NCBI Logo
GEO Logo
   NCBI > GEO > Accession DisplayHelp Not logged in | LoginHelp
GEO help: Mouse over screen elements for information.
          Go
Sample GSM296897 Query DataSets for GSM296897
Status Public on Jun 12, 2008
Title Upland Cotton fiber Expression at 17dpa relative to 5dpa
Sample type RNA
 
Channel 1
Source name Developing Cotton fiber at 17 days post anthesis (dpa)
Organism Gossypium hirsutum
Characteristics flowers were tagged on the day of anthesis (0 days post anthesis (dpa)). Developing bolls from the first fruiting positions closest to the stem were collected at 17 dpa between 8 a.m. and 10 a.m. to eliminate diurnal effects. Bolls were collected from different plants, and immediately mingled, frozen in liquid Nitrogen, and then stored in 50-ml polypropylene tubes at -80°C.
Growth protocol G. hirsutum L. cv. TM1, also known as upland, was grown in the green house under a 30/21°C day/night temperature regime in a randomized block design
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using the modified hot borate method (Wan and Wilkins, 1994; Wilkins and Smart, 1996; Arpat et al., 2004)
Label Alexa Fluor® 555 and Alexa Fluor® 647 (Dye Swap included)
Label protocol Fluorescent-tagged amino-allyl labeled cDNA probes were generated by reverse transcription of cotton fiber total RNA (30 μg) spiked with reference mRNA spike mix (10, 50, 200, 400, 1000, and 2000 pg Alien Spike mRNAs 1 through 6, respectively, Stratagene), 5g poly-T21VQ primers (Operon), 0.2 mM each of dATP, dCTP, and dGTP (Sigma), and a 2:3 ratio of 0.2 mM aminoallyl-dUTP/dUTP mix (Sigma) in a total volume of 40 μl incubated at 42°C for 4 hours using SuperScript II (Invitrogen). Aminoallyl-labeled cDNA was purified using the QiaQuick PCR purification kit (Qiagen), and labeled with Cy3 or Cy5 monofunctional dyes (Amersham) according to manufacturer’s instructions. Labeled cDNA were quality controlled by measuring absorbance at 260, 280, 555, and 650. For each probe, the frequency of incorporation (FOI) of dye molecules expressed as the number of dye molecules per 1000 bps and concentration of cDNA were calculated and probes with an FOI < 20 were discarded.
 
Channel 2
Source name Developing Cotton fiber at 5 days post anthesis (dpa)
Organism Gossypium hirsutum
Characteristics flowers were tagged on the day of anthesis (0 days post anthesis (dpa)). Developing bolls from the first fruiting positions closest to the stem were collected at 5 dpa between 8 a.m. and 10 a.m. to eliminate diurnal effects. Bolls were collected from different plants, and immediately mingled, frozen in liquid Nitrogen, and then stored in 50-ml polypropylene tubes at -80°C.
Growth protocol G. hirsutum L. cv. TM1, also known as upland, was grown in the green house under a 30/21°C day/night temperature regime in a randomized block design
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using the modified hot borate method (Wan and Wilkins, 1994; Wilkins and Smart, 1996; Arpat et al., 2004)
Label Alexa Fluor® 555 and Alexa Fluor® 647 (Dye Swap included)
Label protocol Fluorescent-tagged amino-allyl labeled cDNA probes were generated by reverse transcription of cotton fiber total RNA (30 μg) spiked with reference mRNA spike mix (10, 50, 200, 400, 1000, and 2000 pg Alien Spike mRNAs 1 through 6, respectively, Stratagene), 5g poly-T21VQ primers (Operon), 0.2 mM each of dATP, dCTP, and dGTP (Sigma), and a 2:3 ratio of 0.2 mM aminoallyl-dUTP/dUTP mix (Sigma) in a total volume of 40 μl incubated at 42°C for 4 hours using SuperScript II (Invitrogen). Aminoallyl-labeled cDNA was purified using the QiaQuick PCR purification kit (Qiagen), and labeled with Cy3 or Cy5 monofunctional dyes (Amersham) according to manufacturer’s instructions. Labeled cDNA were quality controlled by measuring absorbance at 260, 280, 555, and 650. For each probe, the frequency of incorporation (FOI) of dye molecules expressed as the number of dye molecules per 1000 bps and concentration of cDNA were calculated and probes with an FOI < 20 were discarded.
 
