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Sample GSM149957 Query DataSets for GSM149957
Status Public on Dec 28, 2007
Title Stage1_Vs_Stage6_13111935
Sample type RNA
 
Channel 1
Source name Total RNA from Soybean Cotyledons in Stage 1 of germination
Organism Glycine max
Characteristics Cultivar Williams. Pooled cotyledons from 10 seedlings in Stage 1 of germination/4 different RNA purifications pooled
Biomaterial provider Dr. L. Vodkin’s laboratory. University of Illinois.
Growth protocol Four Glycine max Williams dry seeds were planted per small pot (4 inches) containing pre-wetted Universal Mix SB300 soil in the green house.
Extracted molecule total RNA
Extraction protocol McCarty D. 1986. Phenol Chloroform, Lithium Chloride extraction method
Label Cy3
Label protocol Direct incorporation using Cy3-dUTP
 
Channel 2
Source name Total RNA from Soybean Cotyledons in Stage 6 of germination
Organism Glycine max
Characteristics Cultivar Williams. Pooled cotyledons from 10 seedlings in Stage 6 of germination/4 different RNA purifications pooled
Biomaterial provider Dr. L. Vodkin’s laboratory. University of Illinois.
Growth protocol Four Glycine max Williams dry seeds were planted per small pot (4 inches) containing pre-wetted Universal Mix SB300 soil in the green house.
Extracted molecule total RNA
Extraction protocol McCarty D. 1986. Phenol Chloroform, Lithium Chloride extraction method
Label Cy5
Label protocol Direct incorporation using Cy5-dUTP
 
 
Hybridization protocol A total of 20 µg of the reference Stage 1 (imbibed seed) RNA was used to be labeled by reverse transcription with Cy3-dUTP and compared to 20 µg of RNA from each of stages 2-7 labeled by reverse transcription with Cy5-dUTP following the protocol by Hedge et al., 2000. The Soybean Oligo array slides were pre-hybridized, hybridized and washed as described by Vodkin et al., 2004. Duplicate dye swaps were set up as well.
Scan protocol The hybridized slides were scanned with a ScanArray Express Microarray Scanner, Packard Bioscience/ PerkinElmer (Shelton, CT) and the fluorescence was quantified by using the ScanArray Gx/ProScanArray, Microarray Analysis System (Packard biosciences/Perkin Elmer, Shelton, CT) using a protocol defined by a corresponding GAL file previously generated.
Description Biological replicate 2 Technical replicate 2. The quantitated GPR files were then transferred to GeneSpring 7.2 Agilent Technologies (Palo Alto,CA) for further analysis. For microarray data analysis using GeneSpring 7.2, Agilent Technologies (Palo Alto, CA) we uploaded initially a soybean Genome or Array file containing the corresponding information for each one of the Oligos represented in the array. A systematic name was defined and listed along with its corresponding EST accession number, Clone ID, Blast X (cutoff 10E-06), top hit GI number and its description, top hit Arabidopsis ID and its description, corresponding gene ontologies to top hits, and associated EST’s numbers. This file was uploaded in GeneSpring 7.2 (Silicon Genetics, CA) and was used as the soybean oligo genome information for further analysis.
Data processing Data from a total of 48 slides, containing the intensity values for the reference and the signal channels as well as the flag values for present, absent or marginal spots was uploaded and sample attributes were defined. The data was initially transformed for dye swap for the appropriate slide samples and all the intensity values less than 0.01 or negative were converted to 0.01 to reset biologically irrelevant or otherwise unacceptable expression values. Time was defined as the only parameter to be taken into account for analysis and 6 different conditions were defined: one for each time point defined. After background subtraction and eliminating all the spots flagged as marginal or absent, data was normalized using an intensity-dependent LOWESS (locally weighted scatter plot smoothing) normalization method (Yang et al., 2002) to minimize systematic non-biological differences and standardize chips for cross-array comparisons. Normalized data was then filtered on expression level to obtain a list of genes with expression values in at least one of the comparisons made. This list was then used for statistical analysis. A Welch ANOVA (parametric test, variances not assumed equal) was carried out with a P-value cutoff 0.05, a false discovery rate (FDR) of 0.05 and between 0.1 and 100 fold expression value change. This list was further filtered on expression level creating restrictions to define relevant genes at any particular time point as well as to find expression profiles of biological relevance for the study.
 
Submission date Dec 13, 2006
Last update date Dec 11, 2007
Contact name Lila O. Vodkin
E-mail(s) [email protected]
Phone 217-244-6147
Organization name University of Illinois
Department Crop Sciences
Lab Lila Vodkin
Street address 1201 W. Gregory Dr.
City Urbana
State/province IL
ZIP/Postal code 61801
Country USA
 
Platform ID GPL4635
Series (1)
GSE6534 Glyoxylate pathway elements involved in the functional transition of soybean cotyledons during seedling development

Data table header descriptions
ID_REF
RATIO Normalized ratio of Signal/Lowess adjusted reference
REFERENCE Lowess adjusted Cy3 value
SIGNAL Cy5 value
FLAGS Type of flag associated with a feature from GenePix
VALUE Log2 of Normalized ratio of Signal/Lowess adjusted reference

Data table
ID_REF RATIO REFERENCE SIGNAL FLAGS VALUE
GM00001P001A01 0 0 0 0 0
GM00002P001A02 0 0 0 0 0
GM00003P001A03 0 0 0 0 0
GM00004P001A04 0 0 0 0 0
GM00005P001A05 4.135 715.1 "2,957" P 2.047887329
GM00006P001A06 0.383 "3,066" "1,174" P -1.384583703
GM00007P001A07 0 0 0 0 0
GM00008P001A08 0 0 0 0 0
GM00009P001A09 0 0 0 0 0
GM00010P001A10 0.0203 "10,317" 209 P -5.622376462
GM00011P001A11 1.897 94 179 A 0.923719679
GM00012P001A12 0 0 0 0 0
GM00013P001A13 0 0 0 0 0
GM00014P001A14 0 0 0 0 0
GM00015P001A15 0 0 0 0 0
GM00016P001A16 0 0 0 0 0
GM00017P001A17 0 0 0 0 0
GM00018P001A18 0.934 544 508 P -0.098505545
GM00019P001A19 0 0 0 0 0
GM00020P001A20 0 0 0 0 0

Total number of rows: 19200

Table truncated, full table size 710 Kbytes.




Supplementary file Size Download File type/resource
GSM149957.gpr.gz 1.6 Mb (ftp)(http) GPR

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