation by Spt5 and Pleiohomeoticgene body of hsp70, but depletion of Spt5 is lethal to cells (Figure 4) making it difficult to evaluate the role of Spt5 in Pho recruitment. Alternatively, Pho and Spt5 may be recruited to target genes independently, but interact when recruited in close proximity. Further studies are required to determine the precise details of how Pho influences polymerase pausing, however our current knowledge of which BTZ043 factors Pho interacts with suggests that it could act by helping to tether the polymerase complex close to TSSs, and/or act by nucleosome remodelling. It has been proposed that paused polymerase is physically held by factors bound to DNA at promoters, since conditions that disrupt protein-protein and protein-DNA interactions allow transcription to run-on [45]. Furthermore, insertion of spacer sequences into the promoter of the Hsp70 gene in Drosophila does not change th.Ocalize around the TSS of the Hsp70Aa gene in S2 cells that have not been heat shocked, consistent with a model in which they interact to establish pausing (Figure 5G). Spt5 is recruited 10781694 to RNAP II during the transition from initiation to early elongation [44] and is involved in all transcription irrespective of promoter proximal pausing, thus it is unlikely that Spt5 recruitment is directly dependent on Pho. Pho is a sequence specific DNA binding protein [12]. However, Pho is also found spread across actively transcribed genes, including hsp70, where it is involved with re-establishing polymerase pausing after heat shock [26]. It is possible that Spt5 recruits Pho to theGene Regulation by Spt5 and PleiohomeoticFigure 5. Meta-analysis of ChIP data for Pho [22], Spt5 [25], NELF [25,31] and GAF [31] binding across the genome of Drosophila S2 cells. Asterisks denote the NELF data from [31]. A) Venn diagram showing peaks the overlap of Pho binding with Spt5. B) Heat maps shows peaks of Spt5, NELF-B and Pho binding relative to the TSS (centre of each column) for all coding genes annotated in the genome from the Ensembl database (Release 5.48). Plots show 200 bp up and downstream of the TSS. SEQMINER was used to cluster and visualise the data using the default settings (the ‘Kmeans raw’ clustering normalization method with 10 expected clusters) [60]. C) Venn diagram showing overlap of Pho and Spt5 peaks with NELF-B binding. D) Overlap of Pho peaks with peaks derived from NELF-B* and NELF-E* datasets. E) Venn diagram showing the overlap between the NELF-B peaks from [25] and NELF-B* and NELF-E* datasets from [31]. Differences in the profiles of NELF binding between these two studies may be due to the use of different antibodies and/or experimental conditions to perform ChIP-chip. F) Overlap between Pho and GAF peaks in S2 cells. Note: the total number of peaks for an individual factor can vary due to the merging of several overlapping peaks into a single peak if multiple peaks of one factor overlap with a single peak of another. G) Overlap of ChIP peaks for Spt5 and Pho binding at the Hsp70Aa gene. Note: There are differences in the publicly available track format of Spt5 (bedgraph) and Pho (smoothed wig) data, and differences in the tiling array used for the ChIP-chip experiments (Spt5: Nimblegen Henikoff_Dmel_r52_ChIP tiling design, mean probe length = 53 bp, mean distance between probes = 12 bp; Pho: Affymetrix Drosophila v2.0R tiling array, probe length = 25 bp, mean distance between probes = 38 bp). doi:10.1371/journal.pone.0070184.gGene Regulation by Spt5 and Pleiohomeoticgene body of hsp70, but depletion of Spt5 is lethal to cells (Figure 4) making it difficult to evaluate the role of Spt5 in Pho recruitment. Alternatively, Pho and Spt5 may be recruited to target genes independently, but interact when recruited in close proximity. Further studies are required to determine the precise details of how Pho influences polymerase pausing, however our current knowledge of which factors Pho interacts with suggests that it could act by helping to tether the polymerase complex close to TSSs, and/or act by nucleosome remodelling. It has been proposed that paused polymerase is physically held by factors bound to DNA at promoters, since conditions that disrupt protein-protein and protein-DNA interactions allow transcription to run-on [45]. Furthermore, insertion of spacer sequences into the promoter of the Hsp70 gene in Drosophila does not change th.