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Sample GSM395592 Query DataSets for GSM395592
Status Public on Apr 12, 2016
Title Hybrid weakness, root of a parental cultivar, Jamaica, biological rep1
Sample type RNA
 
Source name Root, two-week old seedling of Jamaica
Organism Oryza sativa Japonica Group
Characteristics subspecies: japonica
cultivars: Jamaica
Treatment protocol Collected biological samples were frozen in liquid nitrogen and kept at -80˚C until RNA extraction.
Growth protocol Plants were aseptically germinated and cultivated on MS medium at 25˚C under continuous light (20 Em–2 s–1). After two weeks cultivation, seedlings were used for measurement.
Extracted molecule total RNA
Extraction protocol Total RNA was extracted with RNeasy plant mini kit (Qiagen) according to manufacturer's protocol.
Label Cy3
Label protocol Cy3-labeled cRNA were prepared from 100 ng of total RNA using Quick-Amp Labeling Kit (Agilent) according to manufacturer's protocol.
 
Hybridization protocol Fragmentation and hybridization was carried out with Gene Expression Hybridization Kit (Agilent). 400 ng 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.
Description Gene expression of normal roots of a parental cultivar, 'Jamaica'.
Data processing Scanned tiff image files were analyzed with FeatureExtraction 9.5.3.1 (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 median per chip, and the lowest value of scaled signal intensity was set to 0.01. Normalized signal intensities of some probes locating multiple positions on a array were average values of all corresponding probes.
 
Submission date Apr 21, 2009
Last update date Apr 12, 2016
Contact name Nori Kurata
E-mail(s) nkurata@nig.ac.jp
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)
GSE15755 Microarray analysis of a hybrid weakness in the cross between rice cultivars

Data table header descriptions
ID_REF
VALUE Normalized signal intensity

Data table
ID_REF VALUE
Os01g0100100|COMBINER_EST|CI448596|0 2.3063173
Os01g0100200|mRNA|AK059894|CDS+3'UTR 0.10514715
Os01g0100400|mRNA|AK101455|CDS+3'UTR 1.0068243
Os01g0100500|mRNA|AK067316|CDS+3'UTR 4.979232
Os01g0100600|mRNA|AK121362|CDS+3'UTR 3.2744467
Os01g0100700|mRNA|AK059844|CDS+3'UTR 23.85398
Os01g0100700|mRNA|AK121523|CDS+3'UTR 5.0885944
Os01g0100800|mRNA|AK122012|CDS+3'UTR 1.719807
Os01g0100900|COMBINER_EST|CI015509|0 8.491885
Os01g0101200|mRNA|AK067866|CDS+3'UTR 0.29866466
Os01g0101200|mRNA|AK104517|CDS+3'UTR 2.0674672
Os01g0101200|mRNA|AK104625|CDS+3'UTR 2.6477776
Os01g0101200|mRNA|AK104752|CDS+3'UTR 2.3014185
Os01g0101200|mRNA|AK119457|CDS+3'UTR 0.019138264
Os01g0101300|COMBINER_EST|CI016681|6 2.0148666
Os01g0101600|mRNA|AK099952|CDS+3'UTR 0.23758842
Os01g0101600|mRNA|AK103820|CDS+3'UTR 2.47944
Os01g0101600|mRNA|AK122118|CDS+3'UTR 2.4120295
Os01g0101700|COMBINER_EST|CI525185|3 1.6935823
Os01g0101800|mRNA|AK103498|CDS+3'UTR 0.7912086

Total number of rows: 42477

Table truncated, full table size 1928 Kbytes.




Supplementary file Size Download File type/resource
GSM395592.txt.gz 7.5 Mb (ftp)(http) TXT
Processed data included within Sample table

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