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Sample GSM629396 Query DataSets for GSM629396
Status Public on Apr 22, 2011
Title June 6th Gonad S
Sample type RNA
 
Channel 1
Source name pool of 8 sensitive oyster gonad, sampled the 6th June 2005
Organism Magallana gigas
Characteristics sample: pool of 8 gonad oysters
line: sensitive
field: in situ rearing (South Britanny, France)
gender: males and females
tissue: gonad
Biomaterial provider Laboratoire de Physiologie des Invertebres IFREMER Brest
Treatment protocol in situ rearing before summer mortality (South Britanny, France)
Extracted molecule total RNA
Extraction protocol Total RNA was isolated using Extract-All (Eurobio), RNA quality was assessed by Agilent 6000 nano reagents (Agilent), and RNA concentration was measured using an ND-1000 spectrophotometer (Nanodrop).
Label Cy5
Label protocol 5µg of total RNA directly labeled by reverse transcription using the Direct ShipShot labeling kit (Promega).
 
Channel 2
Source name pool of 10 wild oyster
Organism Magallana gigas
Characteristics sample: pool of 10 oysters
line: no selection (wild oysters)
sampling: the 10th May 2007
field: Brest, France
gender: males and females
tissue: all tissues (whole oyster)
Biomaterial provider Laboratoire de Physiologie des Invertebres IFREMER Brest
Extracted molecule total RNA
Extraction protocol Total RNA was isolated using Extract-All (Eurobio). RNA quality was assessed by Agilent 6000 nano reagents (Agilent). RNA concentration was measured using an ND-1000 spectrophotometer (Nanodrop).
Label Cy3
Label protocol 5µg of total RNA directly labeled by reverse transcription using the Direct ShipShot labeling kit (Promega). All these Cy3 reference samples were pooled and then divided once more into several samples to obtain homogeneous reference.
 
 
Hybridization protocol Equimolar amounts of cDNA samples and cDNA reference, labeled with Cy5 and Cy3 respectively, were SpeedVac evaporated and mixed into a single pool with the hybridization buffer (ChipHyb™ hybridization buffer, Ventana Discovery, Tucson, AZ, USA). They were then co-hybridized on the same microarray slide in a Ventana hybridization station (Ventana Discovery, Tucson, AZ, USA). Hybridizations were performed at the INRA IFR 140 transcriptomic facility (Rennes, France). Following pre-hybridization (with ChipSpread buffer, containing 4×SSC and 0.2% SDS), hybridization was conducted overnight at 42°C in a humidified chamber, according to manufacturer’s instructions. The arrays were washed twice with Ribowash solution (0.1 M Tris, 0.05 M EDTA, and 0.4 M NaCl), twice with 0.1×SSC and finally centrifuged to dry.
Scan protocol After the hybridization step, microarray slides were scanned using a Scanner Genepix 4000B (Axon Instruments Inc.) according to the following parameters: Cy 5 Photo Multiplier Tube (PMT): 550 and Cy 3 PMT: 590.
Data processing This process was repeated for each of the hybridized slides. The images (16-bits TIF images) were then analyzed with Genepix pro 5.1 software (Axon Instruments Inc.) according to manufacturer’s instructions. Spots were filtered for quality according to the following criteria: spot shape, median intensity of the spot, homogeneity of the local background pixels and spot pixel intensities. Spots showing inadequate signals were eliminated, as were those with noisy backgrounds and those with more than 20% saturated pixels in both channels. Transformation and normalization of hybridization data were performed to minimize variation arising from technical differences in RNA quality, probe labeling, and hybridization conditions between experiments. First, a logarithmic transformation was performed for each signal intensity (giving “log values”). The “log values” were median centered. Correction was next performed for differences in the variance across the range of gene expression levels using the formula: (corrected Cy5 log value)i = (Cy5 log value)i – (Cy3 log value)i + (mean Cy3 log value), where Cy5 log value represents sample signal intensity, Cy3 log value represents the reference signal intensity, and mean Cy3 log value represents the mean of all green values obtained for the gene “i” across the different conditions.
 
Submission date Nov 24, 2010
Last update date Apr 23, 2011
Contact name Arnaud Huvet
E-mail(s) ahuvet@ifremer.fr
Phone +33 2 98 22 46 93
Fax +33 (0)2 98 22 46 53
Organization name IFREMER
Department Physiologie Fonctionnelle des Organismes Marins
Lab Laboratoire de Physiologie des Invertébrés
Street address Ifremer centre de Brest BP 70
City Plouzane
ZIP/Postal code 29280
Country France
 
Platform ID GPL8639
Series (1)
GSE25614 Microarray analysis highlights immune response of Pacific oysters as a determinant of resistance to summer mortality

Data table header descriptions
ID_REF
VALUE normalized log ratio data (test/reference)

Data table
ID_REF VALUE
cdn19p0001a01.f.1 -2.25773206436492
cdn19p0001a02.f.1 -2.43008686937034
cdn19p0001a03.f.1 -2.28438059878431
cdn19p0001a07.f.1 -1.55476401463332
cdn19p0001a08.f.1 -0.312670173123128
cdn19p0001a09.f.1 -1.15277881230123
cdn19p0001a10.f.1 -1.24694762872092
cdn19p0001a11.f.1 -2.24452356400333
cdn19p0001a13.f.1 -1.28464109685655
cdn19p0001a14.f.1 -1.56087102590393
cdn19p0001a16.f.1 -1.40531335438656
cdn19p0001a17.f.1 -0.116830165091223
cdn19p0001a18.f.1 -1.06942666409109
cdn19p0001a19.f.1 -1.07091585135584
cdn19p0001a20.f.1 -0.749633718374929
cdn19p0001a21.f.1 -0.806062626464504
cdn19p0001a22.f.1 0.105324139715156
cdn19p0001a23.f.1 -1.1255107947991
cdn19p0001a24.f.1 -0.780103884902467
cdn19p0001b01.f.1 -1.39881128848205

Total number of rows: 9058

Table truncated, full table size 348 Kbytes.




Supplementary file Size Download File type/resource
GSM629396.gpr.gz 1.9 Mb (ftp)(http) GPR
Processed data included within Sample table

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