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Sample GSM599754 Query DataSets for GSM599754
Status Public on Sep 01, 2013
Title carb_par_96_48_2
Sample type RNA
 
Channel 1
Source name carbaryl exposed, 96h, r2
Organism Daphnia magna
Characteristics clone: P 32,85
gender: female
treatment: carbaryl exposure
time point: 96h
replicate: 2
Treatment protocol Eighty juveniles per treatment were kept together in 500ml jars at a density of 1 animal/2.5ml medium and exposed to four conditions (two biological replicates per treatment): a control treatment without stress, fish kairomones (Leuciscus idus), carbaryl (5.6µg/l; measured concentration 5.74µg/l) or spores of the parasite Pasteuria ramosa (5x10^6 spores/ml).
Exposures were done every second day starting at day 0. Medium was completely renewed at the moment of a new stress pulse. The two biological samples were collected after 48h, 96h and 144h of exposure. The last pulse was given three hours before freezing the animals for gene expression analysis, respectively, on 45h-, 93h- and 141h-old Daphnia.
Growth protocol P 32,85 clone cultured in standard conditions to avoid maternal effects (see Jansen et al.).
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using Trizol following the manufacturer's protocol.
Label Cy5
Label protocol cDNA collection and sample labelling were done according to Soetaert et al. (2007) and Vandenbrouck et al. (2009). Briefly, total RNA (5µg) together with 2µl mRNA spike from the Lucidea Universal Scorecard (Amersham Biosciences) or from the Spotreport Alien cDNA Array Validation System (Agilent Technologies' Stratagene products) was converted into cDNA using random primers (Invitrogen), a dNTP labelling mix containing aminoallyl-dUTPs and 400U Superscript II reverse transcriptase (Invitrogen). Cy5 and Cy3 (Amersham Biosciences) were covalently coupled to the aminoallyl cDNA samples. After a cleanup reaction (QIAquick PCR purification kit, Qiagen, USA) removing all non-incorporated dyes, the quality of the labelled cDNA was checked spectrophotometrically using the Nanodrop. A total amount of 50 pmol labelled cDNA with a frequency of incorporation between 20 and 50 was vacuum dried to use as probe.
 
Channel 2
Source name parasite exposed, 48h, r2
Organism Daphnia magna
Characteristics clone: P 32,85
gender: female
treatment: parasite exposure
time point: 48h
replicate: 2
Treatment protocol Eighty juveniles per treatment were kept together in 500ml jars at a density of 1 animal/2.5ml medium and exposed to four conditions (two biological replicates per treatment): a control treatment without stress, fish kairomones (Leuciscus idus), carbaryl (5.6µg/l; measured concentration 5.74µg/l) or spores of the parasite Pasteuria ramosa (5x10^6 spores/ml).
Exposures were done every second day starting at day 0. Medium was completely renewed at the moment of a new stress pulse. The two biological samples were collected after 48h, 96h and 144h of exposure. The last pulse was given three hours before freezing the animals for gene expression analysis, respectively, on 45h-, 93h- and 141h-old Daphnia.
Growth protocol P 32,85 clone cultured in standard conditions to avoid maternal effects (see Jansen et al.).
Extracted molecule total RNA
Extraction protocol Total RNA was extracted using Trizol following the manufacturer's protocol.
Label Cy3
Label protocol cDNA collection and sample labelling were done according to Soetaert et al. (2007) and Vandenbrouck et al. (2009). Briefly, total RNA (5µg) together with 2µl mRNA spike from the Lucidea Universal Scorecard (Amersham Biosciences) or from the Spotreport Alien cDNA Array Validation System (Agilent Technologies' Stratagene products) was converted into cDNA using random primers (Invitrogen), a dNTP labelling mix containing aminoallyl-dUTPs and 400U Superscript II reverse transcriptase (Invitrogen). Cy5 and Cy3 (Amersham Biosciences) were covalently coupled to the aminoallyl cDNA samples. After a cleanup reaction (QIAquick PCR purification kit, Qiagen, USA) removing all non-incorporated dyes, the quality of the labelled cDNA was checked spectrophotometrically using the Nanodrop. A total amount of 50 pmol labelled cDNA with a frequency of incorporation between 20 and 50 was vacuum dried to use as probe.
 
 
Hybridization protocol Arrays were hybridized overnight at 42°C. See Vandenbrouck et al. 2009 (PMID 19187980) for more details.
Scan protocol Genepix personal 4100 Scanner and Genepix pro 4.1 software (Axon Instruments).
Description 47_020409(2)
This Sample uses the array with Lucidea controls.
Data processing Statistical analysis was performed using the R package limma (Smyth, 2004). Spots for which red or green FG < BG + 2SD (Sclep et al., 2007) on all arrays were deleted before analysis (FG: median foreground intensity, BG: average local background intensity calculated over the full microarray, SD: standard deviation of local background intensities). Median intensity data were background corrected using a normal-exponential convolution model using the function backgroundCorrect with method 'normexp', offset = 50 (Ritchie et al., 2007). Data were loess-normalized using the function normalizeWithinArrays, method = 'loess' (Smyth & Speed, 2003). Linear models were fitted to intensity ratios, after which probes were ranked in order of evidence of differential expression using an empirical Bayes method (Smyth, 2004). Each stressor was contrasted against the controls. These contrasts were fitted to the linear models and cut off at p < 0.05 and log2FC > 0.75 or log2FC < -0.75 (log2 fold change).
 
Submission date Sep 23, 2010
Last update date Sep 01, 2013
Contact name Mieke Jansen
E-mail(s) Mieke.Jansen@bio.kuleuven.be
Organization name KULeuven
Department Biology
Lab Laboratory of Aquatic Biology and Evolutionary Ecology
Street address Ch. Deberiotstraat 32
City Leuven
ZIP/Postal code 3000
Country Belgium
 
Platform ID GPL10966
Series (1)
GSE24322 Stressor mRNA expression profiling of three different stressors in the water flea Daphnia magna

Data table header descriptions
ID_REF
VALUE Average log2 Lowess-normalized ratio FC (Cy5/Cy3)

Data table
ID_REF VALUE
EBT_DM_CarbU_P14A1 0.063361031
EBT_DM_CarbU_P14A10 -0.003842692
EBT_DM_CarbU_P14A11 -0.172700549
EBT_DM_CarbU_P14A12 -0.850622891
EBT_DM_CarbU_P14A2 0.012083651
EBT_DM_CarbU_P14A3 0.008271619
EBT_DM_CarbU_P14A4 0.319731113
EBT_DM_CarbU_P14A5 0.236188065
EBT_DM_CarbU_P14A6 0.062834865
EBT_DM_CarbU_P14A7 0.052669595
EBT_DM_CarbU_P14A8 -0.195293977
EBT_DM_CarbU_P14A9 0.175815908
EBT_DM_CarbU_P14B1 -0.334162526
EBT_DM_CarbU_P14B10 0.115727318
EBT_DM_CarbU_P14B11 0.106614737
EBT_DM_CarbU_P14B12 -0.054595625
EBT_DM_CarbU_P14B2 -0.112242421
EBT_DM_CarbU_P14B3 -0.222101129
EBT_DM_CarbU_P14B4 0.456466567
EBT_DM_CarbU_P14B5 -0.178881217

Total number of rows: 1918

Table truncated, full table size 55 Kbytes.




Supplementary file Size Download File type/resource
GSM599754.gpr.gz 559.6 Kb (ftp)(http) GPR
Processed data included within Sample table
Processed data are available on Series record

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