 
Hybridization protocol Printed slides were pre-hybridized in a 50-ml solution of 5X SSC, 0.1% SDS, and 0.1 µg/µl BSA in a sealed coplin jar for 45 min @ 42ºC, followed by two washes of 10 sec each in filtered ddH2O, and dried with filtered compressed air. The final hybridization solution (50 µl) contained amino-labeled cDNA in 30% formamide, 5X SSC, 0.1% SDS, and 0.1 µg/µl sheared salmon sperm DNA and was applied to the slide surface using mSeries LifterSlips (Erie Scientific). After incubating at 42ºC for 16-20 hours in a humidified hybridization chamber (Genetix), the LifterSlips were removed by dipping slides in 2X SSC @ 42 °C. Slides were washed sequentially at 42ºC in 2X SSC, 0.2% SDS for 5 min, 0.5X SSC for 3 minutes, 4 times in 0.1X SSC for 1 minute per wash, and 0.05X SSC for 10 seconds, followed by a dip in ddH2O and drying with filtered compressed air.
Scan protocol Hybridized slides were scanned using the 428 Array Scanner (Affymetrix) followed by feature extraction to quantify signal intensities using ImaGene 4.2 software (BioDiscovery).
Description PDF files of detailed experimental protocols for RNA isolation (SOP MA002 v1.1), amino-allyl labeling (SOP MA003 v2.1) and microarray hybridization (SOP MA004 v2.1) can be accessed at Cotton Functional Genomics Center website.
Data processing Microarray images were obtained using the 428 Array Scanner (Affymetrix) and signal intensities were quantified with ImaGene 4.2 (BioDiscovery). Low quality spots (dust particles, scratches, high background, or irregularly shaped spots) were manually flagged following visual inspection. Signal intensity was corrected based on blanks (N=274), and flagged spots with a background corrected intensity smaller than the average plus three standard deviations (>99.99% confidence interval) using a custom PERL script were excluded from further analysis. On average, 91.3% of all genes were present for analysis. Using the GNU statistical computing language R and LIMMA, linear models were applied to the data (Smyth, 2005). To remove any systematic intensity or space-dependent differences between Cy3 and Cy5 channels, data were normalized using a within-slide space-dependent global intensity (print-tip-lowess) normalization function provided in the R software package. The distribution of up and down regulated genes in data sets from hybridizations between distant developmental stages was not symmetrical as assumed for global normalization. To therefore analyze asymmetric results, reference calibration spots, which were spiked-in at a ratio of 1:1 in both channels, were weighted to 10 before initiating normalization procedures. Normalized data was fit to a linear model using the least squares method with an inter-duplicate correlation of 0.75 for duplicated spots. Results were interpreted using the 5 dpa time point as the common reference. The significance of differential expression between developmental stages was determined using the empirical Bayes method to shrink the gene-wise sample variances towards a common value. Resulting statistics were corrected for multiple-testing using Benjamini and Hochberg false discovery rates (Benjamini and Hochberg, 1995) and significant changes in gene expression were identified at p <0.05. Significance test was performed for each time point after 5 dpa relative to all preceding time points.
 
Submission date Jun 05, 2008
Last update date Jun 05, 2008
Contact name Thea A Wilkins
URL http://genomics.ttu.edu
Organization name Texas Tech University
Department Plant and Soil Sciences
Lab Plant Functional Genomics Lab
Street address 2500 Broadway,Campus Box 42122
City Lubbock
State/province TX
ZIP/Postal code TX 79409
Country USA
 
Platform ID GPL6917
Series (1)
GSE11693 Expression profiling of cotton (Gossypium hirsutum L. TM1) fiber transcriptome during the development

Data table header descriptions
ID_REF
VALUE The expression ratio; Lg2-fold changes between test channel and 5dpa (M-value)
A.Value the Average Log2-expression level for the gene across all arrays and channels in the experiment
T.statistics Moderate t-statistics
P.Value P. value
adj.P.Value P. value adjusted for multiple testing (FDR)
B.statistics The log-odds that the gene is differentially expressed

