UT-Austin ChIP Track Settings

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University of Texas, Austin ChIP-chip (UT-Austin ChIP)

This track is part of a parent called 'UT-Austin ChIP'. To show other tracks of this parent, go to the UT-Austin ChIP configuration page.

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	dense	UT Myc HeLa	University of Texas, Austin ChIP-chip (c-Myc, HeLa)	schema
	dense	UT Myc Fb	University of Texas, Austin ChIP-chip (c-Myc, 2091 fibroblasts)	schema
	dense	UT Myc st-Fb	University of Texas, Austin ChIP-chip (c-Myc, FBS-stimulated 2091 fibroblasts)	schema
	dense	UT E2F4 Fb	University of Texas, Austin ChIP-chip (E2F4, 2091 fibroblasts)	schema
	dense	UT Myc HeLa Pk	University of Texas, Austin ChIP-chip (c-Myc, HeLa) Peaks	schema
	dense	UT Myc Fb Pk	University of Texas, Austin ChIP-chip (c-Myc, 2091 fibroblasts) Peaks	schema
	dense	UT Myc st-Fb Pk	University of Texas, Austin ChIP-chip (c-Myc, FBS-stimulated 2091 fibroblasts) Peaks	schema
	dense	UT E2F4 st-Fb Pk	University of Texas, Austin ChIP-chip (E2F4, 2091 fibroblasts) Peaks	schema

Data version: ENCODE Oct 2005 Freeze
Data coordinates converted via liftOver from: May 2004 (NCBI35/hg17)

Description

ChIP-chip analysis of c-Myc and E2F4 was performed using 2091 foreskin fibroblasts and HeLa cells. ChIP was carried out from normally-growing HeLa cells and from 2091 quiescent (0.1% serum FBS), as well as serum-stimulated (10% FBS, 4hrs), fibroblasts. Microarray hybridizations were performed using NimbleGen ENCODE arrays and protocols.

Display Conventions and Configuration

This annotation follows the display conventions for composite tracks. The subtracks within this annotation may be configured in a variety of ways to highlight different aspects of the displayed data. The graphical configuration options are shown at the top of the track description page, followed by a list of subtracks. To display only selected subtracks, uncheck the boxes next to the tracks you wish to hide. For more information about the graphical configuration options, click the Graph configuration help link.

Methods

Chromatin from each cell line under a given condition was cross-linked with 1% formaldehyde, sheared, precipitated with antibody, and reverse cross-linked to obtain enriched DNA fragments. ChIP material was amplified and hybridized to a NimbleGen ENCODE region array. The raw and processed files reflect fold enrichment over the mock ChIP sample, which was used as a reference in the hybridization.

Verification

Each of the four experiments has three independent biological replicates. Data from all three replicates were averaged to generate a single data file. The NimbleGen method for hit identification was used to generate the peaks at a false positive rate of <= 0.05.

Credits

These data were contributed by Jonghwan Kim, Akshay Bhinge, and Vishy Iyer from the Iyer lab at the University of Texas at Austin, in collaboration with Mike Singer, Nan Jiang, and Roland Green of NimbleGen Systems, Inc.

Reference

Kim, J., Bhinge, A., Morgan, X.C. and Iyer, V.R. Mapping DNA-protein interactions in large genomes by sequence tag analysis of genomic enrichment. Nature Methods 2, 47-53 (2005).