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Sample GSM265963 Query DataSets for GSM265963
Status Public on Jun 01, 2008
Title Low capacity runner-soleus-trained-3
Sample type RNA
 
Source name Low capacity runner, Soleus muscle, trained-3
Organism Rattus norvegicus
Characteristics Low capacity runner, Soleus muscle, trained-3
Biomaterial provider National Institutes of Health (USA)
Treatment protocol 4 rats from each strain was exposed to an aerobic interval training program. Briefly, after 10 minutes of warm-up, rats ran uphill (25°) on a treadmill for 1.5 hours, alternating between 8 minutes at an exercise intensity corresponding to 85-90% of VO2max, and 2 minutes active recovery at 50 - 60%. Exercise was performed 5 days per week over 8 week; controls were age-matched rats that remained sedentary. We measured VO2max every week in exercising rats to adjust speed in order to maintain the intended intensity throughout the experimental period. The VO2max-testprotocol consisted of 20 minutes warm-up at 50-60% of VO2max, whereupon treadmill velocity was increased by 0.03 m/s every 2 minute until VO2 plateau despite of increased workload. The animals in the sedentary groups were treated similar to the exercise groups, except being exposed to exercise training and VO2max-tests.
At approximately 7 months of age, and 48 hours after the last exercise session all the animals were sacrificed. One of the soleus muscles was formalin fixated for immunohistochemistry and morphological studies, whereas the other was snap frozen in liquid nitrogen and stored at -80oC for later genetic screening and protein analysis.
Extracted molecule total RNA
Extraction protocol Tissue samples (20 mg) were homogenized in 100 µL TRIzol (Life Technologies, Gaithersburg, MD) using a Mixer Mill MM301 (Company, City, State/Country) at 20-25 Hz. RNA clean-up was performed using RNA Mini kit (Qiagen, Germantown, MD). Total RNA was isolated and RNA clean up was performed according to the manufacturer's instructions.
RNA integrity, purity and quantity were assessed by Bioanalyzer (Agilent Technologies, Santa Clara, CA) and Nanodrop (NanoDrop Technologies, Baltimore, MD). The concentration of total RNA was measured by Nanodrop with ultraviolet spectrophotometry at 260/280 nm. RNA quality was assessed by electrophoresis on Bioanalyzer chips (Agilent Technologies).
High quality RNA was classified as a 260/280 ratio above 1.8. Only samples with a 260/280 ratio between 1.8-2.2 and no signs of degradation were used for analysis.
Label biotin
Label protocol According to manufacture's instructions.
 
Hybridization protocol According to manufacture's instructions. Labeled cRNA was prepared and hybridized to the RAE 230 2.0 chip from Affymetrix GeneChip (Affymetrix, Santa Clara, CA) comprised of 31,042 probe sets. On the Affymetrix GeneChip arrays, each gene is represented by a set of 11-20 probe pairs consisting of a perfect match (PM) and a mismatch (MM) probe. The statistical analysis is based on summary expression measures for each probe set.
Scan protocol According to manufacture's instructions.
Description We used rats artificial selected for high and low aerobic capacity, starting from the N: NIH stock obtained from the National Institutes of Health (USA). Briefly, the rats in each generation were tested for exercise capacity by treadmill running at 11 weeks of age. The individuals with the highest and lowest running capacity were selected and each group served as the mating population for the next generation. Female rats from generation 16 were used in this study. The study includes four groups; LCR trained (LCR-T) (n=4), LCR sedentary (LCR-S) (n=4), HCR trained (HCR-T) (n=4) and HCR sedentary (HCR-S) (n=4). Experimental protocols were approved by the respective Institutional Animal Research Ethics Councils
Data processing Computing summary measures (RMA)
The summary measure for each probeset is computed based on a linear statistical model for background-corrected, normalized and log-transformed PM values for each probe pair by use of the robust multiarray average (RMA) method. The PM values are normalized using the quantile normalization method, normalizing the arrays such that the empirical distribution of the expression measures is equal across arrays.
Statistical analysis for finding differentially expressed genes
For each gene (probeset), a linear regression model, including parameters representing the effect of aerobe capacity is specified. Based on the estimated effects, tests for significant differential expression are performed using moderated T-tests.
To account for multiple testing, we calculated adjusted p-values controlling the False Discovery Rate (FDR), with the use of the Benjamini-Hochberg step-up procedure. Consequently, selecting differentially expressed genes based on a threshold of 0.05 on the adjusted FDR p-values means that the expected proportion of genes falsely classified as differential expressed should be below 0.05.
All statistical analyses on the gene expression data are performed using the R language (R Development Core Team, 2004) and packages affy, affyPLM and limma from the Bioconductor project.
 
Submission date Feb 14, 2008
Last update date Mar 22, 2008
Contact name Anja Bye
E-mail(s) [email protected]
Organization name NTNU
Street address Olav Kyrres gt 9
City TRONDHEIM
ZIP/Postal code 7489
Country Norway
 
Platform ID GPL1355
Series (1)
GSE10527 Genome-wide gene expression in soleus muscle of rats artificially selected for high and low running capacity

Data table header descriptions
ID_REF
VALUE Gene expression

Data table
ID_REF VALUE
1367452_at 10.5681824139908
1367453_at 10.8879340798014
1367454_at 9.63329899835858
1367455_at 11.5765528979032
1367456_at 11.4014055792078
1367457_at 9.24434209028176
1367458_at 8.28750425875128
1367459_at 11.3272787792179
1367460_at 11.0000819240337
1367461_at 8.82517577081025
1367462_at 11.0223537444561
1367463_at 11.2061489511816
1367464_at 9.76536963286364
1367465_at 9.26672465520263
1367466_at 10.1248810406700
1367467_at 11.6024462245276
1367468_at 9.30213060630884
1367469_at 12.1592986173306
1367470_at 10.3876850728696
1367471_at 9.80762483907781

Total number of rows: 31099

Table truncated, full table size 849 Kbytes.




Supplementary file Size Download File type/resource
GSM265963.CEL.gz 2.7 Mb (ftp)(http) CEL
Processed data included within Sample table

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