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Sample GSM527019 Query DataSets for GSM527019
Status Public on Sep 21, 2010
Title 12611-12613-Cy3
Sample type RNA
 
Channel 1
Source name culture type: CM
Organism Homo sapiens
Characteristics sample_name: 12611-12613
sex: M
sample_type: sample
dkfz_patient_comments: B-CLL 44
culture_type: CM
time point (days): 2
Extracted molecule total RNA
Extraction protocol Total RNA isolation by Trizol extraction and purification on RNeasy Mini spin columns. Amplification of RNA by first- and second-strand cDNA synthesis. In vitro transcription of extracted cDNA by RiboMAX Large Scale RNA Production System T7.
Label Cy3
Label protocol Sample labelling by Klenow reaction using Cy3- or Cy5-labeld dUTP. Purification of labelled samples on Microcon YM-30 filter columns. Addition of blocking reagents: 25 μg Cot-1 DNA, 25 μg poly-A RNA, and 75 μg yeast tRNA.
 
Channel 2
Source name culture_type: control
Organism Homo sapiens
Characteristics sample_name: 12611-12612
sex: M
sample_type: control
dkfz_patient_comments: B-CLL 44
culture_type: 0
time point (days): 0
Extracted molecule total RNA
Extraction protocol Total RNA isolation by Trizol extraction and purification on RNeasy Mini spin columns. Amplification of RNA by first- and second-strand cDNA synthesis. In vitro transcription of extracted cDNA by RiboMAX Large Scale RNA Production System T7.
Label Cy5
Label protocol Sample labelling by Klenow reaction using Cy3- or Cy5-labeld dUTP. Purification of labelled samples on Microcon YM-30 filter columns. Addition of blocking reagents: 25 μg Cot-1 DNA, 25 μg poly-A RNA, and 75 μg yeast tRNA.
 
 
Hybridization protocol Array platform: 70 mer oligonucleotides (Human Oligo Set 4.0; Operon, Cologne, Germany). Pretreatment of slides: 2 min in 0.2perc SDS; 2 min in ddH2O at RT; 2 min in ddH2O at 95C, followed by 1 min centrifugation at 1000 rpm. Application of preheated (60 min 60C, 10 min 70C), dye-labeled cDNA in Ultra-Hyb hybridization buffer on microarrays in a GeneTAC Hybridization Station. Hybridization for 40h at 42C with gentle agitation. Wash steps: 36C; 5 min 0.5xSSC, 0.1perc SDS; 3 min 0.05xSSC, 0.1perc SDS; 20s 0.05xSSC; 20s 0.05xSSC, 0.1perc Tween20.
Scan protocol Scanning of hybridized microarrays at 5 μm resolution and variable PMT voltage to obtain maximal signal intensities with < 0.1perc probe saturation, a count ratio of 0.8-1.2 (Cy5/Cy3) and maximal congruence of histogram curves using a GenePix 4000B microarray scanner (Axon Instruments, Union City, USA).
Description log2 ratio Cy5/Cy3
Data processing Spots not recognized by the image analysis software, or not passing the quality criteria were excluded from the calculations. Raw fluorescence intensities were normalized applying the variance stabilization method (W. Huber et al., Bioinformatics 18 Suppl. 1, 2002).
 
Submission date Mar 26, 2010
Last update date Apr 30, 2013
Contact name Grischa Toedt
Organization name German Cancer Research Center (DKFZ)
Department Molecular Genetics (B060)
Lab Prof. Peter Lichter
Street address Im Neuenheimer Feld 280
City Heidelberg
ZIP/Postal code 69120
Country Germany
 
Platform ID GPL9244
Series (1)
GSE18192 Genome-Wide Expression Profiling of cultured B-CLL cells

Data table header descriptions
ID_REF ID column of the reference platform
VALUE normalized log2 Cy3/Cy5
INV_VALUE normalized log2 ratio (Cy5/Cy3)

Data table
ID_REF VALUE INV_VALUE
1 0.124806 -0.124806125766634
2 0.793285 -0.793284973586415
3
4 -0.765934 0.765934081229398
5
6 -0.289839 0.289839188221656
7 -0.498883 0.498883338718528
8
9
10 0.788724 -0.788724113436983
11 0.295467 -0.295466701767012
12 0.405326 -0.405325874333389
13 0.848864 -0.848864011832059
14 -0.152737 0.152736729367573
15 -0.232078 0.232078077578339
16 0.151627 -0.151627378695629
17 0.385906 -0.385906375142223
18 0.123556 -0.123556037837051
19 1.01081 -1.01080660767831
20 -0.0341499 0.034149880502282

Total number of rows: 37632

Table truncated, full table size 813 Kbytes.




Supplementary file Size Download File type/resource
GSM527019.gpr.gz 3.3 Mb (ftp)(http) GPR
Processed data included within Sample table

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