boxplot and statistical analysis Search Results


boxplot comparisons of gene expression and statistical analysis  (GraphPad Software Inc)
90
GraphPad Software Inc boxplot comparisons of gene expression and statistical analysis
Boxplot Comparisons Of Gene Expression And Statistical Analysis, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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boxplots and heatmap for aqua peptides analysis  (GraphPad Software Inc)
90
GraphPad Software Inc boxplots and heatmap for aqua peptides analysis
Boxplots And Heatmap For Aqua Peptides Analysis, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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boxplots, cumulative distribution plots, and statistical analyses  (GraphPad Software Inc)
90
GraphPad Software Inc boxplots, cumulative distribution plots, and statistical analyses
Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of <t>boxplots</t> represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)
Boxplots, Cumulative Distribution Plots, And Statistical Analyses, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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boxplots, frequency distributions, and principal component analysis (pca) analyses  (SAS institute)
90
SAS institute boxplots, frequency distributions, and principal component analysis (pca) analyses
Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of <t>boxplots</t> represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)
Boxplots, Frequency Distributions, And Principal Component Analysis (Pca) Analyses, supplied by SAS institute, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 90 stars, based on 1 article reviews
boxplots, frequency distributions, and principal component analysis (pca) analyses - by Bioz Stars, 2026-03
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boxplots and statistical significance calculations  (GraphPad Software Inc)
90
GraphPad Software Inc boxplots and statistical significance calculations
Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of <t>boxplots</t> represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)
Boxplots And Statistical Significance Calculations, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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boxplots and statistical significance calculations - by Bioz Stars, 2026-03
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boxplot construction and statistical analyses  (GraphPad Software Inc)
90
GraphPad Software Inc boxplot construction and statistical analyses
Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of <t>boxplots</t> represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)
Boxplot Construction And Statistical Analyses, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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kruskal-wallis statistical test and boxplots  (GraphPad Software Inc)
90
GraphPad Software Inc kruskal-wallis statistical test and boxplots
Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of <t>boxplots</t> represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)
Kruskal Wallis Statistical Test And Boxplots, supplied by GraphPad Software Inc, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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visualization of boxplots in alpha diversity, number and abundance and the principal coordinate analysis (pcoa) plots  (OriginLab corp)
90
OriginLab corp visualization of boxplots in alpha diversity, number and abundance and the principal coordinate analysis (pcoa) plots
Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of <t>boxplots</t> represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)
Visualization Of Boxplots In Alpha Diversity, Number And Abundance And The Principal Coordinate Analysis (Pcoa) Plots, supplied by OriginLab corp, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of boxplots represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)

Journal: Epigenetics & Chromatin

Article Title: Impact of 3D genome organization, guided by cohesin and CTCF looping, on sex-biased chromatin interactions and gene expression in mouse liver

doi: 10.1186/s13072-020-00350-y

Figure Lengend Snippet: Cohesin and CTCF ChIP-seq binding strength and proximity to genes. a Box plots of normalized ChIP-seq signal for the peak sets indicated on the x -axis. Peaks with sex differential binding for cohesin ( top graph ) and CTCF (b ottom graph ) are shown. Each pair of boxplots represents the male and female ChIP-seq signal for the same set of peaks, defined by their sex bias and peak type (CAC or CNC, for ΔCohesin peaks; and CAC or Lone CTCF, for ΔCTCF peaks), as indicated below the x -axis. Peak scores were calculated by average intra-peak ChIP signal, normalized by total sequence reads per million in peak (RIPM; see “ ”). Female-biased peaks were, on average, stronger than male-biased peaks by M–W test: p ≤ 0.001 for female vs male CAC(ΔCoh), CAC(ΔCTCF), and for CNC, but not for Lone CTCF peaks. b Distance from each indicated set of cohesin and CTCF peaks to the nearest enhancer DHS. Cumulative frequency curves indicate the fraction of each group on the y -axis, within the distance in kb to the nearest enhancer DHS indicated on the x -axis. Enhancer DHS were defined based on their high ratio of the enhancer histone mark H3K4me1 over the promoter mark H3K4me3 at DHS . Sex-biased CNC peaks are closer to enhancer DHS (median distance to eDHS of 0.22 kb for male-biased CNCs and 0.12 kb for female-biased CNCs; KS pval < 0.0001 for all comparisons) than the other CTCF and cohesin peak classes (M CAC(ΔCTCF): 14.98 kb; F CAC(ΔCTCF) 13.76 kb; M Lone ΔCTCF: 13.88 kb; F Lone ΔCTCF: 7.17 kb). Female-biased CNC peaks are significantly closer to enhancer DHS than are male-biased CNC peaks ( p = 0.0351; KS t -test). Male-biased CAC(ΔCohesin) peaks were closer to enhancers than female-biased CAC(ΔCohesin) peaks ( p = 0.002; KS t -test), however, the reverse was found for CAC(ΔCTCF) peaks ( p = 0.0052; KS t -test). Distance to nearest enhancer was not significantly different between male-biased and female-biased Lone CTCF peaks ( p = 0.1068; KS t -test). P values for comparisons between male-biased and female-biased peaks of the same class are shown for each plot (KS t -test). c Distance from each indicated set of cohesin and CTCF peaks to the nearest TSS. Cumulative frequency curves indicate the fraction of each group on the y -axis within the distance in kb to the nearest TSS indicated on the x -axis. TSS for protein coding (RefSeq) and liver lncRNA genes were considered . Female-biased cohesin and CTCF peaks are closer to TSS than male-biased CTCF and cohesin peaks of the same class (significance by KS t-test is indicated at top left of each plot). Distance to the TSS was not significantly different for male-biased versus female-biased CNC peaks ( p = 0.1458; KS t -test). d Proximity of sex-biased cohesin and CTCF binding sites to sex-biased genes. Peak designations were as follows: Proximal, peaks < 20 kb from a sex-biased gene TSS; Intra-TAD, peaks within the same intra-TAD loop as a sex-biased gene; or TAD, peaks in the same TAD as a sex-biased gene. Each of these groups is mutually exclusive. TAD loop and intra-TAD loop coordinates were from the indicated references. A set of 983 sex-biased biased protein-coding genes was used in this analysis (see Additional file : Table S1 of ). e Cumulative frequency curves show the fraction of each group ( y -axis) within the distance in kb to the nearest sex-biased DHS or H3K27ac genomic region ( x -axis), based on a merged list of published sex-biased DHS and sex-biased H3K27ac ChIP-seq peaks for male and female mouse liver. For this analysis, CAC peaks with sex-biased binding of CTCF and cohesin were combined and presented as a single group [CAC (Both)]. Male-biased and female-biased CNC peaks are significantly closer to sex-biased DHS/H3K27ac than the four other peak classes ( p < 0.001; KS t -test). Female-biased CNC peaks were significantly closer to sex-biased DHS/H3K27ac than male-biased CNC peaks ( p = 0.0094; KS)

Article Snippet: Boxplots, cumulative distribution plots, and statistical analyses were implemented using GraphPad Prism 7.

Techniques: ChIP-sequencing, Binding Assay, Sequencing