Status
Public on Dec 06, 2013
Title
2-APC-iPSC-32 H3K27me3 ChIPseq
Sample type
SRA
Source name
APC-iPSC H3K27me3 ChIPseq
Characteristics
strain: 129-M2rtTA
cell type: APC-derived induced pluripotent stem cells
passage: 10-12
chip antibody: H3K27me3
chip antibody vendor: Millipore
chip antibody cat #: 07-449
chip antibody lot #: JBC1854858
Growth protocol
ES cells and iPS cells were maintained in ES cell media containing 15% FBS and 1,000 Uml-1 of LIF.MEF and APCs were cultured in DMEM supplemented with 10% FBS and penicillin/streptomycin. HPCs was freshly isolated from bone marrow
Extracted molecule
genomic DNA
Extraction protocol
1.5x108 cells were resuspended in lysis buffer and digested with micrococcal nuclease about 5 minutes at 37°C.Then, the lysate was immunoprecipitated with antibody anti-H3K4me2, anti-H3K4me3, anti-H3K27me3; meanwhile, retaining a fraction of input ‘whole-cell extract’ as sequencing control. Immunoprecipitation-enrichment of chromatin fragments were defined and the bound DNA were purified using phenol:chloroform extractions. Chiped DNA was quantified by Qubit 2.0 Fluorometer (life technologies) and Q-PCR was performed to validate the enrichment efficiency. Then the enriched DNA was sonicated to 100-500bp fragments. DNA-end was repaired to overhang a 3’-dA, then adapters was ligated to the end DNA fragments. DNA fragments about 100-300bp, were recovered and amplified to construct the sequencing library. Thirty-nine ChIP library and thirteen input controls were used for sequencing.
Library strategy
ChIP-Seq
Library source
genomic
Library selection
ChIP
Instrument model
Illumina HiSeq 2000
Description
Sample 17
Data processing
The ChIP sequencing reads were mapped to mouse reference genome (mm9/NCBI37) using Bowtie (v0.12.7) software allowing the max mismatch 3nt. And only the unique mapped reads were used. The CCAT (v3.0) software was chosen to identify the modification enriched regions (peaks). The histone ChIPseq datasets were feed to CCAT software and the corresponding input dataset were taken as negative control. The parameters were referred to the original paper (Xu et al. 2010) in that sliding widow 2000nt for the H3K27me3 modification and 500nt for the H3K4me3, H3K4me2 modification. The FDR 0.05 was taken as cutoff.
Genome Build:
H3K27me3_32_peaks.bed: mm9
Submission date
Mar 06, 2012
Last update date
May 15, 2019
Contact name
Tao Cai
Organization name
National Institute Of Biological Sciences, Beijing (NIBS)
Lab
Sequencing Facility
Street address
No. 7 Science Park Road, Zhongguancun Life Science Park
City
Beijing
ZIP/Postal code
102206
Country
China
Series (2)
GSE36292
High-throughput sequencing of sequentially reprogrammed iPS cells reveals key epigenetic modifications correlated with reduced pluripotency of iPS cells [ChIP-seq]
GSE36294
High-throughput sequencing of sequentially reprogrammed iPS cells reveals key epigenetic modifications correlated with reduced pluripotency of iPS cells
Relations
Supplementary file
Size
Download
File type/resource
GSM886507_H3K27me3_32_peaks.bed.gz
163.9 Kb
(ftp) (http)
BED
Raw data are available in SRA
Processed data provided as supplementary file