2004
DOI: 10.1385/ct:4:1:47
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Different global gene expression profiles in benzo[a]pyrene-and dioxin-treated vascular smooth muscle cells of AHR-knockout and wild-type mice

Abstract: Benzo[a]pyrene (B[a]P) and 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD) are potent ligands for the aryl hydrocarbon receptor (AHR). High-density oligonucleotide microarrays were used to generate global gene expression profiles of wild-type and Ahr(-/-) vascular smooth muscle cells (SMCs) from mouse aorta. To determine whether there are signaling pathways other than the AHR involved in B[a]P metabolism, wild-type and AHR knockout (Ahr(-/-) SMCs were exposed to B[a]P. Two signaling pathways, represented by TGF-bet… Show more

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Cited by 50 publications
(31 citation statements)
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“…For each comparison, several hybridizations (four for OPNc versus OPNa and two each for OPNa versus vector and OPNc versus vector) were performed with RNA from distinct soft agar plates and dyeflip of the fluorescent labels. The microarray experiment was carried out as described (Hosack et al, 2003;Karyala et al, 2003;Guo et al, 2004) (see also http://microarray.uc.edu). The human 70-mer oligonucleotide library version 2.0 (21 329 optimized oligos) (Qiagen, Alameda, CA, USA) were printed on aminosilane-coated slides (Cel Associates Inc., Pearland, TX, USA).…”
Section: Soft Agar Growthmentioning
confidence: 99%
“…For each comparison, several hybridizations (four for OPNc versus OPNa and two each for OPNa versus vector and OPNc versus vector) were performed with RNA from distinct soft agar plates and dyeflip of the fluorescent labels. The microarray experiment was carried out as described (Hosack et al, 2003;Karyala et al, 2003;Guo et al, 2004) (see also http://microarray.uc.edu). The human 70-mer oligonucleotide library version 2.0 (21 329 optimized oligos) (Qiagen, Alameda, CA, USA) were printed on aminosilane-coated slides (Cel Associates Inc., Pearland, TX, USA).…”
Section: Soft Agar Growthmentioning
confidence: 99%
“…Data normalization was performed in two steps for each microarray separately [15][16][17]. First, background adjusted intensities were log-transformed and the differences (R) and averages (A) of log-transformed values were calculated as R = log 2 (X1) − log 2 (X2) and A = [log 2 (X1) + log 2 (X2)]/2, where X1 and X2 denote the Cy5 and Cy3 intensities after subtracting local backgrounds, respectively.…”
Section: Data Normalization and Analysismentioning
confidence: 99%
“…The Cy3 and Cy5 fluorescence signal intensities were normalized. Data normalization was done in two steps for each microarray separately (19)(20)(21). First, background-adjusted intensities were log transformed, and the differences (R) and averages (A) of logtransformed values were calculated as R = log 2 (X 1 ) À log 2 (X 2 ) and A = [log 2 (X 1 ) + log 2 (X 2 )] / 2, where X 1 and X 2 denote the Cy5 and Cy3 intensities after subtracting local backgrounds, respectively.…”
Section: V600ementioning
confidence: 99%