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Sample GSM637899 Query DataSets for GSM637899
Status Public on Jan 13, 2011
Title Tumor 3-inVIVO-Normox_Sp8N
Sample type RNA
 
Source name 9L glioma tumor
Organism Rattus norvegicus
Characteristics strain: Fisher
cell type: 9L glioma tumor
condition: Normoxic region
Treatment protocol For in vivo samples: LCM was applied to EF5-positive and negative areas. For in vitro samples: To initiate the experiment, cells were either incubated at ~20% O2 (“Normoxia”) or 0.2% O2 (“Hypoxia”) for 6h or 16h. Cells were subsequently washed with HBSS (Invitrogen), detached with 0.25% trypsin-EDTA and resuspended in RNA lysis solution (Ambion) at a concentration of 50,000cells/100μl lysis solution.
Growth protocol Six week old male Fischer 344 rats (F344/Ncr, NCI-Frederick, MD) were inoculated via subcutaneous injection on the hind flank with 9L cells (106) to generate passage ‘zero’ tumors (p0). The tumor was excised, cut into 1-2mm3 pieces and used to generate subsequent passages. The epigastric tumors were initiated by tying p5 or p6 tumor pieces onto the epigastric artery-vein pair. 9L gliosarcoma cells were grown in MEM media with 12% newborn calf serum with twice-weekly transfer.
Extracted molecule total RNA
Extraction protocol The RNAqueous-micro kit from Ambion which includes an application for LCM-generated tissue was used to isolate total RNA. A DNase I treatment was performed according to the manufacturer’s protocol. An additional centrifugation step (14,000rpm for 1.5 min) and subsequent supernatant removal were performed to ascertain that all resin had been eliminated. Total RNA was linearly amplified using the NuGEN Ovation WT-Pico kit. Briefly, total RNA (2ng/sample) was reverse transcribed to generate cDNA that incorporated an RNA primer binding sequence. After second-strand synthesis, cDNA templates were amplified by ribo-SPIA. T
Label Biotin
Label protocol The resulting amplified cDNA was fragmented, biotinylated and hybridized to Rat Gene 1.0ST Arrays (Affymetrix).
 
Hybridization protocol Microarrays were stained with streptavadin-phycoerythrin and incubated with biotinylated anti-streptavadin to enhance fluorescence signal detection. Comparison of signal intensity yielded relative gene expression under hypoxia/normoxia.
Scan protocol standard Affymetrix scan protocol
Data processing Affymetrix .cel files were imported into Partek Genomics Suite (v6.5b, Partek Inc., St. Louis, MO). Robust Multichip Average (RMA) normalization was applied.
 
Submission date Dec 09, 2010
Last update date Jan 13, 2011
Contact name Constantinos Koumenis
E-mail(s) koumenis@xrt.upenn.edu
Organization name University of Pennsylvania
Department Radiation Oncology
Street address 3620 Hamilton Walk
City Philadelphia
State/province PA
ZIP/Postal code 19146
Country USA
 
Platform ID GPL6247
Series (1)
GSE25980 In vitro and in vivo analysis of hypoxic gene expression in rat gliomas

Data table header descriptions
ID_REF
VALUE log2 GC-RMA signal

Data table
ID_REF VALUE
10778384 8.4432
10739986 10.8012
10769693 7.79391
10904578 7.60654
10908391 6.95821
10860806 7.30963
10860809 7.30963
10860812 7.30963
10890545 10.2771
10791358 8.77835
10909583 10.2719
10860815 7.67982
10905183 7.8872
10725748 5.65626
10771406 9.62868
10702293 6.50498
10853292 7.64448
10911014 8.24823
10742507 7.9879
10858275 8.1961

Total number of rows: 27363

Table truncated, full table size 451 Kbytes.




Supplementary file Size Download File type/resource
GSM637899.CEL.gz 4.1 Mb (ftp)(http) CEL
Processed data included within Sample table

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