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Sample GSM1299365 Query DataSets for GSM1299365
Status Public on Feb 20, 2014
Title GSC1228-DistalBrain-rep3
Sample type RNA
 
Source name Mouse brain parenchyma
Organism Mus musculus
Characteristics tissue: distal mouse brain
Treatment protocol An intracranial orthotopic model in severe combined immunodeficiency (SCID) mice was utilized in order to generate infiltrative glioma xenograft tumors. Brains were handled in RNase free conditions, imbedded in OCT compound, frozen immediately and kept at -80°C. Total cellular RNA isolation was carried out for Affymetrix HG-U133 plus2 or Mouse430_2 GeneChip Arrays, according to the manufacturer instructions (Affymetrix, CA)
Growth protocol Primary GBM glioma stem cells were cultured in NBE medium consisting of Neurobasal A medium with N2 and B27 supplements (Invitrogen, Carlsbad, CA), and human recombinant basic fibroblast growth factor and epidermal growth factor (50 ng/mL each; R&D Systems, Minneapolis, MN). 0923 and 1228A1 (ex vivo culture of 1228 GSCs following one in vivo cycle) GSC lines were used for intracranial mouse glioma models.
Extracted molecule total RNA
Extraction protocol RNA extraction was performed via Rneasy
Label biotin
Label protocol Standard Affymetrix protocol
 
Hybridization protocol Standard Affymetrix protocol
Scan protocol Standard Affymetrix protocol
Description sample was taken from a distal area (uninfiltrated) mouse brain, 100% mouse
Data processing Alternative CDF's were generated by masking probes which showed non-specific hybridization towards mouse in the human arrays and vice versa. Briefly, using raw intensity signals from cel files, individual probes were filtered if they met the following criteria: the net intensity (PM-MM) of each probe pair from the cross-reactive species was less than 10 and greater than 50% of the corresponding signal from human tumor core. Alternatively, to detect cross-reactive human signal on the mouse microarrays, mouse chips were hybridized with pure human cell line RNA and the corresponding same criteria were applied. The remaining probes were grouped into their original probe sets and those that had at least 4 remaining probes were retained in the new chip definition file (cdf). This resulted in alternative cdf’s containing 26,954 probe sets for the HG-U133 plus2 array and 21,675 probe sets for the Mouse430_2 array. The gene expression data were calculated using the MAS5 algorithm following quantile normalization, and the results subjected to statistical analysis using a two-way Anova.
 
Submission date Dec 30, 2013
Last update date Mar 29, 2019
Contact name Margaret C Cam
E-mail(s) maggie.cam@nih.gov
Phone 240-760-7179
Organization name NIH
Street address Bldg 37/3041C
City Bethesda
State/province MD
ZIP/Postal code 20892
Country USA
 
Platform ID GPL18122
Series (1)
GSE53717 Identification of Molecular Pathways Facilitating Glioma Cell Invasion In Situ

Data table header descriptions
ID_REF
VALUE MAS 5.0 signal
ABS_CALL
DETECTION P-VALUE

Data table
ID_REF VALUE ABS_CALL DETECTION P-VALUE
1415670_at 489.4353529 P 0.008980225
1415671_at 3473.062334 P 0.002531077
1415672_at 1982.291789 P 0.001672877
1415673_at 243.6876703 P 0.005859362
1415674_a_at 755.8415955 P 0.013853877
1415675_at 601.0911169 P 0.003842942
1415676_a_at 1707.780462 P 0.003842942
1415678_at 1331.595798 P 0.002531077
1415679_at 1643.637712 P 0.005859362
1415680_at 217.3136634 P 0.013995859
1415681_at 570.0369683 P 0.001672877
1415682_at 258.3750273 P 0.005859362
1415683_at 1350.723563 P 0.005859362
1415684_at 189.4283897 P 0.003842942
1415685_at 506.6184139 P 0.008980225
1415686_at 900.3649225 P 0.003842942
1415687_a_at 2965.505867 P 0.008980225
1415688_at 1447.987204 P 0.003842942
1415689_s_at 299.3067478 P 0.001672877
1415690_at 1409.317025 P 0.001672877

Total number of rows: 26932

Table truncated, full table size 976 Kbytes.




Supplementary file Size Download File type/resource
GSM1299365_M1228_IM3_C_M430V2.CEL.gz 3.8 Mb (ftp)(http) CEL
Processed data included within Sample table

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