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Sample GSM531053 Query DataSets for GSM531053
Status Public on Apr 08, 2010
Title Hyperox.inf.2
Sample type RNA
 
Source name mouse retina, hyperoxia exposed, inferior half
Organism Mus musculus
Characteristics strain: C57BL/6J
treatment: Hyperoxia
tissue: inferior retina
Treatment protocol At the age of P (postnatal) 83-90, some mice were exposed to constant hyperoxia (75% O2) for 14 days. Oxygen-exposed animals were euthanized at the end of the period of hyperoxia; controls were euthanized at the same age. Retinas were removed and divided into superior and inferior halves. Retinal samples from 2 animals (1 male and 1 female) were pooled for each condition.
Growth protocol C57BL/6J mice, a hyperoxia-vulnerable strain , were used for this study. Mice were raised in dim cyclic illumination (12 hr 5 lux, 12 hr dark) and maintained in this level of lighting during the period of experiment.
Extracted molecule total RNA
Extraction protocol RNA extraction was performed using a combination of TRIzol Reagent (Invitrogen™ life technologies, Carlsbad, CA) and RNAqueous-micro kit (Ambion, Foster City, CA). TRIzol was used to isolate the RNA and the RNAqueous kit was used to purify and DNase-treat the RNA.
Label biotin
Label protocol Staining, hybridization, washing and scanning of the array were performed at the Biomolecular Resource Facility at the John Curtin School of Medical Research, Australian National University, following manufacturers’ protocols. Biotinylated sense-strand DNA targets from the entire expressed genome were prepared from 100ng total RNA, according to the Affymetrix Whole Transcript (WT) Sense Target labeling Assay Manual.
 
Hybridization protocol 7.5 ug of fragmented and labeled DNA target were used. Heat hybridization mixture at 99ْC for 5 mins (in lab heat block), then cool to 45ْC (in lab heat block) for 5 mins and centrifuge at max speed for 5 min. Inject approx 100uL of sample into array. Tough Spot the holes over the septa and immediately place the array in 45ْC hybridization oven at 60rpm for 17hours. Arrays were washed and stained in the Fluidics Station using the Prime_450 protocol.
Scan protocol Arrays were scanned using the Affymetrix Launcher. For Mouse, use MoGene 1_0-st-v1 universal Module and the FS450_0007 fluidics protocol.
Description mouse retina, hyperoxia exposed, inferior half, rep 2
Data processing CEL files were imported into Partek Genomics Suite, with the following normalization of their configuration: Probes to import - interrogating probes; Probe filtering - include core; Background correction - RMA background; Log base - 2; Probeset summarization - Median Polish.
 
Submission date Apr 07, 2010
Last update date Apr 07, 2010
Contact name Yuan Zhu
E-mail(s) [email protected]
Phone +61 2 61254489
Organization name Australian National University
Department Research School of Biology
Street address Bldg 46, RSBS, ANU
City Canberra
State/province ACT
ZIP/Postal code 2601
Country Australia
 
Platform ID GPL6246
Series (1)
GSE21246 Differential gene expression in mouse retina related to regional differences in vulnerability to hyperoxia

Data table header descriptions
ID_REF
VALUE Log 2 GC-RMA signal

Data table
ID_REF VALUE
10344614 7.12677
10344616 2.43491
10344618 3.27788
10344620 4.58793
10344622 8.13524
10344624 9.96692
10344633 10.3362
10344637 9.46021
10344653 4.99684
10344658 8.74903
10344674 3.7585
10344679 7.89371
10344705 6.19753
10344707 9.24187
10344713 9.68632
10344715 4.7064
10344717 4.26712
10344719 6.21055
10344721 2.56437
10344723 8.10599

Total number of rows: 28853

Table truncated, full table size 475 Kbytes.




Supplementary file Size Download File type/resource
GSM531053.CEL.gz 4.3 Mb (ftp)(http) CEL
Processed data included within Sample table

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