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Sample GSM6515 Query DataSets for GSM6515
Status Public on Oct 05, 2003
Title Young Treatment Day 10 #40 C
Sample type RNA
 
Source name soleus muscle
Organism Rattus norvegicus
Extracted molecule total RNA
 
Description II. Experiment Description
1) Experimental Design
· Authors: J. Scott Pattison, Thomas Ellis Childs, Lillian Folk, Richard Madsen, and Frank W. Booth.
· Laboratory: Dr. Frank Booth, University of Missouri-Columbia, 1600 E. Rollins St, Columbia, Mo, 65211
· Contact: [email protected]
· Type of experiment: control young muscle (3-4 months) vs control old muscle (30-31 months).
Experiment 3:
· Experimental Factors: Age, Atrophy, Recovery (Time)
· How many hybridizations in the experiment: 95 unique samples were hybridized once per array x 3 arrays each = 285 separate hybridizations in total.
· Experiment Description: Time course of skeletal muscle recovery following atrophy, comparing young and old responses vs. controls.
· Type of experiment: control young muscle (3-4 months) vs immobilized young muscle (3-4 months) vs. control old muscle (30-31 months) vs. immobilized old muscle (30-31 months) at each of recovery times 0, 3, 6, 10, and 30 days.
2) Samples used, Extract preparation, and Labeling
Ø Biosource properties
· Organism: Rattus Norvegicus
· Animal Source: Harlan Labs, NIA colony
· Sex: male
· Age: 3-4 months or 30-31 months after birth
· Organism part: soleus skeletal muscle
· Cell type: mixed in muscle tissue
· Strain or line: Fischer x Brown Norway F1 rats
· Genetic variation: N/A
· Individual genetic characteristics: N/A
· Disease state or normal: normal
· State of muscle: Young Day 10 Treatment muscle
*The strain of rat used has a propensity for increased longevity over most other strains, due to a failure to develop premature diseases including cancers that shorten the life of other rat strains.

Ø Biomaterial manipulations
· Growth conditions: normal
controlled environment
20-22 ºC average temperature
housed in guinea pig cages 2-3/cage
rubber mats covered the bottoms of cages
12/12 hour light/dark cycle
regular rat chow was provided ad libitum
water was available ad libitum
½” x 3” poplar dowel rods doused in apple juice were given for environmental enhancement
· Treatments: N/A
· Tissue handling: both soleus muscles from a single rat were excised, weighed, and immediately frozen in liquid N2, the muscles were then stored at –80ºC until RNA isolation.

Ø Extract preparation
· Extraction method: muscle tissue was powdered over liquid N2 then put into TRIzol solution and homogenized with a Polytron homogenizer for 3 bouts of 15 seconds on setting 7. Total RNA was extracted as per manufacturer instructions. Total RNA from each sample was used to prepare biotinylated target RNA, with minor modifications from the manufacturers recommendations (http://www.affymetrix.com/support/technical/manual/expression_manual.affx). Briefly, 10 µg of total RNA was used to generate first-strand cDNA by using a T7-oligo(dT24) primer. Following, second-strand synthesis, in vitro transcription was performed with biotinylated UTP and CTP (Enzo Diagnostics), resulting in approximately 100-fold amplification of RNA. Finally, the biotinylated populations of cRNA were fragmented according to the linked protocol. A complete description of procedures is available at (http://www.affymetrix.com/support/technical/manual/expression_manual.affx).
· Minor modifications: All incubations were done in a thermocycler instead of a water bath, cDNA was quantified follwing cDNA synthesis, prior to in vitro transcription, using a PicoGreen kit (Molecular Probes). One microgram of cDNA was then in vitro transcribed.
· Target Preparation: Target cDNA generated from each sample were then processed as per manufacturer's recommendation using an Affymetrix GeneChip Instrument System (http://www.affymetrix.com/support/technical/manual/expression_manual.affx).
· Quality control: The quality and amount of starting RNA, cDNA, cRNA, and fragmented cRNA were confirmed using agarose gel analyses.
· Spike controls: Briefly, spike controls were added to 10 µg fragmented cRNA before prior to hybridization. A complete description of these procedures is available at (http://www.affymetrix.com/support/technical/manual/expression_manual.affx).

Ø Hybridization Procedures
· Hybridization: Arrays were pre-hybridized, loaded, and hybridized for 16 hours prior to washing and staining. A complete description of these procedures is available at (http://www.affymetrix.com/support/technical/manual/expression_manual.affx
· Washing and Staining: Arrays were then washed and stained with streptavidin-phycoerythrin, before being scanned on an Affymetrix GeneChip scanner. A complete description of these procedures is available at (http://www.affymetrix.com/support/technical/manual/expression_manual.affx).

