SUNY RIP GeneST Track Settings
 
RNA Binding Protein Associated RNA by RIP-chip GeneST from ENCODE/SUNY Albany   (ENC RNA Binding)

This track is part of a parent called 'ENC RNA Binding'. To show other tracks of this parent, go to the ENC RNA Binding configuration page.

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Minimum P-Value (-log10): (0 to 0.5)
Score range: min: (1 to 1000)
Select subtracks by antibody target and cell line: (help)
 All Antibody Target CELF1  ELAVL1  IGF2BP1  PABPC1  SLBP  T7Tag  RIP-Input 
Cell Line
GM12878 (Tier 1) 
H1-hESC (Tier 1) 
K562 (Tier 1) 
HeLa-S3 (Tier 2) 
HepG2 (Tier 2) 
List subtracks: only selected/visible    all    ()
  Cell Line↓1 Antibody Target↓2   Track Name↓3    Restricted Until↓4
 
dense
 GM12878  CELF1  GM12878 CELF1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 GM12878  ELAVL1  GM12878 ELAVL1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 GM12878  IGF2BP1  GM12878 IGF2BP1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 GM12878  PABPC1  GM12878 PABPC1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 GM12878  SLBP  GM12878 SLBP RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 GM12878  T7Tag  GM12878 T7Tag RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 GM12878  RIP-Input  GM12878 RIP-Input RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 H1-hESC  ELAVL1  H1-hESC ELAV1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-09-10 
 
dense
 H1-hESC  T7Tag  H1-hESC T7Tag RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-09-10 
 
dense
 H1-hESC  RIP-Input  H1-hESC RIP-Input RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-09-10 
 
dense
 K562  CELF1  K562 CELF1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-18 
 
dense
 K562  ELAVL1  K562 ELAVL1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 K562  PABPC1  K562 PABPC1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 K562  SLBP  K562 SLBP RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 K562  T7Tag  K562 T7Tag RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 K562  RIP-Input  K562 RIP-Input RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 HeLa-S3  ELAVL1  HeLa-S3 ELAV1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-18 
 
dense
 HeLa-S3  PABPC1  HeLa-S3 PABPC1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-18 
 
dense
 HeLa-S3  T7Tag  HeLa-S3 T7Tag RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-18 
 
dense
 HeLa-S3  RIP-Input  HeLa-S3 RIP-Input RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
 
dense
 HepG2  ELAVL1  HepG2 ELAVL1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-18 
 
dense
 HepG2  PABPC1  HepG2 PABPC1 RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-18 
 
dense
 HepG2  T7Tag  HepG2 T7Tag RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-18 
 
dense
 HepG2  RIP-Input  HepG2 RIP-Input RBP Associated RNA by RIP-chip GeneST from ENCODE/SUNY    schema   2011-03-01 
     Restriction Policy
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Data coordinates converted via liftOver from: Mar. 2006 (NCBI36/hg18)

Description

This track is produced as part of the ENCODE Project. This track displays transcriptional fragments associated with RNA binding proteins in different cell lines using RIP-Chip (Ribonomic) profiling on Affymetrix GeneChip® Human Gene 1.0 ST Arrays. These sutracks show the genomic location of transcripts associated with the array probes. Data for this track was produced as part of the Encyclopedia of DNA Elements (ENCODE) Project.

In eukaryotic organisms, gene regulatory networks require an additional level of coordination that links transcriptional and post-transcriptional processes. Messenger RNAs have traditionally been viewed as passive molecules in the pathway from transcription to translation. However, it is now clear that RNA-binding proteins play a major role in regulating multiple mRNAs in order to facilitate gene expression patterns. These tracks show the associated mRNAs that co-precipitate with the targeted RNA-binding proteins using RIP-Chip profiling.

Display Conventions and Configuration

This track has multiple subtracks that display individually in the browser. The subtracks within this track correspond to different antibodies/target proteins tested in different cell lines. These subtracks show the genomic location of the mRNA transcripts associated with RNA Binding Proteins as determined by the Affymetrix GeneChip® Human Gene 1.0 ST Array probes. Items are shaded by p-value using the formula (maxPossibleScore-((maxPossibleScore/cutOffValue)*pValue)) so that items with more significant expression levels are shaded darker. The p-values are displayed in the browser convention as -log10(pValue).

