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Sample GSM352278 Query DataSets for GSM352278
Status Public on Feb 23, 2009
Title AD5-DK5
Sample type RNA
 
Channel 1
Source name control vector
Organism Mus musculus
Characteristics Murine neuroblastoma cell line N18 infected with an adenovirus control vector (pAd-Track-CMV vector)
Extracted molecule total RNA
Extraction protocol Trizol (InVitrogen)
Label Cy5-CTP Agilent
Label protocol Briefly, 1-μg aliquots of total RNA were labeled using the Agilent Linear Amplification/Labeling kit (Agilent Technologies).
 
Channel 2
Source name Dyrk1a
Organism Mus musculus
Characteristics Murine neuroblastoma cell line N18 infected with an adenovirus containing coding sequence of Dyrk1a gene (pAd-Dyrk1a vector)
Extracted molecule total RNA
Extraction protocol Trizol (InVitrogen)
Label Cy3-CTP Agilent
Label protocol Briefly, 1-μg aliquots of total RNA were labeled using the Agilent Linear Amplification/Labeling kit (Agilent Technologies).
 
 
Hybridization protocol After checking the labeling efficiency and the product integrity, 750 ng Cy3- and 750 ng Cy5-labeled targets were mixed and incubated on an Agilent microarray slide for 17 hours at 65°C, in a rotating oven, using an Agilent in situ hybridization kit. The slides were washed and then any traces of water were removed by centrifugation at 800 rpm for 1 min.
Scan protocol Slides were scanned using a GenePix 4000B Microarray Scanner (Molecular Devices, Sunnyvale, CA, USA) at 5-μm resolution.
The photo multiplier tube (PMT) levels of the two channels at 635 nm (for Cy5) and 532 nm (for Cy3) were balanced to limit the number of saturated pixels (less than 0.005%) for generating gray scale 16-bit TIFF image files.
Description Murine neuroblastoma cell line N18 infected with an adenovirus containing coding sequence of Dyrk1a gene (pAd-Dyrk1a vector) or with an adenovirus control vector (pAd-Track-CMV vector).
Data processing The resulting images were processed using the GenePix Pro (v6.0.1.26) image analysis software. This included defining the spots, measuring the intensities, flagging the spots having inadequate quality control parameters and evaluating local background
The pre-processing of the data and its quality assessment were done using the MANGO (MicroArray Normalization tool of GODMAP) tools suit (version 1.0, CNRS BioInfome Team [http://bioinfome.cgm.cnrs-gif.fr/]), an R script that allows integrated analysis of two-color microarrays. The background level was calculated using morphological operators (a short closing followed by a large opening) and subtracted. Raw data were normalized using the print-tip lowess method, i.e. local regression normalization within an artificial print-tip block.
 
Submission date Dec 18, 2008
Last update date Feb 23, 2009
Contact name Gilles Maussion
Organization name INSERM U675
Street address 16 rue Henri Huchard
City PARIS
ZIP/Postal code 75018
Country France
 
Platform ID GPL2872
Series (2)
GSE14030 Transcriptional analysis of murine neurobastoma N18 cell line transfected with a pAd-Dyrk1a vector
GSE14105 Down syndrome study

Data table header descriptions
ID_REF
VALUE same as UNF_VALUE but with flagged values removed
log2(DKxAD)_289_ad5-dk5
flags
UNF_VALUE Lowess; log2 (Dyrk1a/control vector)

Data table
ID_REF VALUE log2(DKxAD)_289_ad5-dk5 flags UNF_VALUE
44290 0.352 6.59 0 0.352
44075 0.148 6.613 0 0.148
44289 6.542 -50 0.157
44074 6.632 -50 0.005
44288 0.046 6.595 0 0.046
44073 0.089 6.745 0 0.089
44287 -0.251 7.413 0 -0.251
44072 -0.29 7.605 0 -0.29
44286 -0.27 8.336 0 -0.27
44071 0.16 7.385 0 0.16
44285 -0.024 7.088 0 -0.024
44070 -0.026 6.688 0 -0.026
44284 0.033 6.608 0 0.033
44069 0.197 7.965 0 0.197
44283 -0.204 6.656 0 -0.204
44068 6.511 -50 0.015
44282 -0.145 7.066 0 -0.145
44067 0.02 6.603 0 0.02
44281 0 7.002 0 0
44066 -0.035 6.651 0 -0.035

Total number of rows: 44290

Table truncated, full table size 1090 Kbytes.




Supplementary file Size Download File type/resource
GSM352278.gpr.gz 6.3 Mb (ftp)(http) GPR
Processed data included within Sample table

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