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Sample GSM1036145 Query DataSets for GSM1036145
Status Public on Nov 14, 2012
Title wt-matA-sv071-b
Sample type RNA
 
Channel 1
Source name wt-matA
Organism Saccharomyces cerevisiae
Characteristics strain: BY4742
genotype: wt-matA
Growth protocol yeast-deleteome[grow]
Extracted molecule nuclear RNA
Extraction protocol yeast RNA isolation for robotic amplification v1.0
Label Cy5
Label protocol robot amplification and labeling v1.0
 
Channel 2
Source name refpool
Organism Saccharomyces cerevisiae
Characteristics strain: BY4742
genotype: refpool
Growth protocol yeast-deleteome[grow]
Extracted molecule nuclear RNA
Extraction protocol yeast RNA isolation for robotic amplification v1.0
Label Cy3
Label protocol robot amplification and labeling v1.0
 
 
Hybridization protocol Tecan HS4800 hybridization
Scan protocol scanning of slides using Agilent G256BA
Imagene feature extraction
Description Strains were streaked from -80C stocks onto plates and grown for 3-5 days depending on growth rate. Liquid cultures were inoculated with independent colonies and grown overnight in Synthetic Complete (SC) medium: 2gr/l Drop out mix Complete and 6.71gr/l Yeast Nitrogen Base without AA, Carbohydrate and w/AS (YNB) from US Biologicals (Swampscott, USA) with 2percent D-glucose. Overnight cultures were diluted to an OD600 of 0.15 in 1.5 ml fresh medium and grown at 30C in a 24 well plate in a Tecan Infinite F200 under continuous shaking. Growth curves were made for the mutant cultures (two cultures from two isolates) as well as for two wildtype (wt) inoculates, grown in parallel. Mutant and wt cells were harvested by centrifugation (6100 rpm, 3 min) at mid-log phase at an OD600 of 0.6, and pellets were immediately frozen in liquid nitrogen after removal of supernatant. S. cerevisiae BY4742 deletion mutants and the wild-type strains were cultured in SC Medium (Synthetic Complete; 4gr per 2l Drop out mix 13.42gr per 2l YNB(US biologicals) with 2percent D-glucose)under agitation (230rpm), at 30C. The cells were collected at midlog.
Data processing Normalization was done using print-tip LOESS as described in (Yang et al. 2002), by estimating the LOESS curve for all gene probes using no background substraction and a span of 0.4. Probes flagged as absent, or with a (nearly) saturated signal (i.e., > 2^15) in either channel were not considered for the estimation of the LOESS curve. Signals were corrected for dye bias using intrinsic gene-specific dye biases estimated from a set of wild-type wild-type hybridizations, as described in Margaritis, Lijnzaad et al., Mol. Sys. Biol. 2009.
 
Submission date Nov 13, 2012
Last update date Nov 14, 2012
Contact name Patrick Kemmeren
Organization name UMC Utrecht
Department Department of Molecular Cancer Research
Lab Holstege Lab
Street address Universiteitsweg 100
City Utrecht
State/province Utrecht
ZIP/Postal code 3584 CG
Country Netherlands
 
Platform ID GPL11232
Series (2)
GSE42240 yeast wt-matA pool
GSE45115 Expression profiling of 376 wildtypes to assess day-to-day variance

Data table header descriptions
ID_REF
VALUE normalized log2 ratio (Cy5/Cy3)
Signal Norm_Cy5
Signal Norm_Cy3

Data table
ID_REF VALUE Signal Norm_Cy5 Signal Norm_Cy3
1 0.012345862 3087.67 3061.36
2 0.002953156 238.645 238.157
3 0.0459721 505.18 489.336
4 -0.065122433 53.1861 55.6419
5 -0.075082652 447.012 470.892
6 -0.183758702 123.44 140.208
7 -0.015942636 435.39 440.228
8 0.055603441 931.758 896.53
9 -0.025816915 322.386 328.207
10 -0.029008018 66.961 68.321
11 -0.08624695 3681.2 3907.98
12 -0.101647098 103.373 110.919
13 -0.045289369 163.248 168.454
14 -0.060545676 172.118 179.495
15 0.067167324 2573.33 2456.27
16 0.244964075 117.212 98.9078
17 0.230024 124.909 106.5
18 -0.110484487 8496.97 9173.25
19 -0.140545704 9516.82 10490.6
20 -0.054531936 747.96 776.773

Total number of rows: 15552

Table truncated, full table size 507 Kbytes.




Supplementary file Size Download File type/resource
GSM1036145_4129_raw.txt.gz 682.8 Kb (ftp)(http) TXT
Processed data included within Sample table

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