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Sample GSM2063017 Query DataSets for GSM2063017
Status Public on Mar 01, 2016
Title Nac PolyI:C offspring, biological replicate 6
Sample type RNA
 
Source name C57BL/6 Nucleus Accumbens - frozen brain tissue - POLYI:C
Organism Mus musculus
Characteristics strain: C57BL/6N
prenatal exposure: PolyI:C
age: 12 weeks
tissue: brain
tissue region: Nucleus Accumbens (NAc)
Treatment protocol CC57BL/6 mice were treated with the synthetic viral mimetic poly(I:C) (5 mg/kg, i.v.) or control (saline, i.v.) solution on gestation day 17. Offspring were subjected to cognitive and behavioral testing in adulthood, and then whole genome gene expression analysis with Affymetrix Microarray and subsequent q-PCR validation were performed on the nucleus accumbens.
Extracted molecule total RNA
Extraction protocol [Tissue extraction protocol] The brains from adult offspring (12 weeks) were rapidly extracted from the skull (within < 20 s) and placed on an ice-chilled plate. This was followed by preparing 1-mm coronal brain sections using razorblade cuts and subsequent micro-dissection of the brain areas of interest. We dissected the nucleus accumbens (NAc, including core and shell subregions; bregma +1.5 to +0.5 mm). Brain specimens were collected in 96-well microtiter plates kept on dry ice and allowed to freeze before storage at −80°C until further use. Total DNA and RNA were isolated using the Qiagen AllPrep DNA and RNA Mini ki. Genome-wide gene expression analyses were performed using Affymetrix microarray assays (Mouse Gene 1.1 ST Array Strips on GeneAtlas platform), following the 3’IVT one cycle labelling
Total DNA and RNA were isolated using the Qiagen AllPrep DNA and RNA Mini kit following the manufacturers' instructions
Label biotin
Label protocol Gene expression microarray assays were performed using Mouse Gene 1.1 ST Array Strips on GeneAtlas platform (Affymetrix), following the 3’IVT one cycle labeling and amplification protocol described in the Affymetrix GeneChip Expression Analysis Technical Manuals and in the GeneAtlas™ WT Expression Kit User Manual. In detail, to synthesize First-Strand cDNA, 250ng RNA were reverse-transcribed with the Gene Atlas 3’IVT Express Kit or WT Expression Kit (Affymetrix, Santa Clara, CA, USA) using T7 oligo(dT) primer. Second-Strand cDNA synthesis was carried out using DNA polymerase and RNase H to simultaneously degrade RNA and synthesize second-strand cDNA. This step was followed by the in vitro transcription using IVT Labelling Master Mix to generate multiple copies of biotin-modified antisense-RNA (aRNA) from the double-stranded cDNA templates. Subsequently strand DNA was purified to remove unincorporated NTPs, salts, enzymes and inorganic phosphate.
 
Hybridization protocol Labelled cDNA (10ug) was then fragmented and 5.5ug were hybridized onto Mouse Gene 1.1 ST Array Strips. The reactions of hybridation, fluidics and imaging were performed on the Affymetrix Gene Atlas instrument according to the manufacturer’s protocol.
Scan protocol GeneChips were scanned using the GeneAtlas Platform following the manufacturers' instructions.
Description Gene expression data in PolyI:C offspring
sample 33 gd17 nac
Data processing Affymetrix CEL files were imported into Partek Genomics Suite version 6.6 for data visualization and statistical testing. Quality control assessment was performed using Partek Genomic Suite 6.6. All samples passed the criteria for hybridization controls, labelling controls and 3’/5’ Metrics. Background correction was conducted using Robust Multi-strip Average (RMA) (Irizarry et al, 2003) to remove noise from auto fluorescence. After background correction, normalization was conducted using Quantiles normalization (Bolstad et al, 2003) to normalize the distribution of probe intensities among different microarray chips. Subsequently, a summarization step was conducted using a linear median polish algorithm (Tukey, 1977) to integrate probe intensities in order to compute the expression levels for each gene transcript. Upon data upload, pre-processing of CEL data for the complete data set [total of twelve samples; six biological replicates per sample for vehicle, six biological replicates for GD17 Poly(I:C)] was performed using ANOVA to assess treatment effects.
 
Submission date Feb 16, 2016
Last update date Mar 01, 2016
Contact name Juliet Richetto
E-mail(s) [email protected]
Organization name University of Zurich - Vetsuisse
Department Institute for Pharmacology and Toxicology
Street address Winterthurerstrasse 260
City Zurich
ZIP/Postal code 8057
Country Switzerland
 
Platform ID GPL11533
Series (2)
GSE77971 Expression data from adult mouse Nucleus Accumbens following prenatal infection
GSE77973 Expression data from adult mouse brain regions following prenatal infection

Data table header descriptions
ID_REF
VALUE RMA values

Data table
ID_REF VALUE
10338001 10.296
10338002 4.41545
10338003 8.61992
10338004 7.90168
10338005 2.37227
10338006 2.61424
10338007 2.85462
10338008 3.29034
10338009 5.37478
10338010 2.39451
10338011 4.0867
10338012 2.44609
10338013 2.21959
10338014 2.28315
10338015 2.22945
10338016 5.01505
10338017 11.2515
10338018 4.526
10338019 3.70631
10338020 5.30289

Total number of rows: 35556

Table truncated, full table size 586 Kbytes.




Supplementary file Size Download File type/resource
GSM2063017_sample_33_gd17_nac.ga.cel.gz 4.2 Mb (ftp)(http) CEL
Processed data included within Sample table

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