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Sample GSM19189 Query DataSets for GSM19189
Status Public on Mar 27, 2004
Title GH Treated Male-Male(cy3-cy5) #3-RL
Sample type RNA
 
Channel 1
Source name frozen adult male rat liver tissue prepared using Trizol
Organism Rattus norvegicus
Extracted molecule total RNA
 
Channel 2
Source name frozen adult male rat liver tissue prepared using Trizol
Organism Rattus norvegicus
Extracted molecule total RNA
 
 
Description The genetic expression profile for one male and one female continuous GH treated male liver sample is given as a lowess normalized ratio (f=0.2). This result is from a single random pairing of one of four males and one of four GH treated males. The purpose of this pairwise comparison is to highlight the GH-dependent differences in rat liver gene expression.

Technical Aspects: Adult male and female Fischer 344 rats (8-10 weeks of age) were untreated or were treated with rat growth hormone (GH) (NIDDK, rGH-B-14-SIAFP) given as a continuous infusion using an Alzet osmotic minipump delivering 2 ug GH/100g body weight/h for 7 days. Intact male and female rats were killed and their livers were collected, frozen in liquid N2 and stored at –80ºC. Total liver RNA was isolated from frozen liver samples using Trizol reagent (Invitrogen). Poly(A) RNA was then isolated using a commercial kit (Ambion). RNA samples having an A260/A280 ratio >= 1.8 were deemed suitable for use in subsequent analyses. Total liver RNA and poly(A) RNA samples were treated with DNase I (Ambion). Poly(A) RNA purified from individual livers was labeled with Cy3-dUTP or Cy5-dUTP (PerkinElmer) in a reverse transcription reaction using 1 ug poly(A) RNA and Superscript II (RNase H mutant) enzyme (Invitrogen) at 39oC for 2 hr. Unincorporated dNTPs were removed using the Qiaquick PCR-purification kit (Qiagen). Cy5-labeled male liver cDNA was mixed with Cy3-labeled female or Cy3-labeled GH-treated male liver cDNA followed by co-hybridization of the mixed cDNA population to the microarray for 18 hr at 42oC. Arrays were washed according to the manufacturer’s protocol. RNA from each of four male, female, and GH-treated male livers was converted to cDNA and labeled in duplicate. One series of eight hybridizations (four male + female liver cDNA pairings, and four male + male with GH cDNA pairings) was carried out on MWG Rat Liver arrays. A second series containing the same eight hybridizations was carried out on MWG Rat 5K arrays. The fluorescent cDNA on each microarray was detected using a GenePix 4000B array scanner (Axon Instruments). The data was preprocessed using GenePix Pro 3.0 (Axon Instruments) and analyzed in GeneSpring 6.0 (Silicon Genetics). Any spot where there was no fluorescence is reported as 0. The normalized average ratio is given for all duplicates.

Keywords = Growth hormone
Keywords = liver sexual dimorphism
Keywords = cytochrome P450
Keywords = liver gene expression
Keywords = dual channel cDNA microarray
 
Submission date Mar 25, 2004
Last update date Oct 28, 2005
Contact name David J. Waxman
E-mail(s) djw@bu.edu
Organization name Boston University
Department Department of Biology and Bioinformatics Program
Street address 5 Cummington Mall
City Boston
State/province MA
ZIP/Postal code 02215
Country USA
 
Platform ID GPL529
Series (1)
GSE1146 Sex-dependent and growth hormone (GH)-dependent gene expression

Data table header descriptions
ID_REF
VALUE log ratio (log2 of PRE_VALUE)
PRE_VALUE Lowess Normalized Ratio

Data table
ID_REF VALUE PRE_VALUE
1.1.1.1 -0.3309733 0.795
1.1.1.2 0.1296133 1.094
1.1.1.3 0.3972553 1.317
1.1.1.4 -0.3492353 0.785
1.1.1.5 0.3045113 1.235
1.1.1.6 0.1966073 1.146
1.1.1.7 -0.1811493 0.882
1.1.1.8 -0.0694523 0.953
1.1.1.9
1.1.1.10 0.2178513 1.163
1.1.1.11 0.0635033 1.045
1.1.1.12 0.0028833 1.002
1.1.1.13 -0.0619023 0.958
1.1.1.14 0.3862593 1.307
1.1.1.15 -0.3309733 0.795
1.1.2.1 0.4038133 1.323
1.1.2.2 0.2630343 1.2
1.1.2.3 0.3253863 1.253
1.1.2.4 0.1557493 1.114
1.1.2.5 0.0043223 1.003

Total number of rows: 1440

Table truncated, full table size 34 Kbytes.




Supplementary data files not provided

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