Sample Summary Breast vHMEC Summary Track Settings

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Roadmap Epigenome Breast vHMEC Summary for 12 assay type(s)

Track collection: Sample Summary

Description

All tracks in this collection (213)

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Bv DGF 35 06

UW Breast vHMEC Digital Genomic Footprinting Donor RM035 Library DGF.DS18406 EA Release 9

Data format

Bv DNase 35 06

Breast vHMEC DNase Hypersensitivity Raw Signal from REMC/UW (HOTSPOT_SCORE=0.4808 Pcnt=80)

Data format

Bv DNase 35 38

Breast vHMEC DNase Hypersensitivity Raw Signal from REMC/UW (HOTSPOT_SCORE=0.4762 Pcnt=78)

Data format

Bv H3K27me3 35

Breast vHMEC H3K27me3 Signal from REMC/UCSF-UBC (Hotspot_Score=0.21 Pcnt=70)

Data format

Bv H3K36me3 35

Breast vHMEC H3K36me3 Signal from REMC/UCSF-UBC (HOTSPOT_SCORE=0.1787 Pcnt=57)

Data format

Bv H3K4me1 35 18

Breast_vHMEC H3K4me1HS2618 Histone Modification by Chip-seq Signal from REMC/UCSF (Hotspot_Score=0.3533 Pcnt=37 DonorID:RM035)

Data format

Bv H3K4me1 35 94

Breast_vHMEC H3K4me1HS1994 Histone Modification by Chip-seq Signal from REMC/UCSF (Hotspot_Score=0.2869 Pcnt=26 DonorID:RM035)

Data format

Bv H3K4me3 35 15

Breast_vHMEC H3K4me3 Histone Modification by Chip-seq Signal from REMC/UCSF (Hotspot_Score=0.5139 Pcnt=72 DonorID:RM035)

Data format

Bv H3K9me3 35 17

Breast_vHMEC H3K9me3 Histone Modification by Chip-seq Signal from REMC/UCSF (Hotspot_Score=0.1198 Pcnt=37 DonorID:RM035)

Data format

Bv Input 35 20

Breast vHMEC Histone Modification Input by Chip-seq Signal from REMC/UCSF (Hotspot_Score=0.0258 Pcnt=39 DonorID:RM035)

Data format

Bv Input 35 95

Breast vHMEC Histone Modification Input by Chip-seq Signal from REMC/UCSF (Hotspot_Score=0.019 Pcnt=33 DonorID:RM035)

Data format

Bv MeDIP 35

Breast vHMEC DNA Methylation by MeDIP-seq Signal from REMC/UCSF-UBC (Hotspot_Score=0.4648 Pcnt=95 DonorID:RM035)

Data format

Bv MRE 35

Breast vHMEC DNA Methylation by MRE-seq Signal from REMC/UCSF-UBC (DonorID:RM035)

Data format

Bv mRNA 35

Breast vHMEC mRNA-seq Signal from REMC/UCSF-UBC (DonorID:RM035)

Data format

Bv mRNA 71 61

UCSF-UBC-USC Breast vHMEC mRNA-Seq Donor RM071 Library A18761 EA Release 9

Data format

Bv smRNA 35

Breast vHMEC smRNA-seq Signal from REMC/UCSF-UBC (DonorID:RM035)

GSM:	GSM543034
biomaterial_provider:	"Tlsty Lab, University of California, San Francisco"
biomaterial_type:	"Primary Cell Culture"
cell_type:	"Variant Human Mammary Epithelial Cells"
culture_conditions:	"spilt 1:5 in MEGM medium (Lonza Inc.)"
dateUnrestricted:	2011-02-17
disease:	None
donor_age:	18
donor_ethnicity:	Caucasian
donor_health_status:	Disease-free
donor_id:	RM035
donor_sex:	Female
experiment_type:	smRNA-Seq
extraction_protocol:	"Total RNA was extracted using Trizol from Invitrogen as per manufacturer's instuctions."
extraction_protocol_smrna_enrichment:	"The small RNA fraction was separated by electrophoresis on a Novex 10% TBE-Urea gel and the fraction between approximately 14-30nt was excised. The excisd fraction was then eluted from gel fragements, followed by EtOH precipitation and was resuspended in 6.3ul."
karyotype:	46,XX,1dmin
library_generation_pcr_f_primer_sequence:	"5' AATGATACGGCGACCACCGACAGGTTCAGAGTTCTACAGTCCGA 3'"
library_generation_pcr_number_cycles:	15
library_generation_pcr_polymerase_type:	"Phusion DNA Polymerase (Hot Start), 2U/ul (from NEB)"
library_generation_pcr_primer_conc:	0.25uM
library_generation_pcr_product_isolation_protocol:	"PCR product was separated by electrophoresis on 8% TBE Novex Gel and the PCR product between 92-125bp was excised. Product was then eluted from gel fragements, followed by EtOH precipitation"
library_generation_pcr_r_primer_sequence:	"5' CAAGCAGAAGACGGCATACGA 3'"
library_generation_pcr_template:	"10ul of the first strand cDNA product was used in the PCR"
library_generation_pcr_thermocycling_program:	"98°C for 30sec; 98°C for 10sec, 60°C for 30sec, 72°C for 15sec for 15 cycles; 72°C for 5min"
markers:	NA
passage_if_expanded:	8
rna_preparation_3'_rna_adapter_ligation_protocol:	"3' RNA adapter ligation was set up with 6.3ul of purified 5' ligation product, 1.2ul of 10uM 3' RNA adapter, 1ul of 10x Ligation buffer, 1ul of T4 RNA Ligase (5U/ul from Ambion)), and 0.5ul of Rnase OUT (40U/ul from Invitrogen). The ligation reaction was incubated at 16oC overnight."
rna_preparation_3'_rna_adapter_sequence:	"5' pUCGUAUGCCGUCUUCUGCUUGidT 3' (p=phosphate, idT=inverted deoxythyidine)"
rna_preparation_5'_rna_adapter_ligation_protocol:	"5' RNA adapter ligation was set up with 6.2ul of purified small RNA fraction (14-30nt), 1.3ul of 5uM 5' RNA adapter, 1ul of 10x Ligation buffer, 1ul of T4 RNA Ligase (5U/ul from Ambion), and 0.5ul of Rnase OUT (40U/ul from Invitrogen). Ligation reaction was incubated at 16oC overnight."
rna_preparation_5'_rna_adapter_sequence:	"5' GUUCAGAGUUCUACAGUCCGACGAUC 3'"
rna_preparation_reverse_transcription_primer_sequence:	"5' CAAGCAGAAGACGGCATACGA 3'"
rna_preparation_reverse_transcription_protocol:	"To 4.5ul of purified ligated RNA, 0.5ul of 100uM Small RNA RT-Primer was added and heat denatured at 70oC for 2 mins. Sample was then placed on a rack at room temperature and the following reagents were added immediately to the sample (2.0ul of 5X First Strand Buffer, 0.65ul of 10mM dNTPs (Invitrogen), 1ul of 100mM DTT (Invitrogen) and 0.5ul of RNaseOUT (40U/ul from Invitrogen). Reaction was heated at 48oC for 3mins. 1.0ul of Superscript II RT (200U/ul from Invitrogen) was added to the reaction and was incubated at 44oC for 1 hr. After 1hr of incubation, tube was placed on ice. 12ul of DEPC water was added to the first strand cDNA product to make a final total volume of approximately 20ul."
smrna_preparation_initial_smrna_qnty:	"1000 ng"

