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Sample GSM1933276 Query DataSets for GSM1933276
Status Public on Apr 18, 2017
Title BufoMarinus-Skin_Bd-infected_rep2
Sample type RNA
 
Source name Skin
Organism Rhinella marina
Characteristics excluded from analyses based on qc: 0
tissue: Skin
genotype: Wild-type
phenotype: normal
subject id: Bm2
pathogen infection intensity (zoospore equivalents) for subject: 0
slide id: 540251
cy3 pmt: 6.8
excluded from analyses based on qc: 0
Growth protocol Prior to the experiment the frogs were housed communally, but for the experiement they were each kept in individual tanks. The frogs were kept in a room maintained at 18 degrees C with 12:12 light:dark photoperiod. The frogs were fed crickets twice per week ad libitum with a water change. For both species (Bufo marinus, Bufo boreas), ten out of twenty frogs were experimentally exposed to the chytrid pathogen Batrachochytrium dendrobatidis for 24 hours. The experiement ended 18 days after inoculation, when all frogs were sacrificed and tissues were collected and preserved in liquid nitrogen. Gene expression was analysed in sample size of 6 replicates per species and tissue type.
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using a routine Trizol/Chloroform protocol. RNA quality and concentration was determined by analysis with an Agilent 2100 bioanalyzer (minimum RIN score = 8.0).
Label Cy3
Label protocol Cy3 labeling was performed by performed by University of Idaho Genomic Resources Core following the Nimblegen standard operating protocol.
 
Hybridization protocol Hybridization was performed by University of Idaho Genomic Resources Core following the Nimblegen standard operating protocol.
Scan protocol Scanning was performed by University of Idaho Genomic Resources Core following the Nimblegen standard operating protocol. The chips were scanned on an Axon GenePix 4000B Scanner (Molecular Devices, Sunnyvale, CA) using GenePix Pro v6.1 software (Molecular Devices, Sunnyvale, CA). For scanning, the PMT gain was adjusted for optimal saturation.
Description NA
Bm2A
Data processing Each tissue type (skin, liver, and spleen) was analyzed separately. Using the R package oligo, each array was background corrected and normalized using the quantile normalization procedure. Each probeset was summarized using the median polish procedure as described with the robust multichip average (RMA) procedure (Irizarry et al. Biostatistics 4(2):249). The median polish procedure is a robust method for summarizing all probes contained within each probeset to a single expression value for each gene taking into account individual probe effects. Probesets with low levels of expression variation across all samples (IQR < 0.5) were removed from further analysis, reducing the overall number of statistical tests to be performed
 
Submission date Nov 08, 2015
Last update date Apr 18, 2017
Contact name Thomas Poorten
E-mail(s) tom.poorten@gmail.com
Organization name UC Berkeley
Department Environmental Science, Policy, and Management
Street address 54 Mulford Hall
City Berkeley
State/province CA
ZIP/Postal code 94720
Country USA
 
Platform ID GPL21108
Series (1)
GSE74788 Comparative study of host response to chytridiomycosis in susceptible and resistant toad species

Data table header descriptions
ID_REF
VALUE RMA-normalized, averaged gene-level signal intensity; log2 scale.

Data table
ID_REF VALUE
Cluster_10 5.7228
Cluster_100 7.5061
Cluster_1000 4.4914
Cluster_10003 6.1539
Cluster_10004 4.3579
Cluster_10006 7.7184
Cluster_10008 4.6672
Cluster_10009 12.7124
Cluster_1001 5.9798
Cluster_10010 6.6038
Cluster_10011 6.3171
Cluster_10013 3.3498
Cluster_10014 6.7558
Cluster_10015 5.2794
Cluster_10016 4.5267
Cluster_10017 3.7482
Cluster_10018 5.5718
Cluster_10019 6.6008
Cluster_10020 4.4917
Cluster_10022 6.7496

Total number of rows: 31367

Table truncated, full table size 628 Kbytes.




Supplementary file Size Download File type/resource
GSM1933276_540251_No_ID_Slot_2_A01_2012-08-28_532.xys.gz 734.1 Kb (ftp)(http) XYS
Processed data included within Sample table

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