NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM526874 Query DataSets for GSM526874
Status Public on Dec 01, 2010
Title Egg cell_rep3
Sample type RNA
 
Source name Egg cell, replicate 3
Organism Oryza sativa
Characteristics subspecies: japonica
cultivars: Nipponbare
tissue: Egg cell
Treatment protocol To check influences in gene expression of the isolated cells caused by the transient storage in mannitol solution, we prepared RNA samples derived from ovaries with mannitol treatment and another kind of RNA samples derived from ovaries without mannitol treatment, to look for differences in expression between them. Mannitol treatment consisted of soaking five ovaries in mannitol solution for 8 h.
Growth protocol Wild-type rice plants (Oryza sativa L. cv. Nipponbare) were grown in pots under natural conditions.
Extracted molecule total RNA
Extraction protocol Total RNA was extracted from each cell type and tissue with a PicoPureā„¢ RNA isolation kit (Molecular Devices, Ontario, Canada) following the manufacturer's recommendations. The qualities of the RNA samples were assessed using an RNA 6000 Pico kit on the Agilent 2100 Bioanalyzer (Agilent Technologies, Santa Clara, CA).
Label Cy3
Label protocol Cy3-labeled cRNA were prepared from total RNA using Low RNA Linear Amplification Kit (Agilent) in accordance with the manufacturer's protocol with slight modification. The cDNA synthesis reaction time was extended to 6 hrs.
 
Hybridization protocol Fragmentation and hybridization was carried out with Gene Expression Hybridization Kit (Agilent). 400 - 1400ng of labeled and fragmented cRNA was hybridized to microarray using hybridization oven G2545A (Agilent), and wash step was performed with Gene Expression Wash Buffer Kit (Agilent). All operations were performed according to manufacturer's protocol.
Scan protocol Microarrays were scanned using Agilent DNA microarray scanner G2565BA according to manufacturer's instructions.
Description Gene expression in the rice egg cell
Data processing Scanned tiff image files were analyzed with FeatureExtraction 9.5.1 (Agilent). We slightly modified manufacturer's default extraction protocol called 'GE1-v5_95_Feb07' as follows: 'Background Subtraction Method' was set to 'Average of Negative Control Features', and 'Use Surrogates' was set to 'False'. Then 'gBGSubSignal' columns were extracted from the text data files produced by FeatureExtraction, and introduced into GeneSpring 7.3.1 (Agilent). Positive and negative control features (such as spike-in or dark corner) were removed before data introduction into GeneSpring. Introduced signal intensities were scaled to the 75th percentile per chip (scaled the 75th percentile value was set to 10), and the lowest value of scaled signal intensity was set to 0.01. Microarray intensity values were also normalized per chip by Z score transformation using R software (http://www.r-project.org/).
A scaled data set with the 75th percentile scaling (VALUE) was used in the scatter plot analysis, correlation plot analysis, and to make the lists of the top 10 highly expressed probes. Z-score transformed (per chip) data sets (VALUE2) were also used in the cluster analysis and heat map analysis.
 
Submission date Mar 25, 2010
Last update date Feb 25, 2011
Contact name Nori Kurata
E-mail(s) [email protected]
Phone +81-55-981-6808
Organization name National Institute of Genetics
Lab Plant genetics Lab.
Street address 1111 Yata
City Mishima
State/province Shizuoka
ZIP/Postal code 411-8540
Country Japan
 
Platform ID GPL8852
Series (1)
GSE21074 Gene expression profiles of the egg and synergid cell in rice

Data table header descriptions
ID_REF
VALUE The 75th percentile scaled data
VALUE2 Z score transformed data

Data table
ID_REF VALUE VALUE2
Os01g0100100|COMBINER_EST|CI448596|0 13.19579 -0.067764962
Os01g0100200|mRNA|AK059894|CDS+3'UTR 0.93664616 -0.153809405
Os01g0100400|mRNA|AK101455|CDS+3'UTR 1.6352068 -0.14890635
Os01g0100500|mRNA|AK067316|CDS+3'UTR 1.4631243 -0.150114162
Os01g0100600|mRNA|AK121362|CDS+3'UTR 10.449771 -0.08703872
Os01g0100700|mRNA|AK059844|CDS+3'UTR 280.71545 1.809901286
Os01g0100700|mRNA|AK121523|CDS+3'UTR 84.675644 0.43393754
Os01g0100800|mRNA|AK122012|CDS+3'UTR 4.7708116 -0.126898178
Os01g0100900|COMBINER_EST|CI015509|0 23.195086 0.002418058
Os01g0101200|mRNA|AK067866|CDS+3'UTR 0.22370656 -0.158813384
Os01g0101200|mRNA|AK104517|CDS+3'UTR 2.1663098 -0.145178647
Os01g0101200|mRNA|AK104625|CDS+3'UTR 1.2342113 -0.151720856
Os01g0101200|mRNA|AK104752|CDS+3'UTR 1.3478596 -0.150923182
Os01g0101200|mRNA|AK119457|CDS+3'UTR 0.11895872 -0.159548587
Os01g0101300|COMBINER_EST|CI016681|6 6.2719016 -0.116362329
Os01g0101600|mRNA|AK099952|CDS+3'UTR 3.118312 -0.138496738
Os01g0101600|mRNA|AK103820|CDS+3'UTR 2.5321164 -0.142611123
Os01g0101600|mRNA|AK122118|CDS+3'UTR 2.3031843 -0.144217953
Os01g0101700|COMBINER_EST|CI525185|3 7.52306 -0.107580706
Os01g0101800|mRNA|AK103498|CDS+3'UTR 21.30685 -0.010835098

Total number of rows: 42477

Table truncated, full table size 2453 Kbytes.




Supplementary file Size Download File type/resource
GSM526874.txt.gz 7.6 Mb (ftp)(http) TXT
Processed data included within Sample table

| NLM | NIH | GEO Help | Disclaimer | Accessibility |
NCBI Home NCBI Search NCBI SiteMap