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Sample GSM8297705 Query DataSets for GSM8297705
Status Public on Jun 04, 2024
Title SG-19-Rep2
Sample type RNA
 
Channel 1
Source name Seeds at 21 DAF
Organism Brassica napus
Characteristics sample type: tissue
tissue: development seeds
Treatment protocol The developing seeds at 21 days post-anthesis were collected from B. napus lines grown under field conditions at the AAFC Saskatoon Research Farm in 2009. This time point was selected because approximately 20 days after flowering ( DAF) had previously been identified as a critical stage for cell proliferation and oil deposition (O’Hara et al., 2002; Dong et al., 2004).
Growth protocol The B. napus lines used in this study include the two parental lines DH12075, a Canadian spring-type doubled haploid canola line (generated by Dr. Gerhard Rakow and Dr. Ginette Séguin-Swartz, Agriculture and Agri-Food Canada), and PSA12, a resynthesised B. napus line (generated by Dr. Monica Beschorner and Dr. Derek Lydiate, Agriculture and Agri-Food Canada), and 96 doubled haploid segregating (SG) lines generated from the cross of these two parental lines. PSA12 was developed from an interspecific cross between B. oleracea ssp. alboglabra line A12DH and B. rapa line Parkland Sunshine, and DH12075 was derived from a cross between varieties Cresor and Westar (Mayerhofer et al., 2005).
Extracted molecule total RNA
Extraction protocol Total RNA was extracted from the developing seeds using a method modified from that of Oñate-Sánchez and Vicente-Carbajosa (2008) and described in detail by Parkin et al. (2010). Seeds from field grown plants from two trials (2009 and 2010) were harvested for seed quality analysis.
Label Cy5
Label protocol cRNAs were amplified from total RNA samples (2 µg) and labeled with either cy3 or cy5 using the Quick Amp labeling kit, Two Color (Agilent, Catalogue: 5190-0444) according to the manufacturer’s instructions, followed by purification with the Qiagen RNeasy Mini Kit (Qiagen, Catalogue 74104) and quantification with a NanoDrop ND-1000.
 
Channel 2
Source name Seeds at 21 DAF
Organism Brassica napus
Characteristics sample type: tissue
tissue: development seeds
Treatment protocol The developing seeds at 21 days post-anthesis were collected from B. napus lines grown under field conditions at the AAFC Saskatoon Research Farm in 2009. This time point was selected because approximately 20 days after flowering ( DAF) had previously been identified as a critical stage for cell proliferation and oil deposition (O’Hara et al., 2002; Dong et al., 2004).
Growth protocol The B. napus lines used in this study include the two parental lines DH12075, a Canadian spring-type doubled haploid canola line (generated by Dr. Gerhard Rakow and Dr. Ginette Séguin-Swartz, Agriculture and Agri-Food Canada), and PSA12, a resynthesised B. napus line (generated by Dr. Monica Beschorner and Dr. Derek Lydiate, Agriculture and Agri-Food Canada), and 96 doubled haploid segregating (SG) lines generated from the cross of these two parental lines. PSA12 was developed from an interspecific cross between B. oleracea ssp. alboglabra line A12DH and B. rapa line Parkland Sunshine, and DH12075 was derived from a cross between varieties Cresor and Westar (Mayerhofer et al., 2005).
Extracted molecule total RNA
Extraction protocol Total RNA was extracted from the developing seeds using a method modified from that of Oñate-Sánchez and Vicente-Carbajosa (2008) and described in detail by Parkin et al. (2010). Seeds from field grown plants from two trials (2009 and 2010) were harvested for seed quality analysis.
Label Cy3
Label protocol cRNAs were amplified from total RNA samples (2 µg) and labeled with either cy3 or cy5 using the Quick Amp labeling kit, Two Color (Agilent, Catalogue: 5190-0444) according to the manufacturer’s instructions, followed by purification with the Qiagen RNeasy Mini Kit (Qiagen, Catalogue 74104) and quantification with a NanoDrop ND-1000.
 
 
Hybridization protocol Purified cRNAs (2 µg) were fragmented and hybridized to the Agilent 4x44K Brassica arrays (Parkin et al., 2010) for 17 h at 65°C with a rotation of 10 rpm according to the manufacturer’s protocol.
Scan protocol Arrays were washed with the Agilent Gene Expression Washing buffers according to the manufacturer’s protocol and scanned with GenePix 4000B as described by Parkin et al. (2010). Four and two biological replications were performed for the parental lines and the SG lines, respectively, with dye-swaps applied to the biological replicates to minimize dye effects from the two colour systems (Lee et al., 2004).
Description SG-214-cy3 vs SG-19-cy5 (1).gpr
Biological replicate 2
Data processing The raw array datasets were extracted with Gene Pix Pro 6.0, and were firstly normalized by the lowess LOWNESS (Yang et al., 2002) method within arrays, followed by the quantile (Bolstad et al., 2003) method between arrays, using the R/Bioconductor software (available at http://www.r-project.org/). R package Limma (Smyth, 2005).
 
Submission date May 30, 2024
Last update date Jun 04, 2024
Contact name wentao zhang
E-mail(s) wentao.zhang@nrc-cnrc.gc.ca
Organization name NRC-Canada
Street address 110 Gymnasium Pl
City Saskatoom
State/province SK
ZIP/Postal code S7N 0W9
Country Canada
 
Platform ID GPL15739
Series (1)
GSE268725 A systems genomics and genetics approach to identify the genetic regulatory network for lignin content in Brassica napus seeds

Data table header descriptions
ID_REF
VALUE normalized log10 value of each sample

Data table
ID_REF VALUE
GE_BrightCorner 7.053522527
DarkCorner 1.264064315
A_46_P111109 9.328839761
A_46_P334115 9.521793355
A_46_P175019 5.587325446
A_46_P234899 1.332878582
A_46_P284278 2.539904292
A_46_P098344 7.596491356
A_46_P204289 4.80966403
A_46_P187434 9.24043332
A_46_P126774 2.032772025
A_46_P143639 8.707407238
A_46_P069421 1.336838652
A_46_P159564 7.727685763
A_46_P048826 5.865296296
A_46_P005736 7.477013354
A_46_P131694 12.17386523
A_46_P173454 9.268692802
A_46_P231229 1.748837359
A_46_P002021 1.017786406

Total number of rows: 43663

Table truncated, full table size 1061 Kbytes.




Supplementary data files not provided

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