Methods

RBP-mRNA complexes were purified from cells grown according to the approved ENCODE cell culture protocols. Antibodies specific to the RNA Binding Protein (RBP) in question were first coated onto protein A/G containing magnetic beads and then used to immunoprecipitate the targeted, endogenously-formed mRNP complexes. Antibody-coated beads were incubated/tumbled with cell lysate overnight in the cold followed by extensive rinsing and subsequent purification of associated RNA using Phenol/Chloroform extraction and ethanol precipitation. The associated transcripts were identified using GeneChip® Human Gene 1.0 ST Arrays. Arrays were analyzed using Agilent's GeneSpringGX software (version 11.0).

Arrays were analyzed a group at a time by applying the Iterative PLIER16 algorithm using quantile normalization. Probesets whose normalized expression levels (signal value) fell within the 18 to 98 percentile in at least two of the three replicates were retained for further analysis. A TTest (T7-Tag and RIP-Input) or a one-way ANOVA (samples and controls) was applied to these probesets and a p-value cutoff of .05 was applied. The Benjamini-Hochberg false discovery rate algorithm was then applied to generate corrected p-values, also known as q-values.

The RIP-Input was summarized first and selected probesets were retained for further analysis. Next, the arrays for T7Tag (background/negative control) RIPs were summarized with those retained RIP-input probesets. Probesets that fit the above criteria for either group (RIP-Input or T7Tag) were then filtered for those that showed a minimum 2 fold increase of expression in T7Tag versus RIP-Input. Finally, arrays for treatment RIP samples were summarized together with those for RIP-inputs and T7Tag RIPs. Probesets that fit the above criteria for any group (RIP-Input or T7Tag or samples) were then filtered for probesets that showed a minimum 2 fold increase of expression in treatment over total. A similar list was produced for probesets showing the same enrichment in the T7Tag RIP set. Probesets which appeared in both treatment and negative control at these cutoff stringencies were subtracted from the treatment results as background noise, yielding the final data track.

Verification

All experiments (including controls) were performed in and analyzed as triplicates.

Release Notes

Release 2 (September 2011) of this track corrects the scores and the calculated P and Q values. In this release, the calculated P and Q values are -log10(P) and -log10(Q), and the scores, and therefore the shading of items, reflect the p-values as described in the Display Conventions and Configuration section above.

Credits

These data were produced and analyzed by a collaboration between the Tenenbaum lab at the University at Albany-SUNY, College of Nanoscale Science and Engineering, the Luiz Penalva group at the Greehey Children's Cancer Research Institute, University of Texas Health Science Center and the Microarray Core Facility at the Center for Functional Genomics, Rensselaer, NY .

Contact: Scott Tenenbaum

References

Baroni TE, Chittur SV, George AD, Tenenbaum SA. Advances in RIP-chip analysis : RNA-binding protein immunoprecipitation-microarray profiling. Methods Mol Biol. 2008;419:93-108.

George AD, Tenenbaum SA. MicroRNA modulation of RNA-binding protein regulatory elements. RNA Biol. 2006;3(2):57-9. Epub 2006 Apr 1.

Jain R, Devine T, George AD, Chittur SV, Baroni TE, Penalva LO, Tenenbaum SA. RNA-Binding Protein Immunoprecipitation-Microarray (Chip) Profiling. Methods Mol Biol. 2011;703:247-63

Jayaseelan S, Doyle F, Currenti S, Tenenbaum SA. RIP: An mRNA Localization Technique. Methods Mol Biol. 2011;714:407-422.

Keene JD, Tenenbaum SA. Eukaryotic mRNPs may represent posttranscriptional operons. Mol Cell. 2002;9(6):1161-7.

Penalva LO, Tenenbaum SA, Keene JD. Gene expression analysis of messenger RNP complexes. Methods Mol Biol. 2004;257:125-34.

Tenenbaum SA, Carson CC, Lager PJ, Keene JD. Identifying mRNA subsets in messenger ribonucleoprotein complexes by using cDNA arrays. Proc Natl Acad Sci U S A. 2000 Dec 19;97(26):14085-90.

Tenenbaum SA, Lager PJ, Carson CC, Keene JD. Ribonomics: identifying mRNA subsets in mRNP complexes using antibodies to RNA-binding proteins and genomic arrays. Methods. 2002 Feb;26(2):191-8.

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 here.