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Sample GSM785508 Query DataSets for GSM785508
Status Public on Dec 01, 2011
Title 5-AzaC 5uM TSA 0.3 uM 1
Sample type RNA
 
Source name Prostate cancer LNCaP cells
Organism Homo sapiens
Characteristics treatment: 5-AzaC 5uM TSA 0.3 uM
experiment: 1
cell line: LNCaP
Treatment protocol Cells were treated with dimethylsulfoxide (DMSO) as a control and 5-AzaC (5 microM), and/or TSA (0.3 microM). For combined treatments, TSA was added after 12 hr of pre-treatment with 5-AzaC or control. After 36 hr, all cell treatments were harvested for RNA extraction. DMSO, 5-AzaC and TSA n=5; TSA/5-AzaC n=4 independent experiments.
Growth protocol LNCaP cells were plated at 1x10^6 cells per 10 cm2 for 48 hours post treatment
Extracted molecule total RNA
Extraction protocol Total RNA was isolated with TRIZOL reagent according to the manufacturer protocol
Label Biotin
Label protocol Refer to Liu et al (PNAS 101: 9740-9744 (2004)). 5 ug of total RNA was labeled in reverse transcription at 37C for 90 mins by using biotin-labeled rand-octomer oligo primer. The RT reaction mix was further denatured by using 0.5 N NaOH / 1 mM EDTA at 65C for 15 mins and neutralized by 1 M Tris HCl pH 7.6. Biotin signal was detected with an Alexa 647-Streptavidin conjugate.
 
Hybridization protocol The chips were hybridized on Tecan HS 4800 hybridization station. Chips were pre-hybridized at 25C for 30 min in the buffer of 6x SSPE/ 30% formamide/ 1x Denhardt's solution. The chips were further hybridized with labeled target in 6x SSPE/ 30% formamide at 25C for 18 hr. Hybridization, post-hybridization washing in 0.75x TNT (Tris, sodium, Tween 20) (see PNAS) at 37C for 40 mins. The chips were stained by streptavidin-alexa647 (1:500) dilution in TNT for 30 mins. Post-staining washing in 1x TNT FOR 40 min. Rinse with water and spin dry.
Scan protocol Arrays were scanned on the GenePix scanner and analyzed using the GenePix Pro software package.
Data processing Raw gpr data files were MAS.5 median-based normalization and filtered for probes with low intensities (<10), minimum fold-change (i.e., less than 20% of expression data values with at least a 1.5-fold change in either direction from the gene’s median value) and >50% missing data were excluded. Class comparisons between treatments were carried out using randomized block univariate t-tests across independent experiments.
 
Submission date Aug 23, 2011
Last update date Dec 01, 2011
Contact name Robert Scott Hudson
Organization name NIH
Department NCI
Lab The Laboratory of Human Carcinogenesis
Street address National Cancer Institute Room Blgd.37/3044
City Bethesda
State/province MD
ZIP/Postal code 20852
Country USA
 
Platform ID GPL14184
Series (1)
GSE31620 MicroRNA-1 is a candidate tumor suppressor and prognostic marker

Data table header descriptions
ID_REF
VALUE Log2 Normalized signal intensity

Data table
ID_REF VALUE
1 12.04569912
2 12.33422565
3 8.196907997
4 8.433822632
5 6.073233604
6 9.733383179
7 9.799472809
8 5.923208237
9 8.527798653
10 8.594470024
11 9.22923851
12 9.192814827
13 7.766806602
14 7.942836761
15 6.000169754
16 5.75575161
17 6.766806602
18 11.86941338
19 11.970294
20 9.857504845

Total number of rows: 6572

Table truncated, full table size 105 Kbytes.




Supplementary file Size Download File type/resource
GSM785508_P5628_Ambs_-_24_pmt800_4152009.gpr.gz 514.6 Kb (ftp)(http) GPR
Processed data included within Sample table

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