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Sample GSM1080053 Query DataSets for GSM1080053
Status Public on Sep 17, 2014
Title A549-8 weeks-0.4-rep 1
Sample type genomic
 
Channel 1
Source name Input DNA from A549 cells exposed to 0.4 µM of sodium arsenite for 8 weeks replicate 1
Organism Homo sapiens
Characteristics cell type: A549 human epithelial lung carcinoma cells
treatment: 0.4 µM of sodium arsenite
time: 8 weeks
sample type: input DNA
Extracted molecule genomic DNA
Extraction protocol Cells were washed twice with Hank's Buffered Salt Solution (Invitrogen) and trypsinized. Cell pellets were resuspended in 500 µl digestion buffer (1 mM EDTA; 50 mM Tris–HCl, pH 8.0; 5% SDS) and proteinase K (1 mg/ml) (Ambion) was added. After incubation of 1 hour at 55 °C, the proteinase K was inactivated at 80 °C. RNAse A (400 µg/ml) (Qiagen) treatment was performed for 1 hour at 37 °C. An equal amount of phenol-chloroform-isoamylalcohol (PCI; 25:24:1) (Sigma) was added and shaked manually for 5 min. After centrifugation, the upper phase was again treated with PCI until no protein was visible at the interphase. The upper phase was precipitated with 50 µl 3M NaAc pH 5.6 and 1250 µl cold 100% ethanol. The DNA pellet was washed with cold 70% ETOH, dissolved in 50µl nuclease free water and quantified spectrophotometrically using the NanoDrop 1000 (Thermo Scientific, Waltham, MA). The total amount was at least 10 µg DNA, the 260/280 ratio laid between 1.7-1.9, and the 260/230 was higher than 1.6.
Label Cy3
Label protocol Genomic DNAs were sonicated to obtain fragments ranging from 200 bp to 1000 bp, cleaned up using silica columns (Zymo Research) and eluted in TE buffer. 4.4 µg of each sonicated sample was dissolved in a total volume of 495 µL TE buffer. Ten percent of such prepared mixtures was kept as Input sample (Input) at 4°C, while the remaining was immunoprecipitated with 12 µL of a monoclonal antibody against 5’-methylcytidine (Eurogentec) as described by Weber et al (Weber M, JJ Davies, D Wittig, EJ Oakeley, M Haase, WL Lam and D Schubeler. 2005. Chromosome-wide and promoter-specific analyses identify sites of differential DNA methylation in normal and transformed human cells. Nat Genet 37: 853-862.). Immunoprecipitated DNAs (MeDIP) were purified using silica columns (Zymo Research) and eluted in TE buffer. Forty ng of both Input and MeDIP samples were whole genome amplified (WGA) using the WGA2 kit (Sigma Aldrich) following the manufacturer’s instruction, but omitting the fragmentation step. WGA reactions were cleaned up using silica columns (Sigma Aldrich) and eluted in water.
Labeling and hybridization of arrays was performed according to the manufactures’ protocol. In brief, 1 µg of Input DNA and 1 µg of MeDIP DNA were labeled with Cy3 and Cy5 respectively by random priming using the Dual Color DNA labeling kit (Roche NimbleGen). The labeled samples were precipitated using isopropanol and quantified spectrophotometrically using the NanoDrop 1000.
 
