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Sample GSM1072144 Query DataSets for GSM1072144
Status Public on Apr 01, 2014
Title Mouse623_Cyclosporin
Sample type RNA
 
Source name Mouse623 Liver cells
Organism Mus musculus
Characteristics strain: C57Bl/6
gender: male
age: six-weeks-old
compound: Cyclosporin
class: NGTXC
mouse number: 623
tissue: liver
Treatment protocol For the chemicals used in this study, appropriate dosages were derived from previously performed dose range finding (DRF) studies (2-AAF, Phe, CsA, DEHP, DES, E2, PBB, Res, WY, D-man (van Kreijl et al. 2001; de Vries et al. 1997)) or if not known yet, identified by performing additional 28-day DRF studies prior to the short-term exposure studies (see supplemental information 1 for DRF studies using AFB1, CPPD, BPA, DIDP, SD and TBTO). In short, eight to ten weeks old male C57BL/6J mice (n = 10 per group) were exposed to chemicals, using multiple dosages based on literature or expert advice. Body weight dynamics during the first week and over the full 28-day exposure were monitored to extract suitable (non- or slightly cytotoxic) doses (Supplemental information 1). If body weight dynamics were not conclusive, the liver was studied macroscopically (data not shown). Exposure through feed was continuously during the experiment, application using i.p. injection occurred at day 0, 3 and 6 (autopsy on day 7) and exposure using gavage at day 0, 2, 4 and 6 (autopsy on day 7). Body weights were recorded during this 7-day exposure period (Supplemental information 2). Comparison of different control groups (gavage, i.p. injection or feed) showed no significant differential effect on transcriptional levels (Luijten et al. in preparation), hence only food administrated control samples were implemented in this study
Growth protocol Six-week-old male WT mice (C57BL/6J, n=4 per group) were acclimated for 2 weeks and subsequently treated for 7 days with a GTXC, NGTXC or NC through feed, gavage or i.p. injection. From the day of weaning, the health status of the mice was monitored daily and mice were weighed weekly starting at acclimation. Animals were kept in the same stringently controlled (specific pathogen-free, spf) environment, fed ad libitum and kept under a normal day/night rhythm. After 7 days of exposure, mice were sacrificed at a fixed time of the day. During autopsy, several organs (including the liver), were isolated and stored according to protocol using RNAlater (Qiagen, Valencia, CA, USA).
Extracted molecule total RNA
Extraction protocol Hepatic total RNA was isolated using the miRNeasy kit (Qiagen, Valencia, CA, USA) and the QIAcube (Qiagen, Valencia, CA, USA) according to the manufacturer’s instructions. All samples passed RNA quality control using capillary gel electrophoresis (RIN > 7.6) (Bioanalyzer 2100; Agilent Technologies, Amstelveen, the Netherlands). The same total RNA isolates as used for mRNA were used for isolation of microRNAs. MicroRNA profiling was performed as previously described (Pothof et al. 2009).
Label Cy3
Label protocol Total RNA was labeled using the Createch Cy3 label kit (Createch), 1ug of total RNA was used.
 
Hybridization protocol Labeled materials were hybridized to Custom Exiqon LNA probes for 16 hours at 60°C, subsequently washed and scanned
Scan protocol Samples were finally scanned using the ScanArray Express HT (Tecan). Image generation and feature extraction were performed using Imagene 6.0.
Data processing The raw microRNA data, median signal minus median background, were normalized using quantile normalization. For the CsA, WY and CDDP exposed groups quality control discarded one outlier per group. Duplicate spots on the array were averaged and the normalized values were analyzed for differentially expressed microRNAs using a linear model (bioconductor package Limma; Smyth 2005) and corrected for multiple testing (Benjamini and Hochberg 1995) was applied.
Only the spots corresponding to mouse microRNAs were used.
Note: the annotation is updated for a couple of spots after signal extraction by Imagene. Therefore the annotation in the EL**.txt raw files are not completely correct. The new annotation is available in a separate text file (see 'annotation.txt' linked as supplementary file on Series record).
 
Submission date Jan 29, 2013
Last update date Apr 01, 2014
Contact name Kasper Derks
E-mail(s) kasper.derks@mumc.nl
Organization name Maastricht University Medical Center
Department Clinical Genetics
Street address P. Debyelaan 25
City Maastricht
State/province Limburg
ZIP/Postal code 6229 HX
Country Netherlands
 
Platform ID GPL16560
Series (1)
GSE43847 MicroRNA and mRNA biomarkers for short-term in vivo genotoxic and non-genotoxic carcinogen classification

Data table header descriptions
ID_REF
VALUE quantile-normalisation-signal intensity (log2 scale)

Data table
ID_REF VALUE
EQ_42463 9.706137167
EQ_09938 5.525132132
EQ_42573 10.27225648
EQ_17280 7.281024303
EQ_11027 6.44536831
EQ_42823 2.247008907
EQ_17810 8.584089546
EQ_11048 7.863429138
EQ_19595 2.318375983
EQ_17565 6.01960598
EQ_42708 3.321342815
EQ_11184 2.737712499
EQ_17935 3.920699627
EQ_42898 3.508168872
EQ_10928 8.074558469
EQ_30787 6.381663547
EQ_33596 5.066537597
NotDefined_mmu-miR-126-3p 6.672358278
EQ_42692 5.307630798
EQ_33902 3.065933723

Total number of rows: 557

Table truncated, full table size 11 Kbytes.




Supplementary file Size Download File type/resource
GSM1072144_ELAB95.txt.gz 262.2 Kb (ftp)(http) TXT
Processed data included within Sample table

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