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Sample GSM721255 Query DataSets for GSM721255
Status Public on May 09, 2011
Title canola removed at V8 rep 1 and Canola removed at V4 rep 1 [Alexa 647]
Sample type RNA
 
Source name top 8 cm of the topmost fully expanded leaf of four plants grown in the presence of canola to V8 were harvested and pooled.
Organism Zea mays
Characteristics tissue: top 8 cm of the topmost fully expanded leaf of four plants
stress: grown in the presence of canola to V8
Treatment protocol 8 cm of the top most fully expanded leaf was harvested directly into liquid nitrogen and stored at -80 until RNA extraction.
Growth protocol Corn was planted on May 10, 2008 at South Dakota State Research Farm about 15 miles east of Brookings, SD. The soil parent materials were loess over glacial outwash, and the soil series was Brandt silty clay loam (fine-silty, mixed, superactive, frigid Calcic Hapludolls) (Clay et al. 2009). The water content at planting ranged from 22-24%, and soil pH ranged from 6.0-6.5. Soil N at the beginning of the season was 44.5 (2008) and 41 (2009) kg N ha-1, respectively, from residual nitrate and legume credit. The experimental design was a randomized complete block design with four replications. A commercially available 97-d corn hybrid that had glyphosate-resistance and corn rootworm/corn borer stacked traits was planted on May 10, 2008, and April 28, 2009. The seeding rate was about 79,000 seeds ha-1. Row spacing was 76 cm. Plant matrerial was harvested on July 2, 2008. Weather conditions at harvest were partly cloudy with temperatures in the low to mid 80sF, with an 18 mph wind.
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using Trizol reagent5 and purified using Qiagen RNeasy MinElute cleanup kit6, following the manufacturer’s protocol.
Label Alexa 647
Label protocol First strand cDNA synthesis was performed using 1900 ng total RNA and second strand cDNA synthesis was performed using the resulting first-strand cDNA sample to make double-stranded cDNA using the Aminoallyl Message Amp II kit7. aRNA was synthesized using the resulting double-stranded cDNA. Technical replicates from each treatment were labeled with Alexa Fluor 6478 or Alexa Fluor 5558 dye. An Alexa Fluor 647-labeled sample from one treatment was mixed with an Alexa Fluor 555-labeled sample from another treatment.
 
Hybridization protocol 46,000-element microarray chip developed by the University of Arizona was hybridized using their protocol (International Microarray Workshop Handbook, 2009; Gardiner et al. 2005).
Scan protocol Intensities based on fluorescence for each probe were visualized and quantified with a GenePix scanner9 and GenePix Pro software.
Description 070909 107dB 105dR.txt
Alexa 647: Field experiments were conducted in 2008 at South Dakota State Research Farm about 15 miles east of Brookings, SD. The soil parent materials were loess over glacial outwash, and the soil series was Brandt silty clay loam (fine-silty, mixed, superactive, frigid Calcic Hapludolls (Clay et al. 2009. The water content at planting ranged from 22-24%, and soil pH ranged from 6.0-6.5. Soil N at the beginning of the season was 44.5 kg N ha-1, from residual nitrate and legume credit. Nitrogen application of 236 kg N ha-1 was applied at the beginning of the season. Canola was planted at 7 kg ha-1, drilled 10-cm from the corn row at corn planting. The experimental design was a randomized complete block design with three replications. A commercially available 97-d corn hybrid that had glyphosate-resistance and corn rootworm/corn borer stacked traits was planted on May 10, 2008. The seeding rate was about 79,000 seeds ha-1. Row spacing was 76 cm. Plants were grown to the V8 stage of growth and harvested on July 2, 2008. Weather conditions at harvest were partly cloudy with temperatures in the low to mid 80sF, with an 18 mph wind.
Data processing Data from dual channel hybridization was treated as if it were from single channel hybridizations. Dual channel hybn: canola removed at V8 rep 1 and Canola removed at V4 rep 1

GeneMaths XT software was used to log transform (log 2) the intensity readings and samples from each individual hybridizations were normalize against each other using default parameters in Genemaths XT software (data was treated as if it were from single channel hybridizations). Probes that had hybridization intensity less than 2 times the standard deviation plus the average of the negative controls were deleted (Horvath et al., 2007) and technical replicates for each probe were averaged to reduce any dye bias that existed. GeneMaths XT software was then used to identify P values based on ANOVA and individual t tests between treatments. Probes were considered differentially expressed if P values for any test were ≤0.05.
 
Submission date May 08, 2011
Last update date May 09, 2011
Contact name David Horvath
E-mail(s) david.horvath@ars.usda.gov
Phone 701-239-1255
Organization name US Dept. Agriculture
Department Agr. Research Service
Lab Bioscience Research Lab
Street address 1605 Albrecht Blvd
City Fargo
State/province ND
ZIP/Postal code 58105
Country USA
 
Platform ID GPL6438
Series (1)
GSE29132 Corn under weed, low nitrogen, and shade stress

Data table header descriptions
ID_REF
VALUE log2 normalized intensities of genes that passed quality control

Data table
ID_REF VALUE
10101
10102
10103
10104
10105
10106
10107
10108
10109
10110 -0.302193
10111 -0.586987
10112
10113 0.179404
10114
10115 0.132078
10116
10117
10118 0.535899
10119
10120

Total number of rows: 46128

Table truncated, full table size 447 Kbytes.




Supplementary file Size Download File type/resource
GSM721255_070909_107dB_105dR.txt.gz 6.3 Mb (ftp)(http) TXT
Processed data included within Sample table

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