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Sample GSM485641 Query DataSets for GSM485641
Status Public on Dec 15, 2009
Title Ovary harvested at 156 days replicate 3 [compressed]
Sample type RNA
 
Channel 1
Source name ovary (control)
Organism Oncorhynchus mykiss
Characteristics harvested on which day of the normal photoperiod: Day 0
Treatment protocol Post Spawned Female Rainbow Trout over the course of a compressed photoperiod
Extracted molecule total RNA
Extraction protocol Trizol extraction following the manufacturer's protocol
Label Alexa Fluor 555
Label protocol Labelled using I\nvitrogen’s Superscript cDNA Indirect Labeling kit and the manufacturer's protocol, and Alexa fluors.
 
Channel 2
Source name ovary (test)
Organism Oncorhynchus mykiss
Characteristics harvested on which day of the normal photoperiod: Day 156
Treatment protocol Post Spawned Female Rainbow Trout over the course of a compressed photoperiod
Extracted molecule total RNA
Extraction protocol Trizol extraction following the manufacturer's protocol
Label Alexa Fluor 647
Label protocol Labelled using I\nvitrogen’s Superscript cDNA Indirect Labeling kit and the manufacturer's protocol, and Alexa fluors.
 
 
Hybridization protocol Samples were mixed with 20 µg tRNA and 20 µg Herring Sperm DNA to prevent non specific hybridization, then mixed with 35 µl of modified “Genisphere” hybridization buffer (50% formamide, 40% 20x SSC, 9% Denhardt’s solution, 1% SDS). This mixture was then applied to the arrays and allowed to hybridize overnight (16 hr) at 45 o C. After hybridization, arrays were washed in SSC/SDS buffers with descending stringency to remove any unhybridized or weakly (nonspecifically) hybridized cDNA’s.
Scan protocol Arrays were scanned using a Perkin Elmer ScanArray Express, with laser power and PMT gain varied to equalize fluorescence intensity between channels and to prevent over saturation of signal intensity.
Description Biological replicate 3
Data processing Data were extracted using ScanArray Express software (Perkin Elmer). The median fluorescence intensity with background subtracted was imported Genespring microarray analysis software for further analysis. Data were LOWESS normalized and spots that did not meet a minimum signal intensity were removed.
 
Submission date Dec 15, 2009
Last update date Dec 15, 2009
Contact name Sharon E. Hook
E-mail(s) [email protected]
Phone +61 0297106839
Organization name CSIRO
Department Centre for Environmental Contaminants Research
Street address Private Mail Bag 7
City Bangor
State/province NSW
ZIP/Postal code 2234
Country Australia
 
Platform ID GPL2716
Series (1)
GSE19478 Normal and shortened photoperiods in liver, ovary, and pituitarty

Data table header descriptions
ID_REF
VALUE LOWESS normalized log2 ratio (Ch2/Ch1) representing test/control
PRE_VALUE LOWESS normalized ratio (Ch2/Ch1) representing test/control

Data table
ID_REF VALUE PRE_VALUE
01010101 -0.4150 0.75
01010102 0.2570 1.195
01010103 -0.1282 0.915
01010104 0.2265 1.17
01010105 0.0881 1.063
01010106 -0.4266 0.744
01010107 -0.0218 0.985
01010108 -0.1047 0.93
01010109 0.1916 1.142
01010110 0.0412 1.029
01010111 -0.0816 0.945
01010112 0.5079 1.422
01010113 0.0949 1.068
01010114 -0.2396 0.847
01010115 0.3796 1.301
01010116 -0.6215 0.65
01010117 -0.3622 0.778
01010118 -0.3978 0.759
01010119 -0.5500 0.683
01010201 -0.0395 0.973

Total number of rows: 17328

Table truncated, full table size 378 Kbytes.




Supplementary file Size Download File type/resource
GSM485641.txt.gz 1.6 Mb (ftp)(http) TXT
Processed data included within Sample table

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