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Sample GSM344627 Query DataSets for GSM344627
Status Public on Jun 01, 2010
Title T00306153: cardiomyocytes, time zero control
Sample type RNA
 
Source name cardiomyocytes, time zero control
Organism Rattus norvegicus
Characteristics Rat neonatal cardiomyocytes harvested from day 1 ventricles (n=24). Cells purified via serial Percoll gradients and plated at 2.5x10^5 cells per 100 mm sq dish.
Extracted molecule total RNA
Extraction protocol Extracted using Invitrogen Trizol LS Reagent and Invitrogen's RNA isolation protocol supplied with the reagent.
Label biotin
Label protocol GE Healthcare Amersham CodeLink iExpress Assay Reagent Kit protocol
 
Hybridization protocol GE Healthcare Amersham CodeLink Gene Expression System: Single-Assay Bioarray Hybridization and Detection protocol
Detection dye: streptavidin - Alexa Fluor 647
Scan protocol Scanned using a GenePix 4000B at 600 PMT and CodeLink software (version 5.0).
Description No treatment, time zero control
Data processing The threshold was calculated by removing the top 10% and bottom 10% of negative controls and averaging the remaining intensities. The threshold was subtracted from each of the discovery probes. An average was computed for the following positive controls: LEUB, HISB, FIXB, GND, ENTF, and ARAB. The averages of each of these positive controls was grouped together with its average on all the other arrays in this series. By taking the median of each group, a global median was created which represents the median value for a positive control across all of the arrays. Correction factors for this array were calculated by dividing the average of each positive control by its corresponding global median. It was observed that the arrays behaved differently at high intensity levels compared to low intensity levels. As the positive controls increased in intensity, the correction factors also steadily increased or steadily decreased. Therefore, a correction factor derived from a low intensity positive control was not a good correction for high intensity probes. To accommodate for the effect of intensity, the correction factor for each positive control was graphed versus its intensity and a best-fit regression line was created. The equation of the best-fit line was used to calculate a correction factor for each individual discovery probe based on where it fit into the slope of the correction factors. Negative values were replaced by a placeholder of ".0001".
In summary, the data was normalized by comparing each positive control to its median value across arrays and correcting based on the slope of the positive controls versus intensity. Note that the data was never median normalized or log transformed.
 
Submission date Nov 21, 2008
Last update date Jun 16, 2009
Contact name John Michael Krill-Burger
E-mail(s) burgerm@upmc.edu
Phone 412-656-6727
Organization name University of Pittsburgh Medical Center
Street address Rm. WG21.3 Shadyside Hospital
City Pittsburgh
State/province PA
ZIP/Postal code 15232
Country USA
 
Platform ID GPL2896
Series (1)
GSE13708 Stem Cells Secrete Factors That Induce Proliferation In Differentiated Cardiomyocytes

Data table header descriptions
ID_REF
Raw_Intensity Raw Intensity
VALUE Normalized Intensity

Data table
ID_REF Raw_Intensity VALUE
1001 10461.72949 null
1002 20.61538696 5.433662708
1003 null null
1004 94.80000305 64.38533749
1005 11684.40625 10011.39423
1006 1592.807739 1266.806625
1007 12343.41699 null
1008 12967.5 null
1009 217.7647095 162.2232435
1010 20.35713959 5.228540475
1011 52.85713959 31.04811975
1012 423.8999939 326.5803722
1013 2197.166748 1758.484863
1014 12741.625 null
1015 14930.62891 null
1016 21.5625 6.185946943
1017 3.161289215 0.0001
1018 32.5 14.87417093
1019 14.66666412 0.708847236
1020 3218.54834 2598.194904

Total number of rows: 36736

Table truncated, full table size 1010 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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