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Sample GSM904727 Query DataSets for GSM904727
Status Public on Feb 25, 2013
Title shRNA-control-rep-2
Sample type RNA
 
Source name A375P cells expressing Control shScr
Organism Homo sapiens
Characteristics cell type: Melanoma cell line
cell line name: A375P
expression: Control shScr
Extracted molecule total RNA
Extraction protocol Total RNA was isolated using RNeasy (Qiagen) according to the manufacturer's instructions. The Dana Farber Cancer Institute Microarray Core synthesized single-stranded cDNA from the extracted RNA. RNA ws converted into cDNA using a T7 promoter-tailed oligo-dT primer in the synthesis of the first cDNA strand; second strand cDNA synthesis was then carried out.
Label biotin
Label protocol The double-stranded cDNA was used as the template in an in vitro transcription (IVT) reaction catalyzed by T7 polymerase and containing biotinylated CTP and UTP in addition to the four unmodified ribonucleoside triphosphates. The biotinylated complementary RNA (cRNA) waas purified from the IVT reaction mixture using magnetic particles. The cRNA was quantified spectrophotometrically and purity of the cRNA is also assessed by spectrophometric measurements. The purified cRNA was fragmented in order to facilitate the subsequent hybridization step.
 
Hybridization protocol The fragmented cRNA was added to a hybridization solution containing several biotinylated control oligonucleotides (for quality control), and hybridized to a microarray chip overnight at 45°C. The hybridization solution was then removed. The chips were transferred to a fluidics instrument that performs washes to remove cRNA that has not hybridized to its complementary oligonucleotide probe. The bound cRNA was then fluorescently labeled using phycoerythrin-conjugated streptavidin (SAPE); additional fluors are then added using biotinylated anti-streptavidin antibody and additional SAPE.
Scan protocol Each cRNA bound at its complementary oligonucleotide was excited using a confocal laser scanner, GCS3000, and the positions and intensities of the fluorescent emissions were captured.
Data processing The data were analyzed with RMA (Gene Pattern's ExpressionFileCreator version 8). Parameters: method RMA quantile normalization yes background correct yes compute present absent calls no normalization method none value to scale to clm file annotate probes yes The data were analyzed with RMA (Gene Pattern's ExpressionFileCreator version 8). Parameters: method RMA quantile normalization yes background correct yes compute present absent calls no normalization method none value to scale to clm file annotate probes yes.
 
Submission date Mar 28, 2012
Last update date Feb 25, 2013
Contact name Pere Puigserver
E-mail(s) [email protected]
Phone 617-582-7977
Organization name Dana-Farber Cancer Institute
Street address 450 Brookline Av. CLSB-11144
City Boston
ZIP/Postal code 02215
Country USA
 
Platform ID GPL571
Series (1)
GSE36879 Profiling A375P melanoma cells following PGC1a suppression

Data table header descriptions
ID_REF
VALUE rma normalized

Data table
ID_REF VALUE
1007_s_at 891.5587071
1053_at 1281.469574
117_at 139.9968108
121_at 236.8421825
1255_g_at 13.09827861
1294_at 109.1028914
1316_at 208.8472831
1320_at 25.65430278
1405_i_at 14.07708987
1431_at 51.70085026
1438_at 62.10792918
1487_at 1103.844365
1494_f_at 43.02086897
1598_g_at 317.3113528
160020_at 131.8410825
1729_at 277.0060267
1773_at 166.7837728
177_at 78.95890548
179_at 312.5164294
1861_at 278.0918557

Total number of rows: 22277

Table truncated, full table size 496 Kbytes.




Supplementary file Size Download File type/resource
GSM904727_PP2010103058.CEL.gz 2.2 Mb (ftp)(http) CEL
Processed data included within Sample table

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