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Sample GSM985731 Query DataSets for GSM985731
Status Public on Feb 20, 2013
Title HepG2-WYE control-72h rep2
Sample type RNA
 
Source name HepG2 cell line
Organism Homo sapiens
Characteristics replicate: 2
cell line: HepG2
treatment: WYE control
Treatment protocol The exposure to the selected chemicals was done for a period of 72h at IC10 concentrations.
Growth protocol Hepatocytes were isolated by using a two-step collagenase perfusion technique . The viability was assessed by trypan blue exclusion and the cells (≥85% viability) were cultured as a monolayer at a density of 0.57x105 cells/cm2 in William’s E medium supplemented with 10%v/v fetal bovine serum, 292mg/ml L-glutamine, 7ng/ml glucagon and antibiotics (7.33IU/ml benzylpenicillin sodium, 50µg/ml kanamycin monosulphate, 50µg/ml streptomycin sulphate, and 10µg/ml ampicillin sodium) in an incubator at 37°C (5% CO2 and 95% air, 100% humidity). After 4 hours, the medium was renewed with serum-free culture medium, supplemented with 25µg/ml hydrocortisone hemisuccinate and 1mg/ml bovine insulin. The hES-Hep cells were derived, cultured and characterized from the human embryonic stem cell (hESC) line SA002 (Cellartis AB, Sweden), as previously described, with an additional step of enzymatic passaging for further expansion before the onset of hepatic differentiation (Heins et al. 2006). The differentiation of SA002 cells into hepatocyte-like cells was achieved by the sequential exposure to growth factors, such as human growth factor and differentiation-promoting factors, including hydrocortisone and insulin (Brolen et al. 2010). The hepatocellular carcinoma-derived HepG2 cell line (Rockville, USA) was cultured and handled as previously described (Tolosa et al. 2011). Human hepatoma HepaRG cells (Biopredic International, France) were cultivated as previously described (Gripon et al. 2002; Guillouzo et al. 2007). At day 13 of cultivation, low DMSO-containing medium was added for a period of 7 days.
Extracted molecule total RNA
Extraction protocol Samples for RNA isolation were collected after 72 hours of exposure. Minimum three independent biological experiments were conducted for each compound. The total RNA extraction (RNA extraction kit, Qiagen), including a DNase digestion step, was done according to the manufacturer’s instructions.
Label biotin
Label protocol We used standard Affymetrix labeling protocols
 
Hybridization protocol We used standard Affymetrix hybridisation rotocols
Scan protocol We used standard Affymetrix scanning parameters
Description Control (WYE1)
Data processing The Affymetrix IDs were alternatively remapped to the alternative IDs from Brainarray (http://brainarray.mbni.med.umich.edu/Brainarray/Database/CustomCDF/CDF_download.asp), thus the ensemb version 61 was used (http://brainarray.mbni.med.umich.edu/Brainarray/Database/CustomCDF/14.1.0/ensg.download/HGU133Plus2_Hs_ENSG_14.1.0.zip). All samples were further normalized by GC-RMA algorithm. In the hES-Heps 2NF, BaP, MAN, MPH, NIF, PIPB, SDF and SPB shared one control whereas AFB, CND, TPA, TOL, WYE and CYCLO shared another control. In the HepaRG system several compounds shared also one control. The groups were divided as follows: 1) 2NF, BaP, MPH, NIF, PIPB and SPB; 2) WYE, AFB, CND, CYCLO, TPA and TOL; 3) MAN and SDF; 4) NNK. In the HepG2 system there were shared control among several compounds also. 2NF, BaP, NIF, PIPB and SPB shared one control, AFB, CND, CYCLO, TPA, TOL and WYE shared another control. The third group was MAN, MPH and SDF which had their own control whereas NNK had its own control. In the HepsC and the HepsT systems there were also several groups of compounds having the same control.The compounds were separated as follows: 1)2NF, NIF and PIPB sharing one control; 2)NNK, MAN, SDF and SPB sharing one control; 3)AFB, CND, CYCLO, TPA, TOL and WYE sharing one control; 4) BaP and MPH sharing one control.
 
Submission date Aug 14, 2012
Last update date Feb 20, 2013
Contact name Tatyana Doktorova
Organization name VUB
Department FAFY
Street address Laarbeeklaan 103, building G
City Brussels
State/province Belgium
ZIP/Postal code 1090
Country Belgium
 
Platform ID GPL13916
Series (1)
GSE40117 Analyses of transcriptomic responses generated by hepatocarcinogens in a battery of liver-based in vitro models
Relations
Reanalysis of GSM985643

Data table header descriptions
ID_REF
VALUE GC-RMA signal

Data table
ID_REF VALUE
ENSG00000000003_at 894.204
ENSG00000000005_at 2.928
ENSG00000000419_at 3391.555
ENSG00000000457_at 15.514
ENSG00000000460_at 28.665
ENSG00000000938_at 4.45
ENSG00000000971_at 3.112
ENSG00000001036_at 648.874
ENSG00000001084_at 140.861
ENSG00000001167_at 31.133
ENSG00000001460_at 6.47
ENSG00000001461_at 13.568
ENSG00000001497_at 27.018
ENSG00000001561_at 21.706
ENSG00000001617_at 17.633
ENSG00000001626_at 3.138
ENSG00000001629_at 225.341
ENSG00000001631_at 16.11
ENSG00000002016_at 8.952
ENSG00000002330_at 5.975

Total number of rows: 18919

Table truncated, full table size 473 Kbytes.




Supplementary file Size Download File type/resource
GSM985731_HUL-H-DMSO-72-R-7-1.CEL.gz 4.7 Mb (ftp)(http) CEL
Processed data included within Sample table

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