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Sample GSM208527 Query DataSets for GSM208527
Status Public on Aug 06, 2007
Title Loucy day 3 1uM MRK-003
Sample type RNA
 
Channel 1
Source name Loucy day 3 DMSO
Organism Homo sapiens
Characteristics T-ALL cell line
Treatment protocol T-ALL cell lines were plated at a density of 5e4-1.5e5 cells per ml (depending on doubling time) and were treated with 1uM MRK-003 for 3 days.
Growth protocol T-ALL cell lines were plated at a density of 5e4-1.5e5 cells per ml (depending on doubling time) and were treated with 1uM MRK-003 for 3 days.
Extracted molecule total RNA
Extraction protocol Qiagen RNeasy spin columns with DNAse treatment
Label Cy3
Label protocol custom automated version of the aminoallyl MessageAmp II kit from Ambion.
 
Channel 2
Source name Loucy day 3 1uM MRK-003
Organism Homo sapiens
Characteristics T-ALL cell line
Treatment protocol T-ALL cell lines were plated at a density of 5e4-1.5e5 cells per ml (depending on doubling time) and were treated with 1uM MRK-003 for 3 days.
Growth protocol T-ALL cell lines were plated at a density of 5e4-1.5e5 cells per ml (depending on doubling time) and were treated with 1uM MRK-003 for 3 days.
Extracted molecule total RNA
Extraction protocol Qiagen RNeasy spin columns with DNAse treatment
Label Cy5
Label protocol custom automated version of the aminoallyl MessageAmp II kit from Ambion.
 
 
Hybridization protocol Microarrays are incubated at 40°C for 48 hours in a rotating carousel. Hybridizations to custom Agilent microarrays are completed as previously described (Hughes et al.Nat Biotech (2001), 19(4):342-7). Microarrays are washed to remove non-specific hybridized sample. Afterwards, microarrays are dried in an ozone-free nitrogen chamber.
Scan protocol Microarrays are scanned using the Agilent LP2 laser scanner. The scanner output is a Tiff file, which contains the quantitative hybridization data from each individual microarray. The Tiff files are then processed using Rosetta custom feature extraction software.
Description T-ALL cell line
Data processing Data were processed using the Rosetta Resolver® system. Rosetta's custom feature extraction software performs error modeling before data are loaded into the Resolver system. The Resolver system performs a squeeze operation that combines replicates of the same sequence in an array while applying error weighting. The error weighting consists of adjusting for additive and multiplicative noise. A P-value is generated and propagated throughout the system. The P-value represents the probability that a gene is expressed. The Resolver system allows users to set thresholds, below which genes of a P-value are considered to be significantly expressed. The Resolver system also combines multiple arrays using a squeezing process. If multiple spots reference one sequence, summarization is performed using an error-weighted average as described in Roland Stoughton and Hongyue Dai, Statistical Combining of Cell Expression Profiles. US Patent #6,351,712, February 26, 2002.
 
Submission date Jul 06, 2007
Last update date Aug 14, 2011
Contact name Olivia Fong
E-mail(s) olivia.fong@merck.com
Organization name Merck & Co.
Department Molecular Profiling
Lab Merck Research Laboratories
Street address P.O. Box 2000
City Rahway
State/province NJ
ZIP/Postal code 07065
Country USA
 
Platform ID GPL4372
Series (1)
GSE8416 GSI, Human T-ALL

Data table header descriptions
ID_REF Rosetta generated unique probe identifier
VALUE Corrected Log10 Ratio of channels (CH2/CH1) ('QUALITY = 0' data removed)
LOGINTENSITY Corrected average log intensity of channels
INTENSITY1 Cy3 intensity (CH1)
INTENSITY2 Cy5 intensity (CH2)
PVALUE P-value of LogRatio
QUALITY 1 - if good and non control, 0 - otherwise
UNF_VALUE Corrected Log10 Ratio of channels (CH2/CH1)

Data table
ID_REF VALUE LOGINTENSITY INTENSITY1 INTENSITY2 PVALUE QUALITY UNF_VALUE
10019475365 -0.0238 -0.8225 0.1554 0.1474 6.3908e-001 1 -0.0238
10019481149 -0.0142 -0.6168 0.2475 0.2389 7.7674e-001 1 -0.0142
10019495284 -0.0297 -1.0421 0.0939 0.0877 5.6859e-001 1 -0.0297
10019687586 0.0193 -1.2824 0.0524 0.0548 7.6944e-001 1 0.0193
10019713746 -0.0348 -0.5424 0.2991 0.2766 4.9456e-001 1 -0.0348
10019799479 -0.0199 -0.9046 0.1287 0.1228 6.8122e-001 1 -0.0199
10019809115 -0.0257 -0.4879 0.3377 0.3187 5.7709e-001 1 -0.0257
10019874890 -0.0066 -0.8254 0.1591 0.1572 8.9537e-001 1 -0.0066
10019903058 0.0397 -1.8441 0.0138 0.0150 7.8219e-001 1 0.0397
10019909307 -0.0224 -1.1922 0.0697 0.0663 7.2275e-001 1 -0.0224
10019911222 -0.0413 -1.0325 0.0986 0.0894 4.5902e-001 1 -0.0413
10019924807 -0.0019 -1.4390 0.0384 0.0383 9.8325e-001 1 -0.0019
10019927856 0.0003 -0.6932 0.2026 0.2031 9.9507e-001 1 0.0003
10019932383 -0.0125 -0.2045 0.6340 0.6156 8.0502e-001 1 -0.0125
10019948931 0.0185 -1.0618 0.0874 0.0939 8.3555e-001 1 0.0185
10019975533 0.0296 -1.4072 0.0380 0.0406 7.1602e-001 1 0.0296
10019977224 -0.0574 -1.0799 0.0895 0.0781 3.6808e-001 1 -0.0574
10019977227 -0.0481 -0.2844 0.5526 0.4918 5.4609e-001 1 -0.0481
10019987588 -0.0192 -1.0479 0.0960 0.0915 7.3520e-001 1 -0.0192
10020008603 -0.0555 -0.0389 0.9786 0.8580 3.2180e-001 1 -0.0555

Total number of rows: 39157

Table truncated, full table size 2407 Kbytes.




Supplementary file Size Download File type/resource
GSM208527_1.mage.txt.gz 1.5 Mb (ftp)(http) TXT
GSM208527_2.mage.txt.gz 1.5 Mb (ftp)(http) TXT
Processed data included within Sample table

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