Channel 2
Source name medip DNA from A549 cells exposed to 0.4 µM of sodium arsenite for 8 weeks replicate 1
Organism Homo sapiens
Characteristics cell type: A549 human epithelial lung carcinoma cells
treatment: 0.4 µM of sodium arsenite
time: 8 weeks
antibody: monoclonal antibody against 5’-methylcytidine (Eurogentec, Weber et al (2005), PMID: 16007088)
sample type: immunoprecipitated methyl-DNA (MeDIP)
Extracted molecule genomic DNA
Extraction protocol Cells were washed twice with Hank's Buffered Salt Solution (Invitrogen) and trypsinized. Cell pellets were resuspended in 500 µl digestion buffer (1 mM EDTA; 50 mM Tris–HCl, pH 8.0; 5% SDS) and proteinase K (1 mg/ml) (Ambion) was added. After incubation of 1 hour at 55 °C, the proteinase K was inactivated at 80 °C. RNAse A (400 µg/ml) (Qiagen) treatment was performed for 1 hour at 37 °C. An equal amount of phenol-chloroform-isoamylalcohol (PCI; 25:24:1) (Sigma) was added and shaked manually for 5 min. After centrifugation, the upper phase was again treated with PCI until no protein was visible at the interphase. The upper phase was precipitated with 50 µl 3M NaAc pH 5.6 and 1250 µl cold 100% ethanol. The DNA pellet was washed with cold 70% ETOH, dissolved in 50µl nuclease free water and quantified spectrophotometrically using the NanoDrop 1000 (Thermo Scientific, Waltham, MA). The total amount was at least 10 µg DNA, the 260/280 ratio laid between 1.7-1.9, and the 260/230 was higher than 1.6.
Label Cy5
Label protocol Genomic DNAs were sonicated to obtain fragments ranging from 200 bp to 1000 bp, cleaned up using silica columns (Zymo Research) and eluted in TE buffer. 4.4 µg of each sonicated sample was dissolved in a total volume of 495 µL TE buffer. Ten percent of such prepared mixtures was kept as Input sample (Input) at 4°C, while the remaining was immunoprecipitated with 12 µL of a monoclonal antibody against 5’-methylcytidine (Eurogentec) as described by Weber et al (Weber M, JJ Davies, D Wittig, EJ Oakeley, M Haase, WL Lam and D Schubeler. 2005. Chromosome-wide and promoter-specific analyses identify sites of differential DNA methylation in normal and transformed human cells. Nat Genet 37: 853-862.). Immunoprecipitated DNAs (MeDIP) were purified using silica columns (Zymo Research) and eluted in TE buffer. Forty ng of both Input and MeDIP samples were whole genome amplified (WGA) using the WGA2 kit (Sigma Aldrich) following the manufacturer’s instruction, but omitting the fragmentation step. WGA reactions were cleaned up using silica columns (Sigma Aldrich) and eluted in water.
Labeling and hybridization of arrays was performed according to the manufactures’ protocol. In brief, 1 µg of Input DNA and 1 µg of MeDIP DNA were labeled with Cy3 and Cy5 respectively by random priming using the Dual Color DNA labeling kit (Roche NimbleGen). The labeled samples were precipitated using isopropanol and quantified spectrophotometrically using the NanoDrop 1000.
 
