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Sample GSM333405 Query DataSets for GSM333405
Status Public on Oct 16, 2008
Title Daphnia_1/10LC50_TNB_exp3,rep1
Sample type RNA
 
Channel 1
Source name unexposed_24h
Organism Daphnia magna
Characteristics 40_pooled_14d_old_female
Treatment protocol All exposures to the ORCs were conducted on adult female daphnids 14-16 days old and occurred at 23.50 C for 24 hours
Growth protocol Genetically homogeneous Daphnia magna, purchased from Aquatic Research Organisms (Hampton, NH), were cultured in MHRW and maintained at 23.50 C according to standard protocols (Weber, 1993; Lewis et al., 1994). Weber, C. I. (1993) Methods for Measuring the Acute Toxicity of Effluent and Receiving Waters to Freshwater and Marine Organisms. U.S. Environmental Protection Agency: EPA/600/4-90/027F; Lewis, P. A., Klemm, D. J., Lazorchak, J. M., Norberg-King, T. J., Peltier, W. H. & Heber, M. A. (1994) Short-term Methods for Estimating the Chronic Toxicity of Effluents and Receiving Waters to Freshwater Organisms. US Environmental Protection Agency: EPA/600/4-91/002
Extracted molecule total RNA
Extraction protocol Whole daphnids (40 pooled for each exposure) were initally preserved in RNAlater (Ambion). They were later transferred to liquid nitrogen and ground with a morter and pestle. RNA was isolated using Trizol according to standard methods (Invitrogen, Carlsbad, CA).
Label cy3
Label protocol cDNA was synthesized from 5 ug of total RNA using Superscript III Reverse Transcriptase (Invitrogen, Carlsbad, CA) and labeled following the protocols of the Genisphere 3DNA 350 labeling kit (Genisphere, Hatfield, PA). The dyes were switched for each technical replicate so that the control cDNA was labeled with Cy3 in one hybridization and Cy5 in the other.
 
Channel 2
Source name 1/10LC50_TNB_24h
Organism Daphnia magna
Characteristics 40_pooled_14d_old_female
Treatment protocol All exposures to the ORCs were conducted on adult female daphnids 14-16 days old and occurred at 23.50 C for 24 hours
Growth protocol Genetically homogeneous Daphnia magna, purchased from Aquatic Research Organisms (Hampton, NH), were cultured in MHRW and maintained at 23.50 C according to standard protocols (Weber, 1993; Lewis et al., 1994). Weber, C. I. (1993) Methods for Measuring the Acute Toxicity of Effluent and Receiving Waters to Freshwater and Marine Organisms. U.S. Environmental Protection Agency: EPA/600/4-90/027F; Lewis, P. A., Klemm, D. J., Lazorchak, J. M., Norberg-King, T. J., Peltier, W. H. & Heber, M. A. (1994) Short-term Methods for Estimating the Chronic Toxicity of Effluents and Receiving Waters to Freshwater Organisms. US Environmental Protection Agency: EPA/600/4-91/002
Extracted molecule total RNA
Extraction protocol Whole daphnids (40 pooled for each exposure) were initally preserved in RNAlater (Ambion). They were later transferred to liquid nitrogen and ground with a morter and pestle. RNA was isolated using Trizol according to standard methods (Invitrogen, Carlsbad, CA).
Label cy5
Label protocol cDNA was synthesized from 5 ug of total RNA using Superscript III Reverse Transcriptase (Invitrogen, Carlsbad, CA) and labeled following the protocols of the Genisphere 3DNA 350 labeling kit (Genisphere, Hatfield, PA). The dyes were switched for each technical replicate so that the control cDNA was labeled with Cy3 in one hybridization and Cy5 in the other.
 
 
Hybridization protocol The labeled cDNA pools from the unexposed and exposed D. magna werehybridized the the Daphnia magna microarry using reagents and protocols from Genisphere 3DNA 350 labeling and hybridization kit (Genisphere, Hatfield, PA).
Scan protocol Scanning and quantification was performed using an arrayWoRx Biochip Reader (Applied Precision, Issaquah, WA) and GenePix software version 6.0 (Axon Instruments, Union City, CA).
Description 0.454 mg/L TNB
Data processing Technical replicates were normalized to remove possible non-linearity, if any, and checked for homogeneity using boxplots. As an alternative to between-slide normalization we applied an approach based on sequential single-slide data analysis and utilized the α-outlier-generating model and outlier regions approach to identify differentially expressed cDNAs. Details of the method can be found in: Loguinov, A. V., Mian, I. S. & Vulpe, C. D. (2004) Exploratory differential gene expression analysis in microarray experiments with no or limited replication. Genome Biol. 5, R18.
 
Submission date Oct 15, 2008
Last update date Oct 15, 2008
Contact name Helen C Poynton
E-mail(s) helen.poynton@umb.edu
Phone 617-287-7323
Organization name UMass Boston
Department School for the Environment
Lab Poynton Lab
Street address 100 Morrissey Blvd.
City Boston
State/province MA
ZIP/Postal code 02125
Country USA
 
Platform ID GPL5129
Series (1)
GSE13169 Gene expression profiling in Daphnia magna, Part III: Uncovering Biomarkers for Metal and ORC exposures

Data table header descriptions
ID_REF
VALUE normalized log2 ratio (exposed/unexposed)

Data table
ID_REF VALUE
P1CB1 -0.034606859
P1CB3 -0.138408576
P1CB5 -0.425867464
P1CB7 -1.598266237
P1CB9 -0.309024896
P1CB11 -0.524622321
P1CD1 -0.194621934
P1CD3 -0.496322855
P1CD5 0.19263278
P1CD7 0.040226209
P1CD9 0.255353893
P1CD11 -0.747750609
P1CF1 0.22893962
P1CF3 0.344854404
P1CF5 0.165018604
P1CF7 -0.007687131
P1CF9 0.117333879
P1CF11 -0.003351469
P1CH1
P1CH3 0.155260227

Total number of rows: 7680

Table truncated, full table size 131 Kbytes.




Supplementary file Size Download File type/resource
GSM333405.gpr.gz 738.0 Kb (ftp)(http) GPR
Processed data included within Sample table

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