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Sample GSM840913 Query DataSets for GSM840913
Status Public on Jun 01, 2012
Title Input 3/2, membrane B [070420Chr]
Sample type genomic
 
Source name Control (input) non-immunoprecipitated chromatin fragments, seeds
Organism Arabidopsis thaliana
Characteristics ecotype: Col-0
tissue: seed
developmental stage according to boyes et al. (2004): 11-13 DAP
chip antibody: no
Growth protocol Arabidopsis plants were grown on soil, with a 16 h light/ 8 h dark cycle
Extracted molecule genomic DNA
Extraction protocol Chromatin was isolated from unripe seeds of Arabidopsis thaliana Col-0, harvested 11-13 days after pollination. Cross-linking was done with 1% formaldehyde for 20 min under vacuum, terminated by addition of glycine with a final concentration of 125 mM. Seeds were Potter-homogenized, filtered and the nuclei collected by centrifugation. Nuclear membranes were dissolved with detergents and the chromatin was collected by high speed centrifugation. Chromatin was fragmented to an average size of 500 bp by ultra sonic treatment. 10 µg chromatin were combined with 2 µg anti-ABI3 antibody. The antibody-chromatin complex was captured by protein A coated magnetic beads (Invitrogen). After different washings the TF-DNA complex was eluted from the beads at 65°C for 15 min using 1% SDS. Eluates were incubated overnight at 65°C to reverse the cross-links. DNA fragments were purified using a QIAquick PCR Purification Kit (Qiagen) and their concentration was determined with a NanoDrop 3300 (Thermo Fisher Scientific) fluorescence spectrophotometer. An aliquot (0.5 µg) of non-immunoprecipitated chromatin served as input control. DNA fragments were blunted and ligated with the adapters oJW102 and oJW103 (Young lab:jura.wi.mit.edu/young_public/hESregulation/ChIP.html). Adapter-ligated fragments were amplified using oJW102 as sole primer.
Label [α-33P]dCTP
Label protocol Labelled probes were obtained by combining three parallel random priming reactions using the Megaprime Kit (GE Healthcare, Uppsala, Sweden), 1ng amplified chromatin, and 50µCi [α-33P]dCTP per reaction.
 
Hybridization protocol Arrays were prehybridized for 1h at 65°C in Church buffer (0,5M sodium phosphate, pH7,2, 7% SDS, 1% BSA, 1mM EDTA, 10µg/ml sheared salmon sperm DNA) per cm2 of membrane in a rotating thermal oven. Labelled probes were added and hybridization continued for 4 days. Membranes were washed twice in 0,2x SSC, 0,1% SDS for 20 min at 65°C and then placed on a moist Whatman paper, wrapped in Saran wrap and exposed to a Fuji image plate for 10 days in a lead chamber.
Scan protocol Signals were detected using a FLA 3000 phosphoimager at 50µm resolution and 16 bit grey scale (Fuji). Spot intensities were obtained by aligning the pre-defined spotting pattern using ArrayVision software (GE Healthcare).
Description 070420Chr
Raw data file: 070420_B_CHR.txt
control technical replicate of biol. replicate 3
Hybridization on membrane B
Data processing Five ABI3 ChIP-chip experiments (three biological and two technical replicates) were performed, each consisting of a pair of hybridisations with amplified input chromatin and immuno-precipitated chromatin. For normalization, the median of log2 transformed signal intensities of each hybridisation was centred at zero. Quantile normalization (Bolstad et al. 2003) was applied separately to datasets of input and immuno-precipitated chromatin. Duplicated spotting of each amplicon on the arrays provided an internal quality control, which was used to exclude all signals with a difference of normalized log2 intensities larger than one between the two spots (1.56% of all signals). Missing values were again substituted by the mean of normalized log2 intensities from other hybridisations of the same kind, chromatin or immuno-precipitated chromatin, if the signal was excluded in no more than two hybridisations. Finally, the mean of normalized log2 intensities from both spots of each amplicon was calculated and the mean values of hybridisations with input chromatin were subtracted from the mean values of hybridizations with immuno-precipitated chromatin, resulting in log2 enrichment factors for most (> 99.85%) of the spotted amplicons in all five experiments.
 
Submission date Nov 30, 2011
Last update date Jun 01, 2012
Contact name Gudrun Moenke
E-mail(s) [email protected]
Organization name IPK
Street address Corrensstr. 3
City Gatersleben
ZIP/Postal code 06466
Country Germany
 
Platform ID GPL14942
Series (2)
GSE34041 Identification of target genes of ABI3 [SAP]
GSE34043 Identification of target genes of ABI3

Data table header descriptions
ID_REF
VALUE log2 of quantile normalized (double spot corrected) signal intensities

Data table
ID_REF VALUE
AT5G15840 2.402
AT5G18620 1.936
AT5G16010 0.777
AT5G18840 0.081
AT5G16210 0.741
AT5G19080 0.090
AT5G16450 -0.698
AT5G19320 1.048
AT5G16610 0.325
AT5G19630 -0.464
AT5G16880 -0.391
AT5G19855 2.027
AT5G17070 1.406
AT5G19990 0.217
AT5G17440 0.809
AT5G20130 -0.303
AT5G17610 0.802
AT5G20390 -0.421
AT5G17820 0.991
AT5G20670 -0.178

Total number of rows: 5760

Table truncated, full table size 92 Kbytes.




Supplementary file Size Download File type/resource
GSM840913.txt.gz 178.5 Kb (ftp)(http) TXT
Processed data included within Sample table
Processed data are available on Series record

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