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Sample GSM102076 Query DataSets for GSM102076
Status Public on May 04, 2007
Title DFVF1_pig5_lung_healthy
Sample type RNA
 
Channel 1
Source name Lung tissue, healthy
Organism Sus scrofa
Characteristics Animal: 10-12 week old castrate of Danish Landrace/Yorkshire/Duroc from a high health herd (Specific Pathogen Free)
Tissue: lung
State: healthy
Biomaterial provider Danish Institute for Food and Veterinary Research
Extracted molecule total RNA
Extraction protocol RNeasy Maxi Kit with DNase treatment (Qiagen)
Label Alexa 594
Label protocol Superscript Indirect cDNA Labeling System (Invitrogen) and ARES cDNA labeling kit (Molecular Probes/Invitrogen)
 
Channel 2
Source name Common reference
Organism Sus scrofa
Characteristics Mixture of total RNA purified from infected and healthy pig lung tissue
Biomaterial provider Danish Institute for Food and Veterinary Research
Extracted molecule total RNA
Extraction protocol RNeasy Maxi Kit with DNase treatment (Qiagen)
Label Alexa 488
Label protocol Superscript Indirect cDNA Labeling System (Invitrogen) and ARES cDNA labeling kit (Molecular Probes/Invitrogen)
 
 
Hybridization protocol The slides were pre-hybridized (5 x SSC, 0.1 % SDS, 1 mg/mL BSA, 0.22 µm filtrated) at 42 ºC for 45 min and washed (2x5 dips in water) followed by a dip in isopropanol and centrifugation (300 x g). mSeries LifterSlip (25x60 mm, Erie Scientific Company) were cleaned by dipping in water followed by several dips in ethanol and left for drying. A lifterslip was placed on each slide and incubated at 42 ºC to preheat. The hybridization chamber, a 6x17x22 cm lidded plastic box with a stainless steel “table” and a napkin wetted with hybridization buffer, was placed at 42 ºC to preheat. The purified labeled cDNA were combined pair wise and 20 µg Poly-dA (Invitrogen), 25 µg yeast tRNA (Invitrogen) and 20 µg pig CoT-DNA was added. The samples were speedvaced until dry (medium heat, app. 30 min), resuspended in 70 µL hybridization buffer (50 % formamide, 5x SSC, 0.1 % SDS), incubated at 95 ºC for 3 min, snap cooled on ice and centrifuged. The samples were applied to the pre-heated slides and placed in the hybridization chamber which was sealed and incubated at 42ºC for 12 to 16 hours. Following hybridization, each array was immersed in 100 mL wash-1 (2x SSC, 0.1% SDS, 0.22 µm filtrated) at 42ºC until the lifterslip moves freely away from the slide. The arrays were transferred to a mBox (Erie Scientific Company) and immersed in wash-1 (2x SSC, 0.1% SDS, 0.22 µm filtrated) at 42ºC for 5 min., in wash-2 (0.1x SSC, 0.1% SDS, 0.22 µm filtrated) at ambient temperature for 10 min., 4 times in wash-3 (0.1x SSC, 0.22 µm filtrated) at ambient temperature for 1 min., rinsed in wash-4 (0.01x SSC, 0.22 µm filtrated) for 5 to 10 sec., dipped 5 times in water and dried by centrifugation (300 x g).
Scan protocol Scanner: ScanArray Express HT system (Perkin Elmer), 10 µm resolution, 100 % LP and PMT adjusted individually for each channel. Image analysis software: ScanArray Express, ver. 3.0 (Perkin Elmer) using the histogram method with default settings.
Description RNA from lung tissue was extracted from healthy pig lung tissue and from lung tissue infected with Actinobacillus pleuropneumoniae, reverse transcribed and labeled with Alexa 594. A common reference (equal amounts of RNA from all samples) was reverse transcribed and labeled with Alexa 488. Samples and reference were hybridized simultaneously to DIAS_PIG_27K2_v2 slides and fluorescence in the Alexa 594 and Alexa 488 channels was acquired using a microarray scanner.
Data processing Statistical analysis was carried out in the R computing environment (ver 2.3.0, developmental version, for Windows) using the package Linear Models for Microarray Analysis (Limma, ver 2.4.11) which is part of the Bioconductor project. The log2-transformed ratios of Alexa-594 to Alexa-488 (not background corrected) were normalized within-slide using printtip-loess with default parameters as implemented in Limma and can be found in the “Value” column.
 
Submission date Mar 29, 2006
Last update date May 03, 2007
Contact name Jakob Hedegaard
E-mail(s) Jakob.Hedegaard@ki.au.dk
Phone (+45)89991363
Organization name Aarhus University, Faculty of Agricultural Sciences
Department Department of Genetics and Biotechnology
Lab Molecular Genetics and System Biology
Street address PO-box 50
City Tjele
ZIP/Postal code DK-8830
Country Denmark
 
Platform ID GPL3594
Series (1)
GSE4577 Early pig response to experimental infection with Actinobacillus pleuropneomuniae

Data table header descriptions
ID_REF
VALUE Printtiploess-normalized log2 ratios (594/488)
Ch1 Mean Ch1 (Alexa 594) mean feature intensity
Ch2 Mean Ch2 (Alexa 488) mean feature intensity

Data table
ID_REF VALUE Ch1 Mean Ch2 Mean
100108.4 -0.026832 1116 1277
100108.3 -0.074265 1058 1241
100120.4 -0.047363 1023 1147
100120.3 -0.13364 1019 1234
100156.4 -0.022913 1067 1204
100156.3 -0.063052 1013 1146
100168.4 0.090405 1141 1199
100168.3 0.073398 1051 1079
100204.4 0.112362 1106 1122
100204.3 -0.16771 917 1123
100216.4 -0.006427 1002 1091
100216.3 0.057206 1040 1081
100252.4 0.174367 1173 1163
100252.3 -0.181822 1011 1274
100264.4 -0.343078 1079 2424
100264.3 -0.319947 1065 2258
100300.4 0.20524 1137 1074
100300.3 -0.132717 1024 1246
100312.4 -0.501426 1758 3864
100312.3 -0.333347 1946 3727

Total number of rows: 27648

Table truncated, full table size 762 Kbytes.




Supplementary file Size Download File type/resource
GSM102076_12759827.csv.gz 4.3 Mb (ftp)(http) CSV

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