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Sample GSM5023785 Query DataSets for GSM5023785
Status Public on Jun 14, 2021
Title MeNQ 1500 mg/L, Rep3
Sample type RNA
 
Source name whole animal
Organism Daphnia pulex
Characteristics age: adult
Treatment protocol MeNQ (CAS Number 4245-76-5) was obtained from a commercial vendor (TCI America, product number M0749). According to manufacturer specifications, this MeNQ was 98% pure and was hydrated (25% of mass as water) for safety purposes. MeNQ was used as received from the vendor for preparation of exposure solutions. Water used for preparation of stock solutions and for the control exposures was tap water (City of Vicksburg, MS, municipal source) dechlorinated using carbon filtration for all toxicity bioassays. For the D. pulex bioassay, standard synthetic freshwater bioassay medium (moderately hard reconstituted water) was used (USEPA 2002). Bioassays were conducted at a target temperature of 25 °C for 11 d as this period was required to acquire 3 broods. Exposures were performed in 50 mL beakers with a test solution volume of 40 mL. One test animal was exposed in each beaker, and 10 replicate beakers were tested per treatment. The daily feeding ration mixture consisting of half Raphidocelis subcapitata and half yeast, cereal leaves, and trout chow fish food. Complete water renewals were conducted three times a week on Mondays, Wednesdays and Fridays. The reproductive output was quantified as the total number of neonates produced in three broods per parental adult that survived to assay completion. D. pulex were exposed to MeNQ at control (0 mg/L), 174, 346, 709, 1385, and 2286 mg/L (measured concentrations) as juveniles through three-broods of reproduction. The reproduction assays included 20 animals exposed individually per treatment. The animals remaining at the termination of the assay were randomly assigned to a set of 4 replicate groups of animals per treatment to serve as treatment replicates in the transcriptomic-expression experimental design (6 treatments x 4 replicates). REFERENCE: U.S. Environmental Protection Agency (2002) Methods for measuring the acute toxicity of effluents and receiving waters to freshwater and marine organisms. EPA-821-R-02-012, 5th ed. Office of Water, Washington, DC.
Growth protocol Daphnia pulex were obtained from in-house cultures (originally purchased from EC Testing) and reared in accordance with guidance in Laird et al. (2015). REFERENCE: Laird JG, Kennedy AJ, Melby NL, Gong P. 2015. Development of a Chronic Toxicity Testing Method for Daphnia pulex, US Army, Engineer Research and Development Center Report. ERDC/EL SR-15-5. pp 1-25.
Extracted molecule total RNA
Extraction protocol The D. pulex samples were flash frozen in liquid nitrogen and stored at -80°C until RNA extractions were conducted. Frozen samples were homogenized using disposable mortar and pellet pestles for each sample (Kimble Kontes, Vineland, NJ). Total RNA isolation and on-column DNase digestion was conducted using the Qiagen RNeasy Mini Kit (Qiagen, Germantown, MD) following manufacturer’s recommendations. RNA quantity was assessed using a NanoDrop One Spectrophotometer (NanoDrop technologies, Wilmington, DE, USA) and final quality was determined using an Agilent 2100 Bioanalyzer (Agilent Technologies, Waldbronn, Germany) where electrophoresis gels were visually inspected for degradation prior to use in downstream applications.
Label Cy3
Label protocol The Agilent Low Input Quick Amp Labeling Kit (one color) protocol was followed using 65 ng of total RNA as starting material from each biological sample.
 
Hybridization protocol An Agilent Technologies (Agilent Technologies, Santa Clara, CA, USA) single color custom 8 x 60K microarray format (Amadid #: 063815) was used for all investigations. A completely randomized design was utilized for microarray hybridizations where each individual D. pulex sample was selected at random (using a random number generator) for hybridization onto individual microarrays. The Agilent Low Input Hybridization Kit (one color) was used for microarray hybridizations following manufacturer’s recommendations. A total of 24 microarrays were hybridized which included four replicates for all MeNQ exposures including the control (0 mg/L), 174, 346, 709, 1385, and 2286 mg/L exposure treatments.
Scan protocol An Agilent Technologies, High-Resolution Microarray Scanner (Model G2505C) was used to scan microarray images at 2 μm resolution. Data were extracted from microarray images using Agilent Feature Extraction software, version 10.7.3.1.
Data processing Microarray data were normalized to the 75th percentile within each array followed by median scaling among all exposures using GeneSpring Software version GX 14.9 (Agilent Technologies). GeneSpring was also utilized for the expression analysis where a one-way ANOVA was conducted (p = 0.01) including Benjamini-Hochberg multiple-tests corrections. Post-hoc tests were also conducted where the SNK test was utilized to determine which transcripts had significant differential expression relative to the 0 mg/L control.
 
Submission date Jan 16, 2021
Last update date Jun 14, 2021
Contact name Kurt A Gust
E-mail(s) kurt.a.gust@usace.army.mil
Phone 601-634-3593
Organization name US Army ERDC
Department Environmental Laboratory
Lab Environmental Genomics and Systems Biology Team
Street address 3909 Halls Ferry Rd.
City Vicksburg
State/province MS
ZIP/Postal code 39180
Country USA
 
Platform ID GPL29611
Series (1)
GSE164957 Mechanistic Evaluation of Reduced Reproduction in Daphnia pulex Exposed to the Insensitive Munition, 1-methyl-3-nitro-1-nitroguanidine (MeNQ)

Data table header descriptions
ID_REF
VALUE Normalized, Log Scale (Log base 2)

Data table
ID_REF VALUE
1253 -0.008036137
1099 -0.06975889
3032 -0.0419693
721 -0.31855917
777 -0.010142803
5221 -0.117238045
210 0.061595917
1537 -0.06772423
3083 -0.008173943
2584 -0.077877045
307 -8.58E-04
9201 -0.48475647
51258 0.18373752
20193 -0.055572987
23651 0.07990646
6970 -0.013848782
49820 -0.15446234
10125 0.117922306
57760 0.17746687
15615 0.27228165

Total number of rows: 61331

Table truncated, full table size 1045 Kbytes.




Supplementary file Size Download File type/resource
GSM5023785_US10293825_256381510008_S01_GE1_107_Sep09_2_2.txt.gz 3.3 Mb (ftp)(http) TXT
Processed data included within Sample table

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