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Sample GSM531509 Query DataSets for GSM531509
Status Public on Apr 14, 2010
Title TAX577659 [33K]
Sample type genomic
 
Channel 1
Source name Breast tumor
Organism Homo sapiens
Characteristics disease state: Breast cancer (HER2+)
er: er_neg
osbin: 0
os: 15.50684932
age: 33.49315068
ln: 0
size_mm: 50
primary: 1
grade: NA
Extracted molecule genomic DNA
Extraction protocol Genomic DNA from fresh frozen breast tumor tissue was extracted using overnight digestion with proteinase K at 55C, followed by repeated phenol-chloroform purification steps. Genomic DNA from FFPE tissue was extracted according to protocol from http://cancer.ucsf.edu/array/protocols/index.php. DNA concentrations were measured using a Nanodrop.
Label Cy3
Label protocol Fluorescently labeled DNA targets for hybridization were prepared according to manufacturers' instructions using the Invitrogen Bioprime aCGH Genomic Labeling Module as described (PMID:17334996).
 
Channel 2
Source name promega male reference
Organism Homo sapiens
Characteristics reference: Promega male reference DNA
Extracted molecule genomic DNA
Extraction protocol Genomic DNA from fresh frozen breast tumor tissue was extracted using overnight digestion with proteinase K at 55C, followed by repeated phenol-chloroform purification steps. Genomic DNA from FFPE tissue was extracted according to protocol from http://cancer.ucsf.edu/array/protocols/index.php. DNA concentrations were measured using a Nanodrop.
Label Cy5
Label protocol Fluorescently labeled DNA targets for hybridization were prepared according to manufacturers' instructions using the Invitrogen Bioprime aCGH Genomic Labeling Module as described (PMID:17334996).
 
 
Hybridization protocol BAC aCGH microarrays were hybridized as described (PMID: 17334996)
Scan protocol Arrays were washed as described (PMID: 17334996) and fluorescence was recorded using an Agilent G2565AA microarray scanner (Agilent Technologies).
Description n/a
Data processing TIFF images were analyzed using the Gene Pix Pro software (Axon Instruments, Foster City, CA), and the quantified data matrix was loaded into a local installation of BioArray Software Environment (BASE) (http://base.thep.lu.se). Quantified intensities for tumor sample were stored as channel 1 (ch1) whereas quantified intensities for reference sample were stored as channel 2 (ch2). Median spot pixel values were used to calculate background corrected intensities (Int1 and Int2). Spots were removed and regarded as missing values if either: (1) flagged during image-analysis, (2) background corrected intensity value >64999 signal units, (3) background corrected intensity value <0 signal units, or (4) spot diameter less than 40 um. For spots, log ratio (M) was calculated as log2(Int1/Int2) and average intensity (A) was calculated as log10(Int1*Int2)/2. Normalization was performed by applying popLowess (PMID: 17953745). Spots from dye-swap hybridization were merged using geometric mean of ratios after normalization.
 
Submission date Apr 08, 2010
Last update date Apr 14, 2010
Contact name Johan Staaf
Organization name SCIBLU - Swegene Centre for Integrative Biology at Lund University
Street address Medicon Village
City Lund
ZIP/Postal code SE-223 81
Country Sweden
 
Platform ID GPL7247
Series (1)
GSE21259 High-resolution aCGH analyses of copy number alterations in HER2-amplified breast cancer

Data table header descriptions
ID_REF
VALUE Normalized log2 ratio (tumor/reference male DNA).

Data table
ID_REF VALUE
28065 -0.305025144
23532 0.022865339
7034 -0.121602598
14459 -0.092342891
27309 0.007842947
8491 -0.288208909
19769 -0.145698655
14081 -0.199475234
20900 0.047284302
33192 0.345376297
34676 -0.067900447
18070 -0.315587129
5213 0.181341675
14336 -0.277845362
293 -0.101670096
1050 -0.137210718
13404 0.453102256
24746 0.103246044
3583 -0.083936499
11717 null

Total number of rows: 32573

Table truncated, full table size 569 Kbytes.




Supplementary file Size Download File type/resource
GSM531509_TAX577659_Cy3_1.gpr.gz 2.7 Mb (ftp)(http) GPR
Processed data included within Sample table

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