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Sample GSM384921 Query DataSets for GSM384921
Status Public on Jul 31, 2009
Title D.rerio_embryo_CR_vs_PBS_embryo_2hpiA
Sample type RNA
 
Channel 1
Source name D.rerio_embryo_CR
Organism Danio rerio
Characteristics reference: Common reference (CR) consisting of a mixture of samples from embryo infections
Biomaterial provider Astrid van der Sar, VUMC
Treatment protocol For the duration of bacterial injections embryos were kept under anaesthesia in egg water containing 0.02% buffered 3-aminobenzoic acid ethyl ester (tricaine, Sigma). Embryos were staged at 28 hours post fertilization (hpf) by morphological critera (Kimmel et al.) and approximately 50 cfu of E11 bacteria were injected into the caudal vein close to the urogenital opening. As a control an equal volume of PBS was likewise injected. Infection experiments were carried out in triplicate on separate days and pools of 15-20 embryos were taken at 2, 24 and 120 hours post infection (hpi).
Growth protocol Embryos were grown at 28,5 -30 °C in egg water (60µg/ml Instant Ocean see salts).
Extracted molecule total RNA
Extraction protocol Embryos were directly homogenized in TRIZOL® Reagent. The RNA samples were incubated for 20 min at 37° with 10 units of DNaseI (Roche Applied Science) to remove residual genomic DNA prior to purification using the RNeasy MinElute Cleanup kit (Qiagen) according to the RNA clean up protocol. The integrity of the RNA was confirmed by Lab-on-chip analysis using the 2100 Bioanalyzer (Agilent Technologies). Samples used for microarray analysis had an average RIN value of 9 and a minimum RIN value of 8.
Label Cy3
Label protocol Amino Allyl modified aRNA was synthesized in one amplification round from 1 μg of total RNA using the Amino Allyl MessageAmp™ II aRNA Amplification Kit (Ambion). Subsequently, 6 ug of Amino Allyl modified aRNA was used for coupling of monoreactive Cy3 dye(GE Healthcare) and column purified.
 
Channel 2
Source name D.rerio_embryo_PBS_2hpi
Organism Danio rerio
Characteristics tissue: 15-20 embryos
time: 2 hours post injection
agent: PBS
Biomaterial provider Astrid van der Sar, VUMC
Treatment protocol For the duration of bacterial injections embryos were kept under anaesthesia in egg water containing 0.02% buffered 3-aminobenzoic acid ethyl ester (tricaine, Sigma). Embryos were staged at 28 hours post fertilization (hpf) by morphological critera (Kimmel et al.) and approximately 50 cfu of E11 bacteria were injected into the caudal vein close to the urogenital opening. As a control an equal volume of PBS was likewise injected. Infection experiments were carried out in triplicate on separate days and pools of 15-20 embryos were taken at 2, 24 and 120 hours post infection (hpi).
Growth protocol Embryos were grown at 28,5 -30 °C in egg water (60µg/ml Instant Ocean see salts).
Extracted molecule total RNA
Extraction protocol Embryos were directly homogenized in TRIZOL® Reagent. The RNA samples were incubated for 20 min at 37° with 10 units of DNaseI (Roche Applied Science) to remove residual genomic DNA prior to purification using the RNeasy MinElute Cleanup kit (Qiagen) according to the RNA clean up protocol. The integrity of the RNA was confirmed by Lab-on-chip analysis using the 2100 Bioanalyzer (Agilent Technologies). Samples used for microarray analysis had an average RIN value of 9 and a minimum RIN value of 8.
Label Cy5
Label protocol Amino Allyl modified aRNA was synthesized in one amplification round from 1 μg of total RNA using the Amino Allyl MessageAmp™ II aRNA Amplification Kit (Ambion). Subsequently, 6 ug of Amino Allyl modified aRNA was used for coupling of monoreactive Cy5 dye(GE Healthcare) and column purified.
 
 
Hybridization protocol The dual colour hybridization of the microarray chips was performed at ServiceXS (ServiceXS, Leiden, The Netherlands) according to Agilent protocol G4140-90050 v.5.7 (www.Agilent.com) for Two-Color Microarray-Based Gene Expression Analysis.
Scan protocol Microarray data were processed from raw data image files with Feature Extraction Software 9.5.3 (Agilent Technologies).
Description CR_vs_PBS_embryo_2hpiA
Data processing Processed data were subsequently imported into Rosetta Resolver 7.1 (Rosetta Biosoftware, Seattle, Washington) and subjected to default ratio error modelling. Data were analyzed at the level of UniGene clusters (UniGene build #105). The significance cut-off for ratios of infected versus control was set at P ≤ 10-4.
 
Submission date Mar 20, 2009
Last update date Jun 02, 2009
Contact name Anna Magdalena Zakrzewska
E-mail(s) ania.zakrzewska@gmail.com
Phone 020-6923990
Fax -
URL http://-
Organization name University of Leiden
Department IBL
Lab A. Meijer
Street address Wassenaarseweg 64
City Leiden
ZIP/Postal code 2333 AL
Country Netherlands
 
Platform ID GPL7735
Series (1)
GSE15328 Specificity of the zebrafish host transcriptome response to acute and chronic mycobacterial infection

Data table header descriptions
ID_REF
VALUE log2 ratio (test/reference)
P-value value of significance assigned after normalization via Rosetta Resolver analysis pipeline
PRE_VALUE fold-change (test/reference)

Data table
ID_REF VALUE P-value PRE_VALUE
A_15_P100001 -0.2774 0.17721 -1.21203
A_15_P100002 0.0719 0.72474 1.05112
A_15_P100003 -0.1338 0.82007 -1.09717
A_15_P100004 0.0912 0.90162 1.06522
A_15_P100005 -0.1732 0.39735 -1.12757
A_15_P100006 1.0683 0.00000234 2.09694
A_15_P100007 0.0234 0.90868 1.01636
A_15_P100008 0.1001 0.62468 1.07187
A_15_P100009 -0.0413 0.83958 -1.02905
A_15_P100010 -1.2535 8.79E-08 -2.38427
A_15_P100011 -0.2986 0.14695 -1.22992
A_15_P100012 0.2044 0.31848 1.15222
A_15_P100013 0.4766 0.02255 1.39144
A_15_P100014 0.3732 0.08769 1.29518
A_15_P100015 -0.4120 0.04708 -1.33053
A_15_P100016 -0.6730 0.00175 -1.59439
A_15_P100017 -0.3458 0.20365 -1.27085
A_15_P100018 0.1073 0.60938 1.07719
A_15_P100019 0.0000 1 1
A_15_P100020 -0.4931 0.13461 -1.40749

Total number of rows: 43370

Table truncated, full table size 1478 Kbytes.




Supplementary file Size Download File type/resource
GSM384921.txt.gz 12.2 Mb (ftp)(http) TXT
Processed data included within Sample table

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