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Sample GSM802605 Query DataSets for GSM802605
Status Public on Mar 01, 2012
Title mammary gland , J50, control untreated, biological rep1
Sample type RNA
 
Source name pool of 5 RNA
Organism Rattus norvegicus
Characteristics tissue: mammary gland
strain: Wistar Han
treatment: none
Treatment protocol Females and males Wistar Han rats at eight weeks of age (Harlan France Sarl, Gannat, France) were maintained in an animal facility and fed a purified diet (phytoestrogen-free, INRA, France) and water ad libitum. Procedures for handling and experimentation followed ethical guidelines and were previously described [37, Reprod Toxicol]. At gestational day 1, determined by the presence of intravaginal sperm plug, the dams were randomly divided into groups of 15. From the first gestational day (GD1) until the weaning (PND 21), each pregnant female were orally gavaged once daily with genistein (G), vinclozoline (V) alone or in combination (GV) at 1 mg/kg body weight/day, as previously described ( ). At weaning, immature rats were dispatched. Female offspring were randomized (one female per litter), identified by implanted chips, and fed the purified diet until sacrifice (PND 35 and PND 50) (Fig. 1). Twenty pubertal or cycling female offspring animals per treatment group were used for subsequent analysis.
Growth protocol Females and males Wistar Han rats at eight weeks of age (Harlan France Sarl, Gannat, France) were maintained in an animal facility and fed a purified diet (phytoestrogen-free, INRA, France) and water ad libitum. Procedures for handling and experimentation followed ethical guidelines. At gestational day 1, determined by the presence of intravaginal sperm plug, the dams were randomly divided into groups of 15. From the first gestational day (GD1) until the weaning (PND 21), each pregnant female were orally gavaged once daily with genistein (G), vinclozoline (V) alone or in combination (GV) at 1 mg/kg body weight/day, as previously described. At weaning, immature rats were dispatched. Female offspring were randomized (one female per litter), identified by implanted chips, and fed the purified diet until sacrifice (PND 35 and PND 50). Twenty pubertal or cycling female offspring animals per treatment group were used for subsequent analysis
Extracted molecule total RNA
Extraction protocol Total RNA was extracted from individual mammary glands with Trizol extraction.
Label biotin
Label protocol cDNA is end labelled with biotin using Terminal Transferase (using the WT terminal labelling kit of Affymetrix)
 
Hybridization protocol cDNA is then hybridized to GeneChip® rat Gene (Affymetrix) at 45°C for 17 hours
Scan protocol After overnight hybridization, chips are washed on the fluidic station FS450 following specific protocols (Affymetrix) and scanned using the GCS3000 7G
Data processing Raw data were preprocessing using the Robust Multichip Algorithm
 
Submission date Sep 27, 2011
Last update date Mar 01, 2012
Contact name Florent Dumont
E-mail(s) florent.dumont@u-psud.fr
Organization name Université Paris-Saclay
Street address 17 avenue des sciences
City 91400 Orsay
State/province Ile de France
ZIP/Postal code 91400
Country France
 
Platform ID GPL6247
Series (1)
GSE32432 Expression data from in utero exposure to genistein, vinclozolin and the mixture of genistein and vinclozolin on the mammary gland

Data table header descriptions
ID_REF
VALUE Log expression signal

Data table
ID_REF VALUE
10701620 5.04712
10701630 2.81928
10701632 3.2563
10701636 4.50614
10701643 3.04653
10701648 3.72224
10701654 3.90548
10701663 6.47298
10701666 4.52552
10701668 6.31325
10701671 4.09422
10701674 4.79975
10701679 5.00498
10701684 6.28981
10701689 7.67439
10701691 7.05277
10701697 8.20451
10701699 7.24915
10701709 9.6982
10701714 5.9616

Total number of rows: 27342

Table truncated, full table size 450 Kbytes.




Supplementary file Size Download File type/resource
GSM802605.CEL.gz 4.2 Mb (ftp)(http) CEL
Processed data included within Sample table

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