GIS RNA-seq Track Settings
 
RNA-seq from ENCODE/Genome Institute of Singapore   (ENC RNA-seq)

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

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 GM12878  Cytosol  PolyA+  Alignments  1  GM12878 cytosol polyA+ RNA-seq Alignments rep 1 from ENCODE/GIS    schema   2010-07-29 
 
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 GM12878  Cytosol  PolyA+  Minus Raw Signal  1  GM12878 cytosol polyA+ RNA-seq Minus raw signal rep 1 from ENCODE/GIS    schema   2010-07-29 
 
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 GM12878  Cytosol  PolyA+  Plus Raw Signal  1  GM12878 cytosol polyA+ RNA-seq Plus raw signal rep 1 from ENCODE/GIS    schema   2010-07-29 
 
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 H1-hESC  Whole Cell  PolyA+  Alignments  1  H1-hESC polyA+ RNA-seq Alignments rep 1 from ENCODE/GIS    schema   2010-07-29 
 
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 H1-hESC  Whole Cell  PolyA+  Minus Raw Signal  1  H1-hESC whole cell polyA+ RNA-seq Minus raw signal rep 1 from ENCODE/GIS    schema   2010-07-29 
 
dense
 H1-hESC  Whole Cell  PolyA+  Plus Raw Signal  1  H1-hESC whole cell polyA+ RNA-seq Plus raw signal rep 1 from ENCODE/GIS    schema   2010-07-29 
 
dense
 K562  Cytosol  PolyA+  Alignments  1  K562 cytosol polyA+ RNA-seq Alignments rep 1 from ENCODE/GIS    schema   2010-07-29 
 
dense
 K562  Cytosol  PolyA+  Alignments  2  K562 cytosol polyA+ RNA-seq Alignments rep 2 from ENCODE/GIS    schema   2010-07-29 
 
dense
 K562  Cytosol  PolyA+  Minus Raw Signal  1  K562 cytosol polyA+ RNA-seq Minus raw signal rep 1 from ENCODE/GIS    schema   2010-07-29 
 
dense
 K562  Cytosol  PolyA+  Minus Raw Signal  2  K562 cytosol polyA+ RNA-seq Minus raw signal rep 2 from ENCODE/GIS    schema   2010-07-29 
 
dense
 K562  Cytosol  PolyA+  Plus Raw Signal  1  K562 cytosol polyA+ RNA-seq Plus raw signal rep 2 from ENCODE/GIS    schema   2010-07-29 
 
dense
 K562  Cytosol  PolyA+  Plus Raw Signal  2  K562 cytosol polyA+ RNA-seq Plus raw signal rep 2 from ENCODE/GIS    schema   2010-07-29 
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Description

This track is produced as part of the ENCODE Transcriptome Project. It shows high throughput sequencing of RNA samples from tissues or sub cellular compartments from cell lines included in the ENCODE Transcriptome subproject. The overall goal of the ENCODE project is to identify and characterize all functional elements in the sequence of the human genome.

Display Conventions and Configuration

This track is a multi-view composite track that contains multiple data types (views). For each view, there are multiple subtracks that display individually on the browser. 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.

Color differences among the views are arbitrary. They provide a visual cue for distinguishing between the different cell types.

Plus Raw Signal
The Plus Raw Signal view graphs the base-by-base density of alignments on the + strand.
Minus Raw Signal
The Minus Raw Signal view graphs the base-by-base density of alignments on the - strand.
Alignments
The Alignments view shows reads mapped to the genome, both split alignments and alignments mapped to one exon. Sequences determined to be transcribed on the positive strand are shown in blue. Sequences determined to be transcribed on the negative strand are shown in red. Sequences for which the direction of transcription was not able to be determined are shown in black. For more information on the XL XJ and XU custom tags used in these files, please contact the producing lab. Please see the Bowtie Manual for more information about the SAM Bowtie output (including other tags) and the SAM Format Specification for more information on the SAM/BAM file format.

Methods

The RNA-Seq data were generated from high quality polyA RNA, and the RNA-Seq libraries were constructed using SOLiD Whole Transcriptome (WT) protocol and reagent kit. Total RNA in good quality was used as starting materials and purified twice through MACs polyT column aimed to enrich polyA and remove any contaminants (e.g., rRNA, tRNA, DNA, protein etc.). A one microgram enriched polyA RNA sample was then fragmented to small pieces, and a gel-based selection method was performed to collect fragmented random polyA at a size-range of 50-150 nt in length. The collected fragmental RNA was then hybridized and ligated to a mix of adapters provided from ABI, followed by reverse transcription to generate corresponding cDNAs. The resulting cDNA library was further amplified by PCR and sequenced by SOLiD platform for single reads at 35 bp length (new version in 50 bp length). Cells were grown according to the approved ENCODE cell culture protocols.

Data: The SOLiD-generated RNA-Seq reads were 35 bp in length. An initial filtering process was performed to remove any non-desirable contamination sequences, such as rRNA, tRNA, and repeats etc. A read-split mapping approach was developed to map the 35 bp reads onto the reference genome (GRCh37/hg19) excluding mitochondrion, haplotypes, randoms and chromosome Y.

Mapping parameters: Strand specific mapping was done using Applied Biosystems' SOLiD alignment where all the reads were mapped to the genome, and to exon-exon junction database. Seed and extend strategy is adopted where initial seed length of 25 is mapped with maximum of 2 mismatches and then extended to read length, each color space match is awarded a score of +1 and each mismatch is awarded a penalty of -2.

After extension each read is trimmed to its maximum score, shortest length. The color space sequences are then converted into base space and checked to ensure that each sequence has a maximum of 2 base pair mismatches. If any sequence has more than 2 mismatches, then that sequence is discarded.

Credits

The GIS RNA-seq libraries and sequence data for transcriptome analysis were produced at the Genome Institute of Singapore. The data were mapped and analyzed by scientists from the Genome Institute of Singapore.

Contact: RUAN Xiaoan

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.