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Sample GSM572679 Query DataSets for GSM572679
Status Public on Dec 31, 2012
Title Sc-2289-180-43-0308-3j
Sample type RNA
 
Source name Total RNA extracted from a pool of 1 to 2 mm antral follicles, determined as healthy using microscopic examination after Feulgen staining of some granulosa cells, originating from sow52495
Organism Bos taurus
Characteristics annotation pf/mf/gf: PF
group: small follicles
date hybridation-genovul: 2008-03-25
status: S (healthy follicles)
animal-number_genovul: 52495
Extracted molecule total RNA
Extraction protocol Once ovaries collected, all visible antral follicles larger than 1 mm in diameter for sows and 3 mm for cows were isolated carefully using a binocular microscope. After dissection, follicle diameter was measured and each follicle was classified according to size, animal and follicular quality. Follicles were allocated to two size classes: small (noted SF, 1-2 mm for sows and 3-5mm for cows) and large (noted LF, 7-8 mm for sows and 15-20mm for cows). Granulosa cells were recovered from all individual follicles and they were stored at -80°C until RNA extraction. For each follicle, a sample of granulosa cells was smeared on a histological slide, and then Feulgen stained to determine follicular quality by microscopic examination. Only healthy follicles (presence of mitosis and absence of pycnosis in granulosa cells) were kept for this study. RNA was extracted from granulosa cells according to the technique described by Chomczynski and Sacchi with minor modifications using pools of granulosa cells from the same follicle size class and the same animal. The quality of each RNA sample was checked through the Bioanalyser Agilent 2100 (Agilent Technologies, Massy, France) and low-quality RNA preparations were discarded.
Label P33
Label protocol The arrays were hybridized with 33P-labelled complex probes synthesized from 5 µg of each RNA sample, using SuperScript II RNAse H-reverse transcriptase (Invitrogen, Cergy-Pontoise, France)
 
Hybridization protocol Micro-arrays were first hybridized with a 33P-labelled oligonucleotide sequence present in all PCR products to control the quality of the spotting process and to evaluate the amount of DNA in each spot. After stripping, the arrays were hybridized with 33P-labelled complex probes synthesized from 5 µg of each RNA sample, using SuperScript II RNAse H-reverse transcriptase (Invitrogen, Cergy-Pontoise, France). Each complex probe has been hybridized on membrane exposed 1, 3 or 7 days to radioisotopic-sensitive imaging plates (BAS-2025, Fujifilm, Raytest, Courbevoie, France).
Scan protocol The imaging plates were scanned thereafter with a phosphor imaging system at 25µm resolution (BAS-5000, Fujifilm, Raytest, Courbevoie, France). Hybridization images obtained from oligonucleotide and complex probes were quantified using the semi-automated AGScan software.
Description A pig nylon micro-array is hybridized with a complex 33P labelled probe
Data processing Data exploration and analysis were performed using R software. The data coming from complex probes hybridization were analysed on the logarithmic scale. As a first step, negative spot with >7 intensity values were checked on images and replaced by the median of negative spots in case of obvious overshining effect or hybridization stain. Then, luciferase positive controls were removed and the correlations of the data from each membrane were examined intra condition. Hybridizations with a lower than 0.80 correlation coefficient were discarded. Spots with low signal value (below the average of empty spots + 3 standard deviations) were considered as unexpressed and were excluded from the analysis. Finally, the negative control spots were removed and the remaining data were centred for each membrane.
 
Submission date Jul 30, 2010
Last update date Dec 31, 2012
Contact name Gwenola Tosser-Klopp
E-mail(s) gwenola.tosser@toulouse.inra.fr
Phone 33 5 61 28 51 14
Organization name INRA
Lab Genetique Cellulaire
Street address Chemin de Borde-Rouge BP 52627
City Castanet-Tolosan Cedex
ZIP/Postal code 31326
Country France
 
Platform ID GPL3729
Series (2)
GSE23335 SABRE-Bt-Ssc_020410
GSE24221 Genovul-Bt-Ssc_020410
Relations
Reanalyzed by GSM596957

Data table header descriptions
ID_REF
VALUE see data processing protocol
QIM_CONST image signal intensity constant diameter
QFIT_VAR fit signal intensity varariable diameter
FIT_CORR fot correction
QIM_VAR image signal intensity variable diameter
QFIT_CONST fit signal intensity constant diameter
DIAM variable diameter
SPOT_QUAL spot quality
OVER_CORR overshining correction
QM quality measure

Data table
ID_REF VALUE QIM_CONST QFIT_VAR FIT_CORR QIM_VAR QFIT_CONST DIAM SPOT_QUAL OVER_CORR QM
CVU03687 null 313 386 0.00443 385 314 350 1 0 0.83491
scan0030.h.10 -0.132424586 226 287 0.00519 287 225 350 0 0 0.84909
scan0024.i.17 null 120 15 0.00565 14 123 104.196 0 0 0.89979
scan0018.i.20 null 133 172 0.00482 172 133 344.533 0 0 0.87603
scan0012.e.11 -0.201101451 211 254 0.00548 254 212 321.669 0 0 0.84263
scan0006.g.08 -0.618485652 139 179 0.00161 179 138 350 0 0 0.88211
scaj0002.k.04 0.170625517 306 375 0.00384 373 307 350 1 0 0.889
scac0041.n.08 -0.647684806 135 77 0 182 62 350 0 0 0.58976
scac0033.p.05 null 133 47 0 177 37 350 0 0 0.41917
scac0029.i.06 -0.732678019 124 163 0 168 130 350 0 0 0.84491
scac0025.g.14 null 124 75 0 166 60 350 0 0 0.61622
CVU03687_1 null 164 79 0.00615 80 169 195.667 0 0 0.86309
scan0036.n.11 null 190 238 0.00384 237 191 350 0 0 0.88082
scan0030.h.17 -0.42306087 169 229 0 223 181 350 0 0 0.87519
scan0024.i.20 null 128 161 0 178 129 350 0 0 0.83802
scan0018.i.22 null 142 186 0 186 148 350 0 0 0.85317
scan0012.e.18 null 165 105 0 219 86 350 0 0 0.64155
scan0006.g.17 -0.141313533 224 285 0.00164 288 224 350 0 0 0.86857
scaj0002.p.11 0.897510837 633 724 0.00361 719 631 330.338 1 0 0.83882
scac0041.n.11 0.218481538 321 406 0.00801 405 320 350 0 0 0.87797

Total number of rows: 9216

Table truncated, full table size 550 Kbytes.




Supplementary data files not provided
Processed data included within Sample table

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