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Sample GSM3455533 Query DataSets for GSM3455533
Status Public on Dec 10, 2018
Title S-ALR2-6DAF: Stress Aleurone Cell Replicate 2
Sample type RNA
 
Source name AL Aleurone Cell
Organism Oryza sativa
Characteristics cultivar: Koshihikar
tissue: Endosperm
developmental stage: Aleurone Cell
Treatment protocol Control and high temperature condition were set at 26/20 oC and 33/27 oC (day/night), respectively. Day and night length was 13 (0600-1900 h) and 11 (1900-0600 h) hours, respectively. Plants were kept in the chambers from three days after flowering until 30-35 DAF
Growth protocol Rice plants cv. 'Koshihikari' were grown in 1/2000 pots. At three days after flowering (DAF), pots were moved to the naturally-illuminated temperature controlled chamber.
Extracted molecule total RNA
Extraction protocol Developing caryopses was fixed with the ice-cooled mixture of ethanol-acetic acid (3 :1), embeded in 2% carboxymethyl cellulose following the method of Ishimaru et al. (2007). After making the cryo-section, fine tissues of developing endosperm were microdissected with AS LMD system (Leica Microsystems, Germany). Total RNA was extracted with Picopure RNA isolation kit (Arcturus Engineering).
Label Cy5
Label protocol Total RNA (5.0 ng) was amplified to obtain complementary RNA (cRNA) using two-color Quick Amp Labeling kit (Agilent technologies). RNA extracted from control and high-temperature condition was labeled with cyanine-3 (Cy3)-CTP and cyanine-5 (Cy5)-CTP, respectively. Three biological replicates were prepared from high temperature conditions as well under control conditions.
 
Hybridization protocol 1250 ng of labeled cRNAs were fragmented and hydridized on a slide glass of rice 4 × 44K microarray RAP-DB (G2519F#1524 ; Agilent Technologies).
Scan protocol Slides were scanned on an Agilent G2505B DNA microarray scanner, and background of the Cy3 and Cy5 raw signals was corrected using the Feature Exraction (ver. 10.5.1.1, Agilent Technologies).
Description Raw data file: US22502560_251524110215_S01_GE2-v5_91_0806_1_2.txt
A microdissected samples of aluerone cells at 7DAF (days after fertilization) from high-temperature condition;Biological replicate 2 of 3.
Data processing The two channels Agilent microarray expression data of 12 microdissected samples of dorsal aluerone cells (AL), dorsal starchy endosperm (DSE), central starchy endosperm (CSE) and lateral starchy endosperm (LSE) at 7DAF from control and at 6DAF from heat stressed tissues consisting of three replicates was further processed (ratio computation, log transformation and baseline transformation) using the software GeneSpring GX version 12 (Agilent, Santa Carla, CA).
Limma R (Ritchie et al., 2015) package is used following the empirical Bayes method (Smyth, 2004) to shrink the probe-wise sample variances towards a common value and to augmenting the degrees of freedom for the individual variances. The P-values adjustment method was used (Bonferroni, 1936). The top-ranked genes having an adjusted P-value below <=0.05 and log2 fold change above +/- 1 were selected.
 
Submission date Nov 02, 2018
Last update date Dec 10, 2018
Contact name Tsutomu Ishimaru
E-mail(s) [email protected]
Organization name Central Region Agricultural Research Center, National Agriculture and Food Research Organization (CARC/NARO)
Street address 1-2-1 Inada, Joetsu, Niigata
City Niigata
ZIP/Postal code 941-0193
Country Japan
 
Platform ID GPL8852
Series (1)
GSE122115 Laser microdissection-based tissue specific transcriptome analyses reveals novel regulatory network of genes involved in heat-induced grain chalk in rice endosperm.

Data table header descriptions
ID_REF
VALUE Normalized intensity

Data table
ID_REF VALUE
GE_BrightCorner -0.4382887
DarkCorner -0.3199649
Os01g0532600|mRNA|AJ491820|CDS+3'UTR 0.04580307
Os01g0721700|COMBINER_EST|CI557169|4 -0.2588892
Os06g0215600|mRNA|AK104039|CDS+3'UTR -0.29398918
Os09g0379500|mRNA|AK069390|CDS+3'UTR 0.054024696
Os03g0199100|mRNA|AK069890|CDS+3'UTR 0.05374241
Os01g0508500|mRNA|AK120501|CDS+3'UTR -0.48694754
Os06g0130000|mRNA|AK064427|CDS+3'UTR -0.33602095
Os08g0446400|mRNA|AK102368|5'UTR+CDS -0.5792861
Os05g0433800|COMBINER_EST|Os05g0433800|8 -0.75448895
Os12g0152700|mRNA|AK099473|CDS+3'UTR -0.15932274
Os03g0685100|mRNA|AK059852|CDS+3'UTR -0.6991472
Os05g0285900|mRNA|AK061533|CDS+3'UTR -0.15869236
Os03g0449000|COMBINER|CI260116|6 -0.960886
Os03g0775000|COMBINER_EST|AU057613|7 0.035725117
Os11g0213500|COMBINER_EST|Os11g0213500|8 -0.17184544
Os09g0261100|mRNA|AK121607|CDS+3'UTR -0.022657394
Os02g0236600|COMBINER_EST|CI552267|0 -0.3618989
Os10g0469200|mRNA|AK108708|CDS+3'UTR -0.7726083

Total number of rows: 42537

Table truncated, full table size 2000 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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