Data table
ID_REF VALUE A.Value T.statistics P.Value adj.P.Value B.statistics
GA_10dpa_fiberEST_12195|Ed_XGI.screen.Contig2348 1.888083701 12.4973168 11.31409737 4.35E-11 5.21E-07 14.98739418
GA_10dpa_fiberEST_01869|GA__Ed0043C03r 2.542207402 10.31688508 10.06623804 4.47E-10 2.67E-06 12.90398861
GA_10dpa_fiberEST_04411|CON_001_18758 -1.567317626 10.51920402 -9.358914171 1.82E-09 7.25E-06 11.62566927
GA_10dpa_fiberEST_03870 1.749043935 12.02513577 8.42997177 1.27E-08 3.78E-05 9.834088966
GA_10dpa_fiberEST_11492|Ed_XGI.screen.Contig1269 2.745163048 8.136821014 8.221010086 1.99E-08 4.76E-05 9.41310282
GA_10dpa_fiberEST_03934|CON_001_19299 -1.23005854 11.0848199 -8.006276362 4.33E-08 7.41E-05 8.694900674
GA_10dpa_fiberEST_06582|CON_001_19884 -2.24563549 7.93731137 -7.671667838 6.71E-08 7.56E-05 8.274809517
GA_10dpa_fiberEST_08936|CON_001_24931 2.000639272 9.047425261 7.665281097 6.81E-08 7.56E-05 8.261308261
GA_10dpa_fiberEST_03016|Ed_contig_829 -1.720362638 10.12967858 -7.656228399 6.95E-08 7.56E-05 8.242160858
GA_10dpa_fiberEST_11434|Ed_XGI.screen.Contig1245 -1.207198815 11.02939024 -7.630217701 7.37E-08 7.56E-05 8.18707738
GA_10dpa_fiberEST_04153|CON_001_19307 1.473432611 9.506934292 7.617545184 7.59E-08 7.56E-05 8.160203903
GA_10dpa_fiberEST_06183|CON_001_20330 2.133490884 10.89862011 7.651995259 9.32E-08 8.58E-05 7.976946853
GA_10dpa_fiberEST_12207|Ed_XGI.screen.Contig2350 -1.73495261 10.08371019 -7.491366323 1.01E-07 8.63E-05 7.891324189
GA_10dpa_fiberEST_03470|Ed_contig_1595 -1.98434916 8.815747104 -7.322587192 1.48E-07 0.000105716 7.527987508
GA_10dpa_fiberEST_01227|GA__Ed0015A02f -1.01247593 11.9185938 -7.319745864 1.49E-07 0.000105716 7.521835123
GA_10dpa_fiberEST_11234|Ed_XGI.screen.Contig2915 -0.957653352 12.4875144 -7.310372432 1.53E-07 0.000105716 7.501530291
GA_10dpa_fiberEST_12002|Ed_XGI.screen.Contig1325 -1.192626563 10.6453462 -7.292682677 1.59E-07 0.000105716 7.463175653
GA_10dpa_fiberEST_05299|CON_001_20158 -1.110623815 10.92815053 -7.137045144 2.28E-07 0.000143503 7.123770236
GA_10dpa_fiberEST_01896|GA__Ed0044D04f 1.245780377 10.40970162 6.996487127 3.16E-07 0.000189151 6.814266931
GA_10dpa_fiberEST_09226|CON_001_19065 2.596108233 12.7996255 6.804184351 4.97E-07 0.000232597 6.386333352

Total number of rows: 12263

Table truncated, full table size 1342 Kbytes.




Supplementary file Size Download File type/resource
GSM296897_tw002773_filtered_Cy5.txt.gz 1.5 Mb (ftp)(http) TXT
GSM296897_tw002774_filtered_Cy3.txt.gz 1.7 Mb (ftp)(http) TXT
Processed data included within Sample table

| NLM | NIH | GEO Help | Disclaimer | Accessibility |
NCBI Home NCBI Search NCBI SiteMap