Accession | CRX017981 |
Organism | Mus musculus |
Title | 4-cell R3 |
BioProject | PRJCA000241 |
BioSample | SAMC013114 |
Platform | Illumina HiSeq X Ten |
Library |
Library name |
Construction protocol |
Strategy |
Source |
Selection |
Layout |
|
In Situ Hi-C library generation was performed with some modification accordingto the procedures described in detail elsewhere (Rao et al., 2014). All samples were crosslinked with 1%formaldehyde at room temperature for 10 minutes. Nuclei were permeabilized. DNAwas digested with 10 units of MboI, and the ends of restriction fragments werelabeled using biotinylated nucleotides and ligated in a very small volume. Thecrosslinks, ligated DNA was pelleted, washed with 10mM Tris buffer once, thenreversed in 10mM Tris buffer and 1.25mg/ml proteinase K (Qiagen, 19133),incubated at 65°C for 5h and 75°C for 30min to inactivate the protease. The reversedDNA was sheared to a length of ~400bp, and directly treated with EndRepair/dA-Tailing Module (NEB, E7442L) and Ligation Module (NEB, E7445L).The biotin-labelled ligation junction DNA was pulled down with streptavidin beadsand amplified for 12-14 cycles. The amplification mixture was purified usingAMPURE XP beads to select size 400-600bp. The result |
OTHER |
GENOMIC |
unspecified |
PAIRED
|
|
Processing |
Planned read length (bp) for mate 1: 150
Planned read length (bp) for mate 2: 150
|
Release date | 2017-07-13 |
Run |
Run accession |
Run data file information |
File name | File size (MB) |
CRR008689 |
CRD018317
CRD018316
CRD018315
CRD018314
|
35,485.06
40,471.41
35,088.34
39,991.95
|
|
Submitter | Xuepeng Chen (chenxp@big.ac.cn) |
Organization | Beijing Institute of Genomics, Chinese Academy of Sciences |
Date submitted | 2017-05-28 |