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Sample GSM3059520 Query DataSets for GSM3059520
Status Public on May 03, 2019
Title Sample 76
Sample type genomic
 
Source name FACS-sorted neurons from the frontal cortex of the human brain
Organism Homo sapiens
Characteristics tissue: frontal cortex of the brain
sampleID: 8
tissuebank.id: 4835
age: 56
Sex: Male
race: White
dist.dx: Bipolar
tissuebank: Sepulveda
pmi: 19.3
cell.type: NeuN+
Treatment protocol Neuronal nuclei were separated using a flow cytometry-based approach, similar to as previously described (PMID: 25369517,PMID: 19078943). Human brain tissue (250 mg) for each sample was minced in 2 mL PBSTA (0.3 M sucrose, 1X phosphate buffered saline (PBS), 0.1% Triton X-100). Samples were then homogenized in PreCellys CKMix tubes with a Minilys (Bertin Instruments) set at 3,000 rpm for three 5 sec intervals, 5 min on ice between intervals. Samples homogenates were filtered through Miracloth (EMD Millipore), followed by a rinse with an additional 2 mL of PBSTA. Samples were then place on a sucrose cushion (1.4 M sucrose) and nuclei were pelleted by centrifugation at 4,000 × g for 30 min 4°C using a swinging bucket rotor. For each sample, the supernatant was removed and the pellet was incubated in 700 μl of 1X PBS on ice for 20 min. The nuclei were then gently resuspended and blocking mix (100 μl of 1X PBS with 0.5% BSA (Thermo Fisher Scientific) and 10% normal goat serum (Gibco) was added to each sample. NeuN-488 (1:500; Abcam) was added and samples were incubated 45 min at 4°C with gentle mixing. Immediately prior to flow cytometry sorting, nuclei were stained with 7-AAD (Thermo Fisher Scientific) and passed through a 30 μM filter (SystemX). Nuclei positive for 7-AAD and either NeuN+ (neuronal) or NeuN- (non-neuronal) were sorted using an Influx (BD Biosciences) at the Faculty of Medicine Flow Cytometry Facility at the University of Toronto (Toronto, ON, Canada). Approximately 1 million NeuN+ nuclei were sorted for each sample. Immediately, after sorting nuclei were placed on ice and then precipitated by raising the volume to 10 mL with 1X PBS and adding 2 mL 1.8 M sucrose, 50 μl 1M CaCl2 and 30 μl Mg(Ace)2 and centrifugation at 1,786 × g for 15 min at 4°C. The supernatant was removed from NeuN+ and NeuN- samples and pellets were stored at -80°C.
Growth protocol DNA was extracted from post-mortem brain samples. No growth protocols were used.
Extracted molecule genomic DNA
Extraction protocol Genomic DNA from each NeuN+ and NeuN- fraction of each sample was isolated using standard phenol-chloroform extraction methods.
Label Cy5 and Cy3
Label protocol Reagent/array were purchased from Illumina. The experiment was carried out in Sickkids TCAG Microarray facility according to the recommended protocol by Illumina.
 
Hybridization protocol Reagent/array were purchased from Illumina. The experiment was carried out in Sickkids TCAG Microarray facility according to the recommended protocol by Illumina.
Scan protocol Reagent/array were purchased from Illumina. The experiment was carried out in Sickkids TCAG Microarray facility according to the recommended protocol by Illumina.
Description neurons from post-mortem human brain
Data processing Data generated from the microarrays were preprocessed with Minfi v1.19.12. Normalization was performed with noob, followed by quantile normalization. All samples had sex matching that predicted from the methylome. Probes that overlapping SNPs (MAF > 5%) on the CpG or single-base extension were excluded (11,812 probes), as were probes known to be cross-reactive (42,558 probes; PMID: 27330998) and those that failed detectability (P>0.01) in >20% samples (1,170 probes). After processing, 812,663 probes were left. Based on principal component analysis (PCA) co-clustering, one sample, despite being labeled NeuN+, clustered with NeuN- samples and was excluded from downstream analyses. Downstream analyses were performed using beta values ; only samples that were also genotyped were used in differential methylation analyses.
 
Submission date Mar 21, 2018
Last update date May 03, 2019
Contact name Shraddha Pai
E-mail(s) shraddha.pai@utoronto.ca
Organization name University of Toronto
Street address 160 College Street, Room 602
City Toronto
State/province ON
ZIP/Postal code M5S 3E1
Country Canada
 
Platform ID GPL21145
Series (2)
GSE112179 DNA methylation in neurons from post-mortem brains in schizophrenia and bipolar disorder (Methylation)
GSE112525 DNA methylation in neurons from post-mortem brains in schizophrenia and bipolar disorder

Data table header descriptions
ID_REF
VALUE Minfi-processed noob and quantile normalized beta values.

Data table
ID_REF VALUE
cg26928153 0.612138128413612
cg16269199 0.578353804589873
cg13869341 0.745046941714714
cg24669183 0.88022731599161
cg26679879 0.628273000322834
cg22519184 0.711790321631945
cg15560884 0.5150353076969
cg01014490 0.0710787646103903
cg24063007 0.0582135807069882
cg10692041 0.913982651455015
cg09961319 0.810754911175705
cg02339369 0.920264868602348
cg17505339 0.953512382451974
cg09499020 0.424069742181461
cg16535257 0.688207598876671
cg15979415 0.541946887760485
cg11954957 0.886409982935516
cg04747364 0.951252909343429
cg26304905 0.953249459750914
cg20434134 0.956330867384899

Total number of rows: 812663

Table truncated, full table size 23039 Kbytes.




Supplementary file Size Download File type/resource
GSM3059520_200357150067_R08C01_Grn.idat.gz 7.2 Mb (ftp)(http) IDAT
GSM3059520_200357150067_R08C01_Red.idat.gz 7.1 Mb (ftp)(http) IDAT
Processed data included within Sample table

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