Schema for Histone Modifications - Histone modifications in embryonic tissue (8 marks, 12 tissues, 8 ages) from ChIP-seq by ENCODE 3 (UCSD/Ren)

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Database: mm10 Primary Table: encode3Ren_facial_prominence_H3K9ac_E14 Data last updated: 2019-02-10
Big Bed File Download: /gbdb/mm10/encode3/histones/ENCFF745OYR.bigBed
Item Count: 36,689
Format description: BED6+4 Peaks of signal enrichment based on pooled, normalized (interpreted) data.

field	example	description
`chrom`	chr1	Reference sequence chromosome or scaffold
`chromStart`	130462142	Start position in chromosome
`chromEnd`	130463089	End position in chromosome
`name`	Peak_13547	Name given to a region (preferably unique). Use . if no name is assigned
`score`	52	Indicates how dark the peak will be displayed in the browser (0-1000)
`strand`	.	+ or - or . for unknown
`signalValue`	8.91908	Measurement of average enrichment for the region
`pValue`	30.48171	Statistical significance of signal value (-log10). Set to -1 if not used.
`qValue`	28.03249	Statistical significance with multiple-test correction applied (FDR -log10). Set to -1 if not used.
`peak`	624	Point-source called for this peak; 0-based offset from chromStart. Set to -1 if no point-source called.

Sample Rows

chrom	chromStart	chromEnd	name	score	strand	signalValue	pValue	qValue	peak
chr1	130462142	130463089	Peak_13547	52	.	8.91908	30.48171	28.03249	624
chr1	130548096	130548576	Peak_16299	34	.	6.67706	18.48872	16.18034	164
chr1	130714615	130718153	Peak_749	417	.	47.04948	272.67102	268.34448	3197
chr1	130718270	130718610	Peak_21274	22	.	4.96502	10.35044	8.17593	175
chr1	130878038	130878528	Peak_15750	37	.	7.09438	20.38403	18.05076	291
chr1	131050614	131050963	Peak_43642	14	.	3.31001	5.11155	3.09612	209
chr1	131053118	131053378	Peak_28109	17	.	4.01930	7.21332	5.11563	103
chr1	131053562	131053806	Peak_48218	14	.	3.17225	4.84843	2.85201	119
chr1	131059281	131059738	Peak_26325	18	.	3.96404	7.91200	5.79938	281
chr1	131060866	131061283	Peak_29186	17	.	4.01294	7.20074	5.11109	309

Histone Modifications (encode3RenHistone) Track Description

Description

The ENCODE project has established an epigenomic resource for mammalian development, profiling a diverse panel of mouse tissues at eight developmental stages from 10.5 days post conception until birth.

This track set presents the results of a comprehensive study of chromatin state across these developmental stages, based on 1,128 ChiP-seq assays of 8 histone modifications in 12 tissues, performed by the laboratory of Bing Ren as part of the ENCODE Consortium, phase 3.

Histone modifications are post-translational chemical modifications (e.g. methylation, acetylation) of histone proteins present in chromatin. Histone modifications are core components of a cell's epigenome, and influence gene expression by modulating the activity of DNA sequences.

Display Conventions and Configuration

This track is a multi-view composite track that contains two data types (views). For each view, there are multiple subtracks that display individually on the browser. Instructions for configuring multi-view tracks are here. The views in this track are:

Peaks: Regions of statistically significant signal enrichment
Signal: Density graph of signal enrichment.

Peaks displayed in this track set are replicated peaks called with the Irreproducible Discovery Rate (IDR) framework These peaks are identical to those in the "replicated peaks" files on the ENCODE data portal. Signals displayed in this track correspond to the "fold change over control" files from merged replicates, reflecting the fold enrichment of ChIP signal over the input control. Data for individual replicates are available through the ENCODE portal.

Tracks are colored by histone modification. The table below list shows the assigned track color and the genomic region type and activity level characteristic of each modification.

Modification		Regions	Activity Level
H3K4me3	dark blue	promoters	active, poised
H3K4me2	royal blue	promoters, enhancers	active, poised
H3K4me1	light blue	enhancers	active, poised
H3K27ac	dark green	promoters, enhancers	active
H3K9ac	light green	promoters, enhancers	active
H3K36me3	gold	exons	active
H3K27me3	dark red	introns, intergenic	repressed
H3K9me3	light red	heterochromatin	repressed

Methods

ChIP-seq data generation

ChIP-seq experiments for all marks and tissues from E11.5 - P0 were performed as described in Shen et. al 2012 (see References below). The ChIP-seq protocol was modified slightly for all E10.5 experiments due to the low amount of input ("micro" ChIP-seq). Detailed protocols for both standard and micro ChIP-seq are available from the ENCODE project portal (see Data Access section, below).

Standard ChIP-seq (E11.5-P0) Tissue fixation & sonication, Immunoprecipitation, Library preparation.
Micro-ChIP-seq (E10.5) Tissue fixation & sonication, Immunoprecipitation & Library preparation.

ChIP-seq antibodies

A full list of antibodies used by the Ren Lab for ENCODE can be found here. The antibody catalog and lot numbers are available for each experiment on the ENCODE portal.

ChIP-seq data processing

ChIP-seq data were analyzed using a software pipeline implemented by the ENCODE Data Coordinating Center (DCC) for the ENCODE Consortium. Each step of the pipeline corresponds to a script written in the Python programming language that assembles the input files, runs external programs, and calculates quality-control metrics. The ENCODE histone ChIP-seq pipeline is among the collection of ENCODE Uniform Processing Pipelines that can be found here.

ChIP-seq peak calling

Replicated peaks were called using an approach based on Irreproducible Discovery Rate to ensure an adequate sampling of noise for subsequent replicate comparisons. Briefly, peaks were initially called at a relaxed p-value threshold of 1 x 10-2. Such relaxed peak sets were generated for each biological replicate, for the replicates pooled, and for pooled pseudoreplicates of each true replicate (each pseudoreplicate consists of half the reads sampled without replacement). Peaks from the pooled replicate set were retained in the replicated peak set if they overlapped by at least half their length (in bases) peaks from both biological replicates. Additionally, peaks that overlapped both pooled pseudoreplicates were added to the replicated peak set. In this way very strong biological replicates "rescue" peaks that were only marginal in a second replicate.

Data Access

Data from this and all phases of ENCODE are publicly available through the ENCODE portal. The specific experiments included in this track set are listed here.

Credits

Thanks to David Gorkin and Yanxiao Zhang at the Ren lab (UCSD/Ludwig Institute for Cancer Research) and Iros Barozzi of the Environmental Genomics and Systems Biology Division at the Lawrence Berkeley National Laboratory for providing this data and assisting with track development at UCSC.

References

Gorkin et al. An atlas of dynamic chromatin landscapes in the developing mouse fetus. Nature, In Press. (pre-print: doi: https://doi.org/10.1101/166652)

Sloan CA, Chan ET, Davidson JM, Malladi VS, Strattan JS, Hitz BC, Gabdank I, Narayanan AK, Ho M, Lee BT et al. ENCODE data at the ENCODE portal. Nucleic Acids Res. 2016 Jan 4;44(D1):D726-32. PMID: 26527727; PMC: PMC4702836

Shen Y, Yue F, McCleary DF, Ye Z, Edsall L, Kuan S, Wagner U, Dixon J, Lee L, Lobanenkov VV et al. A map of the cis-regulatory sequences in the mouse genome. Nature. 2012 Aug 2;488(7409):116-20. PMID: 22763441; PMC: PMC4041622