Data format

Assembly: Human Feb. 2009 (GRCh37/hg19)

Vizhub @ Wash U built this track, and Roadmap Epigenomics Consortium is responsible for its contents.

Description

These tracks are genome-wide DNA methylation maps generated by Roadmap Epigenomics Project. Each track is collection of DNA methylation experiment data on one sample type.

DNA methylation of human DNA mostly happens on cytosine bases of CpG dinucleotides. The methylated DNA usually prevent accessibility of regulatory proteins and hampers transcription, while unmethylated DNA is usually indicative of open chromatin. The MeDIP-Seq and MRE-Seq experiments are usually performed on same sample to identify genome-wide DNA methylation pattern. MeDIP-Seq (methylated DNA immunoprecipitation and sequencing) is a ChIP-based approach utilizing antibody against methylated cytosine. This method enriches methylated DNA and high read count indicates high likelihood of underlying region is methylated. The MRE-Seq (methylation restriction enzyme sequencing) uses methylation-sensitive restriction enzymes to digest DNA, and only cut at unmethylated restriction sites. The cut restriction sites will be detected by sequencing where reads aligned to a restriction site on reference genome means the restriction site is unmethylated.

The MethylC-Seq (MethylC sequencing) uses bisulfite to convert methylated cytosines to thymines before sequencing. The percentage of reads with a T versus a C indicates the percentage methylation at the cytosine. Details can be found in this paper Lister R, et al., Nature. 2009 Nov 19;462(7271):315-22. .

RRBS (Reduced-Representation-Bisulfite-Sequencing) is similar to MethylC-seq except RRBS uses restriction enzyme to fragment the genome into fragments suitably-sized for sequencing. While RRBS produces percent methylation similar to MethylC-seq, it is limited to cytosines that are within restriction fragments of a suitable size and tend to measure CpG dense regions only. Details can be found in this paper: Meissener, A. et al., Nucleic Acids Res. 2005; 33(18): 5868-5877. .

Display conventions

Each track can be turned on/off individually. Inside each track, sub-tracks are displayed in same vertical space and are overlayed with transparent colors for contrast. All tracks displays read density data in form of wiggle plots. Number of aligned reads is counted at each base pair, and a summarized value is computed for each 20 bp interval for display. Sub-tracks sharing same space use same scale.

Methods

Experimental protocols: follow this link for experimental protocols.

Data processing: EDACC carried out data processing and quality assessment. Details are fully explained here . In brief, sequencing reads were aligned with 'Pash' program to derive read density data. The read density data is prepared into 'wiggle' format files with fixed step length of 20 bp. Data in wiggle and other formats have been deposited in NCBI Gene Expression Omnibus database for public access.

Quality control: the HotSpot was one of the methods used to assess quality of MeDIP-Seq experiments. The long track name includes a "Hotspot_Score" field indicates the percentage of sequencing reads found inside hotspot regions. The "Pcnt" field shows the percentile of current experiment score in all MeDIP-Seq experiments. This value is subject to change in next Data Release. The most comprehensive and up-to-date description on QC Metrics used by the consortium can be found here .

Release Notes

The data is combination of Release II, III, IV, V, VI, VII, VIII and IX which were mapped to human reference genome version hg19. The data is production of Roadmap Epigenomics Project.

Please follow the link for Roadmap Epigenomics data access policy

Credits

These data were generated in labs from three institutions: UCSF, UBC, UCSD as part of Roadmap Epigenomics Project.

Useful links

Roadmap Consortium project home page
NCBI Epigenomics Gateway portal to all project data in GEO database
Epigenome Data and Analysis Coordination Center/EDACC