Description
This track was produced as part of the ENCODE Project.
It shows the locations of protein factor
mediated chromatin interactions determined by
Chromatin Interaction Analysis with Paired-End Tag (ChIA-PET) data
(Fullwood et al., 2010)
extracted from five different human cancer cell lines
(K562 (chronic myeloid leukemia), HCT116 (colorectal cancer),
HeLa-S3 (cervical cancer), MCF-7 (breast cancer), and NB4
(promyelocytic)). A chromatin interaction is
defined as the association of two regions of the genome that are
far apart in terms of genomic distance, but are
spatially proximate to each other in
the 3-dimensional cellular nucleus.
Additionally, ChIA-PET experiments generate
transcription factor binding sites. A binding site
is defined as a region of the genome
that is highly enriched by specific Chromatin
ImmunoPrecipitation (ChIP) against a transcription
factor, which indicates that the transcription
factor binds specifically to this region.
The protein factors displayed in the track
include estrogen receptor alpha (ERα), RNA polymerase II (RNAPII),
and CCCTC binding factor (CTCF).
Display Conventions and Configuration
In the graphical display, the PETs are
represented by two blocks one for each end.
These blocks are connected by a horizontal
line if both ends are in the same chromosome.
If the two ends are on different chromosomes, only
one block will display.
PET sequences that overlap at both ends form
PET clusters. The number of PETs in a cluster reflects
the strength of a chromatin interaction.
Singleton PETs (PETs without a cluster) are
potentially false positives, whereas PET clusters of
more than 3 PETs could indicate genuine
chromatin interactions. The density graph of the
tags shows the ChIP enrichment at different points
of genome, and high peaks indicate transcription
factor binding sites.
Instructions for configuring multi-view tracks are
here.
To show only selected subtracks, uncheck the boxes next to the tracks that
you wish to hide.
- Interactions
- ChIA-PET Chromatin Interaction PET clusters:
Two different genomic regions in the chromatin are
genomically far from each other or in different
chromosomes, but are spatially close to each
other in the nucleus and interact with each
other for regulatory functions.
BED12 format is used to represent the data.
- Signal
- Density graph (wiggle) of signal enrichment based on aligned read density.
Metadata for a particular subtrack can be found
by clicking the down arrow in the list of subtracks.
Methods
Chromatin interaction analysis with paired-end tag
sequencing (ChIA-PET) is a global de novo
high-throughput method for characterizing the 3-dimensional
structure of chromatin in the nucleus. In the
ChIA-PET protocol, samples were cross-linked and
fragmented, then subjected to chromatin immunoprecipitation.
The DNA fragments that were brought together
by the chromatin interactions were then
proximity-ligated. During this proximity-ligation
step, the half-linkers (created by the
fragmentation) containing flanking
MmeI sites (type IIS restriction enzymes) were
first ligated to the DNA fragments and then
ligated to each other to form full
linkers. Full linkers bridge either two ends of a
self-circularized fragment, or two ends of two
different chromatin fragments. The material was
then reverse cross-linked, purified and digested
with MmeI. MmeI cuts 20 base pairs away from its
recognition site. Tag-linker-tag (paired-end
tag, PET) constructs were sequenced by ultra-high-throughput
methods (Illumina or SOLiD paired-end sequencing).
ChIA-PET reads were processed with
the ChIA-PET Tool (Li et al., 2010)
by the following steps: linker filtering,
short reads mapping, PET classification, binding site
identification, and interaction cluster identification.
The high-confidence binding sites and
chromatin interaction clusters were reported.
Verification
Chromatin interactions identified by ChIA-PET have been
validated by 3C, ChIP-3C, 4C and DNA-FISH (Fullwood et al., 2009).
Credits
Genome Institute of Singapore: Guoliang Li, Xiaoan Ruan, Kuljeet Singh Sandhu, Fabianus Hendriyan Mulawadi, Huay Mei Poh, Yufen Goh, Su Qin Peh, Wing-Kin Sung, Yijun Ruan
Stanford University: Raymond Auerbach, Michael Snyder
Contact:
Yijun Ruan
References
Fullwood MJ, Han Y, Wei CL, Ruan X, Ruan Y.
Chromatin interaction analysis using paired-end tag sequencing.
Curr Protoc Mol Biol. 2010 Jan;Chapter 21:Unit 21.15.1-25.
Fullwood MJ, Liu MH, Pan YF, Liu J, Xu H, Mohamed YB, Orlov YL, Velkov S, Ho A, Mei PH et al.
An oestrogen-receptor-alpha-bound human chromatin interactome.
Nature. 2009 Nov 5;462(7269):58-64.
Li G, Fullwood MJ, Xu H, Mulawadi FH, Velkov S, Vega V, Ariyaratne PN, Mohamed YB, Ooi HS, Tennakoon C et al.
ChIA-PET tool for comprehensive chromatin interaction analysis with paired-end tag sequencing.
Genome Biol. 2010;11(2):R22.
Publications
Li G, Ruan X, Auerbach RK, Sandhu KS, Zheng M, Wang P, Poh HM, Goh Y, Lim J, Zhang J et al.
Extensive promoter-centered chromatin interactions provide a topological basis for transcription regulation.
Cell. 2012 Jan 20;148(1-2):84-98.
Data Release Policy
Data users may freely use ENCODE data, but may not, without prior
consent, submit publications that use an unpublished ENCODE dataset until
nine months following the release of the dataset. This date is listed in
the Restricted Until column, above. The full data release policy
for ENCODE is available
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