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Sample GSM4444287 Query DataSets for GSM4444287
Status Public on May 19, 2020
Title 201503670155_R07C01
Sample type genomic
 
Source name blood samples
Organism Homo sapiens
Characteristics age: 39
Sex: F
person id: 47758
disease state: normal
Extracted molecule genomic DNA
Extraction protocol bisulphite conversion of 500 ng of each DNA sample was performed using the EZ DNA Methylation-Lightning Kit according to the manufacturer’s protocol (Zymo Research, Orange, CA).
Label biotin (ddCTP and ddGTP) and 2,4-dinitrophenol (DNP) (ddATP and ddTTP)
Label protocol Illumina Infinium HD Methylation protocol
 
Hybridization protocol Then, bisulfite-converted DNA was used for hybridization on the Infinium HumanMethylation EPIC BeadChip, following the Illumina Infinium HD Methylation protocol. Briefly, a whole genome amplification step was followed by enzymatic end-point fragmentation and hybridization to HumanMethylation EPIC BeadChips at 48°C for 17 h, followed by single nucleotide extension. The incorporated nucleotides were labelled with biotin (ddCTP and ddGTP) and 2,4-dinitrophenol (DNP) (ddATP and ddTTP).
Scan protocol the BeadChip was scanned using the Illumina HiScan SQ scanner. The intensities of the images were extracted using in-house software written for the R statistical computing environment. The methylation score for each CpG was represented as a β-value according to the fluorescent intensity ratio representing any value between 0 (unmethylated) and 1 (completely methylated).
Description normal blood sample
Data processing DNA methylation (DNAm) data were pre-processed and normalized using in-house software written for the R statistical computing environment, including background and color bias correction, quantile normalization, and Beta MIxture Quantile dilation (BMIQ) procedure to remove type I/type II probes bias, as described elsewhere (Fiorito et al., 2017). DNAm levels were expressed as the ratio of the intensities of methylated cytosines over the total intensities (β values). Cross-reactive and polymorphic probes - with minor allele frequency greater than 0.01 in Europeans (Y. A. Chen et al., 2013) - were excluded. Methylation measures were set to missing if the detection p-value was greater than 0.01. Samples with the bisulfite conversion control fluorescence intensity lower than 10,000 for both type I and type II probes and those with total call rate lower than 95% were excluded. Finally, samples were excluded if the predicted sex (based on chromosome X methylation) did not match that self-reported.
DNAm levels were expressed as the ratio of the intensities of methylated cytosines over the total intensities (β values).
 
Submission date Mar 30, 2020
Last update date May 19, 2020
Contact name Oliver Robinson
E-mail(s) o.robinson@imperial.ac.uk
Phone 02075942067
Organization name IMPERIAL COLLEGE LONDON
Department School of Public Health
Lab MRC Centre for Environment and Health
Street address St Mary's Campus, Norfolk Place
City London
State/province London
ZIP/Postal code W21PG
Country United Kingdom
 
Platform ID GPL21145
Series (1)
GSE147740 DNA methylation analysis of human peripheral blood mononuclear cell collected in the AIRWAVE study

Supplementary file Size Download File type/resource
GSM4444287_201503670155_R07C01_Grn.idat.gz 6.8 Mb (ftp)(http) IDAT
GSM4444287_201503670155_R07C01_Red.idat.gz 7.0 Mb (ftp)(http) IDAT
Processed data are available on Series record

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