 
Hybridization protocol The pellet was dissolved in hybridization solution using the NimbleGen Hybridization kit. After denaturing the probe was hybridized overnight on the 2.1M Deluxe Promoter Arrays using the HX1 mixers and the NimbleGen Hybridization system 4.
Scan protocol Slides were scanned using the 2 µm high resolution NimbleGen MS 200 micro array scanner per manufacturer's protocol.
Description Sample name: 522507
Data processing Signal intensity data was extracted from the scanned images of each array using NimbleScan v2.6 software and quantile normalized on a per channel basis. Log2 ratios of the intensities were computed (ratio of MeDIP signal/Input signal) for each array. Detection of differential methylation was performed using the Probe Sliding Window-ANOVA algorithm (PSW-ANOVA). PSW-ANOVA (Roche NimbleGen) leverages the “neighbor effect” characteristics of Methylation Dependent ImmunoPrecipitation on chip (MeDIP-chip) data from high density oligonucleotide arrays, where enriched fragments sizes far exceed the spacing between probes. In other words, probes within close proximity have a greater likelihood of reporting signals derived from the same enriched fragment during MeDIP procedure. PSW-ANOVA uses a sliding window approach to identify potential sites of differential enrichment and then assigns probability scores (p values) to each probe on the array using a repeated measure ANOVA model. PSW-ANOVA is implemented in the R statistical programming environment as a custom script and was provided by Roche NimbleGen in collaboration.
Briefly, for each probe, a sliding window is determined based on the sliding window size parameter, centering on the probe in question. Within each sliding window, a repeated measures ANOVA is used to assess the difference between the various experimental groups for all probes located within the sliding window, using the probe ID as the reference to reduce the amount of error arising from different probes within a sliding window. It is assumed that the background and non-specific hybridization behavior of adjacent probes within a sliding window can be larger than the changes in intensity difference between the two channels, but within the sliding window, the log ratios will still be proportional to the intensity difference between groups of samples.
PSW-ANOVA (sliding window of 750 bp comprising 7 probes, and a FDR adjusted p- value < 0.05) was used to identify differential methylated regions (DMR) which were statistically significantly different between the different conditions tested in the experiment. Peaks were identified in the DMR by searching for the number of probes (default = 2) above a p-value minimum cutoff (-log10, default = 1.3) within 150 bp distance of each other. Peaks within 500 bp were merged. Peaks were mapped to promoter regions (from 3 kb upstream to 1 kb downstream of the transcription start site) and CpG islands of genes using the NimbleScan v2.6 software.
 
Submission date Feb 08, 2013
Last update date Sep 17, 2014
Contact name Simone G van Breda
E-mail(s) s.vanbreda@maastrichtuniversity.nl
Phone 0031433882127
Organization name Maastricht University
Department Toxicogenomics
Street address Universiteitssingel 50
City Maastricht
State/province Limburg
ZIP/Postal code 6229 ER
Country Netherlands
 
Platform ID GPL16284
Series (2)
GSE44173 Sodium arsenite induced DNA methylation changes in A549 human epithelial lung carcinoma cells
GSE44174 Sodium arsenite induced changes in A549 human epithelial lung carcinoma cells

Data table header descriptions
ID_REF
VALUE scaled, log2 (medip/Input) ratio for demethylated regions

Data table
ID_REF VALUE
CHR01FS000015738_chr1:15366-44081 0.0116322405820041
CHR01FS000016058_chr1:15366-44081 0.826782192215501
CHR01FS000016770_chr1:15366-44081 0.944724850444329
CHR01FS000017334_chr1:15366-44081 1.28797999026015
CHR01FS000017588_chr1:15366-44081 0.867499088544755
CHR01FS000017864_chr1:15366-44081 0.282251669928813
CHR01FS000018156_chr1:15366-44081 1.08087533384752
CHR01FS000018710_chr1:15366-44081 0.799289769217198
CHR01FS000018838_chr1:15366-44081 1.11536095510338
CHR01FS000019822_chr1:15366-44081 0.817643652259098
CHR01FS000020184_chr1:15366-44081 0.64084134078066
CHR01FS000020366_chr1:15366-44081 0.772960545440882
CHR01FS000020764_chr1:15366-44081 0.970295446429096
CHR01FS000020848_chr1:15366-44081 1.64301983018214
CHR01FS000020986_chr1:15366-44081 1.12630189968147
CHR01FS000021090_chr1:15366-44081 2.13505563444377
CHR01FS000021314_chr1:15366-44081 2.1849450414015
CHR01FS000021466_chr1:15366-44081 2.20031050263456
CHR01FS000021836_chr1:15366-44081 1.42563747382094
CHR01FS000021924_chr1:15366-44081 1.80483648360474

Total number of rows: 2077859

Table truncated, full table size 120004 Kbytes.




Supplementary file Size Download File type/resource
GSM1080053_522507_532.pair.gz 42.7 Mb (ftp)(http) PAIR
GSM1080053_522507_635.pair.gz 42.3 Mb (ftp)(http) PAIR
Processed data included within Sample table

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