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Sample GSM2358945 Query DataSets for GSM2358945
Status Public on Jun 20, 2017
Title chip7_0Cu_Cy3_75Cu_Cy5 Replicate 3
Sample type RNA
 
Channel 1
Source name Seedlings
Organism Oryza sativa
Characteristics treatment: 0µM CuSO4
variety: Nippombare
age: 8 days
Treatment protocol Rice (Oryza sativa subsp japonica), cv. Nipponbare, seeds were surface-sterilized and stratified for 2 d at 4° C, and then germinated on ½MS plates with 1% Sucrose (Murashige and Skoog 1962). Two different Cu concentration conditions were compared, slight Cu deficiency (0 µM CuSO4) and Cu excess (75 µM CuSO4).
Growth protocol The plants were cultured in plates during 8 days under diferent concentration of CuSO4 in the medium.
Extracted molecule total RNA
Extraction protocol Total RNAs were isolated with the RNeasy plant mini kit (QIAgen, Hilden, Germany; Ref. 74904), following the manufacturer’s instructions. The aRNA amplification and labeling were performed with the AminoAllyl MessageAmpTM II aRNA Amplification kit (Ambion) according to the manufacturer’s instructions. One microgram of total RNA of each sample was used for the amplification. The final concentration of obtained aRNA was determined with NanoDrop ND1000 Spectrophotometer.
Label Cy3
Label protocol The obtained amplified RNA (aRNA) was labeled by using the CyDye Post-Labeling Reactive Dye Pack, which generates fluorescent Cy3- and Cy5-labeled probes by a post-labeling (amino allyl) method (GE Healthcare). Each biological replicate was labeled with Cy3 and Cy5 to produce four pairs of replicate dye-swaps, which were used for microarray hybridization
 
Channel 2
Source name Seedlings
Organism Oryza sativa
Characteristics treatment: 75µM CuSO4
variety: Nippombare
age: 8 days
Treatment protocol Rice (Oryza sativa subsp japonica), cv. Nipponbare, seeds were surface-sterilized and stratified for 2 d at 4° C, and then germinated on ½MS plates with 1% Sucrose (Murashige and Skoog 1962). Two different Cu concentration conditions were compared, slight Cu deficiency (0 µM CuSO4) and Cu excess (75 µM CuSO4).
Growth protocol The plants were cultured in plates during 8 days under diferent concentration of CuSO4 in the medium.
Extracted molecule total RNA
Extraction protocol Total RNAs were isolated with the RNeasy plant mini kit (QIAgen, Hilden, Germany; Ref. 74904), following the manufacturer’s instructions. The aRNA amplification and labeling were performed with the AminoAllyl MessageAmpTM II aRNA Amplification kit (Ambion) according to the manufacturer’s instructions. One microgram of total RNA of each sample was used for the amplification. The final concentration of obtained aRNA was determined with NanoDrop ND1000 Spectrophotometer.
Label Cy5
Label protocol The obtained amplified RNA (aRNA) was labeled by using the CyDye Post-Labeling Reactive Dye Pack, which generates fluorescent Cy3- and Cy5-labeled probes by a post-labeling (amino allyl) method (GE Healthcare). Each biological replicate was labeled with Cy3 and Cy5 to produce four pairs of replicate dye-swaps, which were used for microarray hybridization
 
 
Hybridization protocol From http://ag.arizona.edu/microarray/Microarraymethod1.doc Microarrays were re-hydrated by exposing them to water vapor for 10 seconds (four times). Next microarrays were cross-linked by ultraviolet (UV) irradiation of 180 mJ in a Stratalinker 1800 UV (Stratagene). Subsequently, microarrays were washed with 1% SDS (w/v) (Sodium Dodecyl Sulfate) for 5 min and 10 times with H2O milliQ (Millipore), washed with 100% ethanol 5 times and then dried by centrifugation at 200 g. After this pre-treatment, microarrays were hybridized overnight at 55 °C with hybridization solution [48 pmol of each labeled sample; deionized formamide 50% (v/v);] 3X SSC (Saline-Sodium Citrate); Denhardt´s solution [5 X and SDS 0.1% (w/v)]. The hybridization solution was denaturalized for 5 min at 65 °C and applied between the microarray and a coverslip LifterSlipTM (Erie Scientific).
Scan protocol The hybridized microarray slides were washed and scanned using a Gene Pix Autoloader (Axon/Molecular Devices, 4200A01, Sunnyvale, CA). Spot finding and data extraction was done using GenePix Pro 6 software (Axon/Molecular Devices, Sunnyvale, CA).
Data processing Quality control, normalization and determination of the differentially expressed genes were conducted in R using the Limma package (Smyth 2005), as previously described in (Andrés et al. 2009). To determine the false-positive ratio (FDR), the P values were adjusted by a test multiple test according to the method of Benjamini and Hochberg´s (Benjamini and Hochberg 1995). The genes that showed a differential expression with fold-change (FC) minimum of 2 for both conditions, represented as log2(FC) ≥ |1|of > 2-fold (-1 > log-fold change [½MS + 75 µM/ ½MS] > 1) with a P value of 0.05 (FDR = 0.5%) were selected.
 
Submission date Oct 24, 2016
Last update date Jun 20, 2017
Contact name Fernando Andres
E-mail(s) andres@mpipz.mpg.de
Organization name Max Planck Institute for Plant Breeding Research
Department Plant Developmental Biology
Lab Prof George Coupland
Street address Carl von Linne 10
City Cologne
ZIP/Postal code 50829
Country Germany
 
Platform ID GPL8756
Series (1)
GSE89109 Global tanscriptome analysis in Oryza sativa identifies genes regulated by copper in the medium

Data table header descriptions
ID_REF
VALUE Log2 fold-change (M-value) ratio (75 µM CuSO4/0 µM CuSO4)

Data table
ID_REF VALUE
TR030001 0.05273267
TR030002 -0.200066571
TR030003 0.286614578
TR030004 -1.542399868
TR030005 -0.28431756
TR030006 -1.709763014
TR030007 -0.553021817
TR030008 1.325767014
TR030009 1.274060719
TR030010 0.673524996
TR030011 1.971632994
TR030012 0.694194096
TR030013 -0.267648004
TR030014 -0.285194788
TR030015 -0.268100089
TR030016 -0.653128032
TR030017 -0.340523517
TR030018 -0.102208887
TR030019 0.397023637
TR030020 -0.371098465

Total number of rows: 43311

Table truncated, full table size 904 Kbytes.




Supplementary file Size Download File type/resource
GSM2358945_chip7.gpr.gz 3.9 Mb (ftp)(http) GPR
Processed data included within Sample table

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