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Sample GSM343317 Query DataSets for GSM343317
Status Public on Nov 18, 2008
Title Eilenburg-0 vs RIL2019 (R/G)
Sample type RNA
 
Channel 1
Source name Eilenburg-0
Organism Arabidopsis thaliana
Characteristics Arabidopsis thaliana accession Eil-0
Growth protocol stratified for 48 hrs at 4°C, grown in tissue culture on basic solid medium with macro- and micronutrients (0.5 x MS) and 0.9% agar (Duchefa, Netherlands), supplemented with 2% sucrose at 21°C under continuous light of 130 μE intensity. Plant material for RNA analysis was harvested at 9 days after germination.
Extracted molecule total RNA
Extraction protocol Total RNA from plants was isolated using the Plant RNeasyTM kit (QIAGEN, Netherlands) according to the manufacturer’s instructions.
Label Cy5
Label protocol Total RNA from the seedling pools was amplified using the MessageAmpTM aRNA II kit (Ambion, NY, U.S.A.). 5 microgram of amplified RNA were reverse transcribed into cyanin3 or cyanin 5 labeled cDNA, purified with QiaquickTM columns (Qiagen, Netherlands) and hybridized on custom microarrays (GEO accession number GPL6147)
 
Channel 2
Source name RIL2019
Organism Arabidopsis thaliana
Characteristics Recombinant inbred line from a cross between Eil-0 and Lc-0
Growth protocol stratified for 48 hrs at 4°C, grown in tissue culture on basic solid medium with macro- and micronutrients (0.5 x MS) and 0.9% agar (Duchefa, Netherlands), supplemented with 2% sucrose at 21°C under continuous light of 130 μE intensity. Plant material for RNA analysis was harvested at 9 days after germination.
Extracted molecule total RNA
Extraction protocol Total RNA from plants was isolated using the Plant RNeasyTM kit (QIAGEN, Netherlands) according to the manufacturer’s instructions.
Label Cy3
Label protocol Total RNA from the seedling pools was amplified using the MessageAmpTM aRNA II kit (Ambion, NY, U.S.A.). 5 microgram of amplified RNA were reverse transcribed into cyanin3 or cyanin 5 labeled cDNA, purified with QiaquickTM columns (Qiagen, Netherlands) and hybridized on custom microarrays (GEO accession number GPL6147)
 
 
Hybridization protocol Hybridisation buffer was 3xSSC and 0,4%SDS. Incubation at 64°C O/N without agitation. Washing conditions: twice for 5 minutes in 2xSSC 0.1% SDS, twice for 1 minute in 0.2xSSC, 1 minute in 0.1xSSC, 5 minutes in 0.1xSSC 0.1% TritonX100. All washes at room temperature.
Scan protocol Agilent microarray scanner, 10 μm resolution
Description none
Data processing GenePix Pro 6.0 was used to analyse the images and generate gpr files; raw data without background substraction were print-tip loess normalized to calculate M values. Bioconductor open source software was used for data processing.
 
Submission date Nov 17, 2008
Last update date Nov 17, 2008
Contact name Johann Weber
Organization name University of Lausanne
Department Center for integrative Genomics
Lab DNA array facility
Street address Genopode Building
City Lausanne
State/province VD
ZIP/Postal code CH 1015
Country Switzerland
 
Platform ID GPL6147
Series (1)
GSE13628 Comprehensive analysis of Arabidopsis expression level polymorphisms with simple inheritance

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

Data table
ID_REF VALUE
CATMA2a08450 -0.131631682
CATMA2a08520 -0.059067517
CATMA2a08550 -0.050849694
CATMA2a08580 -0.145275944
CATMA2a22110 -0.402172615
CATMA2a22140 -0.357876459
CATMA2a22155 0.115699515
CATMA2a22180 -0.584365979
CATMA2a32140 0.044266037
CATMA2a32170 0.331511362
CATMA2a32190 -0.560670149
CATMA2a32220 -0.109768715
CATMA2a42070 -3.057325701
CATMA2a42120 -0.496819941
CATMA2a42140 -0.107790507
CATMA2a42160 -0.159581428
CATMA3a00760 -0.417635833
CATMA3a00790 -0.063874763
CATMA3a00810 0.434897724
CATMA3a00830 0.267823927

Total number of rows: 24942

Table truncated, full table size 617 Kbytes.




Supplementary file Size Download File type/resource
GSM343317.gpr.gz 2.0 Mb (ftp)(http) GPR
Processed data included within Sample table

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