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Sample GSM3385277 Query DataSets for GSM3385277
Status Public on May 08, 2019
Title RSV_Control [8650489034_B]
Sample type RNA
 
Source name RSV_Control
Organism Mus musculus
Characteristics mouse strain: C57BL/6
mouse model: Respiratory syncytial virus (RSV)
condition: Control
infection protocol: Plaque-purified human RSV A2 strain originally obtained from the ATCC was grown to high titer (≥107 focus-forming units per ml) in Hep-2 cells, snap frozen, and assayed for infectivity prior to use. Female C57BL/6/J mice (MRC NIMR) were infected i.n. with 1x106 FFU of RSV diluted in 100ml PBS. Control uninfected mice received PBS only. Lung samples were collected from individual mice on day 2 post infection.
tissue: lung
Extracted molecule total RNA
Extraction protocol Tissues were collected in TRI-Reagent (Sigma-Aldrich) (for Toxoplasma gondii samples –tissues were collected and samples were stored in RNAlater (Ambion), and then transferred to TRI-Reagent). Total RNA was extracted using the RiboPure™ Kit (Ambion).
Label biotin
Label protocol cRNA was prepared from 200 ng tissue total RNA using the Illumina TotalPrep RNA Amplification Kit (Ambion). Quality was checked using an RNA 6000 Nano kit (Agilent) using a BioAnalyzer 2100 (Agilent). Biotinylated cRNA samples were randomized.
 
Hybridization protocol 1.5 µg cRNA was then hybridized to Mouse WG-6 v2.0 bead chips (Illumina) according to the manufacturer’s protocols.
Scan protocol Standard Illumina scanning protocol
Description raw data file: MRC29.txt
Control samples from Respiratory syncytial virus (RSV) infection model
Data processing Microarray data was processed in GeneSpring GX v14.8 (Agilent Technologies). Flags were used to filter out the probe sets that did not result in a ‘present’ call in at least 10% of the samples, with the ‘present’ lower cut-off of 0.99. Signal values were then set to a threshold level of 10, log2 transformed, and per-chip normalised using 75th percentile shift algorithm. Next, per-gene normalisation was applied by dividing each messenger RNA transcript by the median intensity of all the samples. Next, transcripts were filtered to select the most variable probes: those that had a minimum of 1.5-fold expression change compared with the median intensity across all samples, in greater than 10% of all samples.
 
Submission date Sep 12, 2018
Last update date May 08, 2019
Contact name Akul Singhania
E-mail(s) akul.singhania@crick.ac.uk
Phone +442037963319
Organization name The Francis Crick Institute
Street address 1 Midland Road
City London
ZIP/Postal code NW1 1AT
Country United Kingdom
 
Platform ID GPL17543
Series (2)
GSE119849 Global transcriptional profiling unveils the interferon network in blood and tissues across different diseases [microarray_lung_6]
GSE119856 Global transcriptional profiling unveils the interferon network in blood and tissues across different diseases

Data table header descriptions
ID_REF
VALUE GeneSpring GX v14.8 per-chip and per-gene normalised log2 expression values

Data table
ID_REF VALUE
ILMN_2735294 0.9145733
ILMN_2545897 -0.3607328
ILMN_2762289 0.0590899
ILMN_1248788 0.06422281
ILMN_3092673 0.15614653
ILMN_1243193 -0.41615987
ILMN_2543688 0.019926548
ILMN_2816356 -0.06973219
ILMN_1224596 1.173913
ILMN_2808939 0.11683273
ILMN_2634564 -0.27829075
ILMN_1216623 -0.24514008
ILMN_2435996 0.009164095
ILMN_1215157 -0.010589123
ILMN_1236537 0.00915432
ILMN_2772422 1.2445974
ILMN_2739275 0.34207392
ILMN_2734484 0.50276136
ILMN_2952292 -0.08354664
ILMN_2551266 0.060506225

Total number of rows: 17397

Table truncated, full table size 411 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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