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Sample GSM713147 Query DataSets for GSM713147
Status Public on May 02, 2011
Title seq-SDQ3590_EFL1_N2_L3_1
Sample type SRA
 
Source name whole body
Organism Caenorhabditis elegans
Characteristics tissue: whole body
strain: N2
Stage: L3
chip antibody: SDQ3590 EFL1
chip antibody supplier: SDI
chip antibody catalog#: 44960002
chip antibody lot#: G3048-110A01 Animal number SDQ3590
Treatment protocol Worms are frozen, ground, and crosslinked for 10 minutes in 1% formaldehyde. Formaldehyde is quenched and cross-linked tissue washed, then resuspended in FA buffer and subjected to sonication in Bioruptor (14 pulses of 30 seconds with 1 minute rests in between). Extracts are then spun down and soluble fraction is stored for quality tests and future ChIP. http://wiki.modencode.org/project/index.php/Worm_L3_extraction:JL:PK1
Growth protocol About 2-7 million of worms are bleached and then hatched in M9 for 24-42 hrs. About 100 embryos are seeded onto the plate to test for contamination and hatching efficiency. Remaining hatched L1 larvae are inoculated in a proper volume of liquid culture. Next day when larvae reach the L3 stage they are cleaned by M9 washes and sucrose gradient and collected by freezing in liquid nitrogen. Just before collection DIC pictures are taken and about 50ul of worms are stained for DAPI to assess the stage. http://wiki.modencode.org/project/index.php/Worm_L3_growth_and_harvest:JL:PK1
Extracted molecule genomic DNA
Extraction protocol Libraries were prepared according to Illumina's instructions for "Preparing Samples for ChIP Sequencing of DNA", with some variation. DNA was end-repaired using T4 DNA polymerase, Klenow DNA polymerase and T4 DNA polymerase. A's were then added to the 3' ends of the fragments using Kelow fragment (3' 5' exo minus). Paired-end adapters were then ligated onto the ends of the fragments. DNA library was size selected by gel purification, fragments of 250-500 bp were band isolated from an agarose gel. DNA was PCR amplified for 18 cycles. The Bioanalyzer was used to verify fragment purification and quantify DNA.
 
Library strategy ChIP-Seq
Library source genomic
Library selection ChIP
Instrument model Illumina Genome Analyzer II
 
Description input control: GSM706161
Chromatin IP against EFL1. http://wiki.modencode.org/project/index.php/Worm_chromatin_immunoprecipitation:JL:IL2
Data processing BWA is a fast light-weighted tool that aligns relatively short sequences to a sequence database. The algorithms is based on Burrows-Wheeler Transform (BWT). See the link @ http://bio-bwa.sourceforge.net/. It runs as DEFAULT for both bwa aln and bwa samse.
ChIP-Seq MACS Peak-calling:JL:1. Peak calls were determined by using Model-based Analysis of ChIP-Seq (MACS) software. MACS was supplied with the following parameters: tagSize = 25 mfold = 10,30 genomeSize = 90000000 bandwidth = 300 pvalue = 1e-5
Processed data file build: ce6
 
Submission date Apr 21, 2011
Last update date May 15, 2019
Contact name Tristan De Buysscher
Organization name University of North Carolina at Chapel Hill
Department Biology
Lab Lieb
Street address CB# 3280, Coker Hall
City Chapel Hill
State/province NC
ZIP/Postal code 27599-3280
Country USA
 
Platform ID GPL9269
Series (1)
GSE28768 seq-SDQ3590_EFL1_N2_L3
Relations
SRA SRX059252
BioSample SAMN00261271
Named Annotation GSM713147_seq-SDQ3590_EFL1_N2_L3_1_catted.wig.gz

Supplementary file Size Download File type/resource
GSM713147_seq-SDQ3590_EFL1_N2_L3_1_catted.wig.gz 27.8 Mb (ftp)(http) WIG
GSM713147_seq-SDQ3590_EFL1_N2_L3_1_macs14_peaks.gff.gz 45.3 Kb (ftp)(http) GFF
SRA Run SelectorHelp
Raw data are available in SRA
Processed data provided as supplementary file

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