Ø Measurement data and specifications of data processing
· Scanning: The scanning protocols are available at (http://www.affymetrix.com/support/technical/manual/expression_manual.affx).
· Raw Image Analysis/Quality Control: After scanning, array images were assessed to confirm scanner alignment. The corners were examined by eye for proper grid alignment. Images were also scanned for the absence of bubbles, scratches, and speckling. If any images with small scratches or speckles that skewed >25% of a given feature, that feature was masked and not quantitated in future analyses. 3'/5' ratios for GAPDH and beta-actin were confirmed to be ~1.0. From the QC report, spike controls were found to be present on all chips, with BioB, BioC, BioD and CreX being found present in increasing intensity.
· Scaling/Normalization: All data were scaled to a target intensity of 1500 (using Affymetrix MAS 5.0 array analysis software), scaling factors for all arrays were within acceptable limits, as were background, and mean intensities. No further normalization was applied.
· Data Analysis:
· Experiment 3:
· Only those probe sets found to be called “present” or “marginal” in > 60% of all samples in an age group were statistically analyzed. The signal values for all sufficiently detected probe sets were analyzed for significant differences via a 3-way ANOVA. A Bonferroni adjustment was applied to all data to control for multiple testing, where a Bonferroni-adjusted p<0.05 were considered significant.
· The final list of statistically changing genes can be found at (Supporting Data to be linked to journal web site upon paper acceptance)
 
Submission date May 08, 2003
Last update date Oct 28, 2005
Contact name Scott Pattison
E-mail(s) [email protected]
Phone 573.882.0820
Organization name University of Missouri
Street address
City Columbia
State/province MO
ZIP/Postal code 65211
Country USA
 
Platform ID GPL87
Series (1)
GSE353 Effect of age on skeletal muscle

Data table header descriptions
ID_REF
Row Row in source file (administrative only)
Source_File Source filename (administrative only)
Stat_Pairs Affymetrix MAS 5.0 The number of probe pairs in the probe set
Stat_Pairs_Used Affymetrix MAS 5.0 The number of probe pairs in the probe set used in the Detection call
VALUE Affymetrix MAS 5.0 A quantitative measure of the relative abundance of a transcript
ABS_CALL Affymetrix MAS 5.0 A qualitative measurement indicating if the transcript is detected (Present), not detected (Absent), or marginally detected (Marginal)
Detection_p-value Affymetrix MAS 5.0 A p-value indicating the significance of the Detection call

Data table
ID_REF Row Source_File Stat_Pairs Stat_Pairs_Used VALUE ABS_CALL Detection_p-value
AFFX-MurIL2_at 1 Y_Imm_10d_#40_RG_U34C 20 20 12.9 A 0.672921
AFFX-MurIL10_at 2 Y_Imm_10d_#40_RG_U34C 20 20 5.7 A 0.814869
AFFX-MurIL4_at 3 Y_Imm_10d_#40_RG_U34C 20 20 2.1 A 0.749204
AFFX-MurFAS_at 4 Y_Imm_10d_#40_RG_U34C 20 20 21.8 A 0.41138
AFFX-BioB-5_at 5 Y_Imm_10d_#40_RG_U34C 20 20 189.8 P 0.018281
AFFX-BioB-M_at 6 Y_Imm_10d_#40_RG_U34C 20 20 345.3 P 0.001796
AFFX-BioB-3_at 7 Y_Imm_10d_#40_RG_U34C 20 20 139.7 P 0.01667
AFFX-BioC-5_at 8 Y_Imm_10d_#40_RG_U34C 20 20 639.3 P 0.000195
AFFX-BioC-3_at 9 Y_Imm_10d_#40_RG_U34C 20 20 398.7 P 0.000195
AFFX-BioDn-5_at 10 Y_Imm_10d_#40_RG_U34C 20 20 596.7 P 0.000857
AFFX-BioDn-3_at 11 Y_Imm_10d_#40_RG_U34C 20 20 4333.5 P 0.000169
AFFX-CreX-5_at 12 Y_Imm_10d_#40_RG_U34C 20 20 5239.6 P 0.000044
AFFX-CreX-3_at 13 Y_Imm_10d_#40_RG_U34C 20 20 8945.4 P 0.000044
AFFX-BioB-5_st 14 Y_Imm_10d_#40_RG_U34C 20 20 40.8 A 0.368438
AFFX-BioB-M_st 15 Y_Imm_10d_#40_RG_U34C 20 20 29.2 A 0.544587
AFFX-BioB-3_st 16 Y_Imm_10d_#40_RG_U34C 20 20 15.4 A 0.868639
AFFX-BioC-5_st 17 Y_Imm_10d_#40_RG_U34C 20 20 14.4 A 0.9273
AFFX-BioC-3_st 18 Y_Imm_10d_#40_RG_U34C 20 20 6.4 A 0.891021
AFFX-BioDn-5_st 19 Y_Imm_10d_#40_RG_U34C 20 20 32 A 0.425962
AFFX-BioDn-3_st 20 Y_Imm_10d_#40_RG_U34C 20 20 28.6 A 0.300606

Total number of rows: 8790

Table truncated, full table size 548 Kbytes.




Supplementary data files not provided

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