Arly estrogen) responsiveness [1,20,34]. Since some of these commercial and consumer product extracts contain substantial AhR agonist activity, it is possible that they can also contain chemicals that can produce endocrine disrupting effects in exposed animals. Since these extracts are likely complex mixtures of chemicals, and numerous structurally diverse xenobiotics have been shown to bind to and activate steroid hormone receptor signaling pathways [35?8], it is likely that these extracts also contain steroid hormone receptor agonists. In fact, DMSO and ETOH extracts of the rubber products produce a substantial estrogenic induction response in a recombinant human ovarian carcinoma (BG1) cell line (BG1Luc4E2) containing a stably transfected estrogen receptor responsive luciferase Oltipraz reporter gene [38], demonstrating that they contain estrogen receptor agonists (Figure 5). While endocrine disrupting chemicals (EDCs) have been identified in extracts of environmental and food matrices, personal care products, sunscreens and a limited number of commercial and consumer products [39?2], most studies have focused on identification of known EDCs, rather than assessing the overall EDC activity of a sample extract and then identifying the responsible chemicals. Using hormone receptor based screening approaches, like that described here for the AhR, extracts of a very limited number of paper, rubber and plastic materials have been previously shown to contain estrogenic, antiestrogenic, androgenic, and/or antiprogesteronic activity [43?5]. Thus, in Homatropine (methylbromide) custom synthesis addition to AhR agonists, commercial and consumer products also contain extractable estrogenic EDCs. The effect of these extracts on other nuclear receptor signaling pathways remains to be determined. While the identities of the AhR- and ER-active chemicals described here and their toxicological impacts remain to beCommercial/Consumer Products Contain AhR AgonistsFigure 3. Induction of AhR-dependent luciferase reporter gene activity in stably transfected mouse, rat and human hepatoma cells by extracts of commercial and consumer products. Recombinant mouse (H1L1.1c2), rat (H4L1.1c4) and human (HG21.1c3) 23727046 hepatoma cell lines were incubated with the indicated extract (10 ml/ml) for 4 hr and luciferase activity determined as described in Material and methods. Values are expressed as a percentage of the maximal luciferase induction by TCDD and represent the mean 6 SD of triplicate determinations. The results shown are representative of duplicate experiments and those values significantly greater than that of solvent alone (p#0.05 as determined by the students T-test) are indicated by an asterisk. doi:10.1371/journal.pone.0056860.gCommercial/Consumer Products Contain AhR AgonistsFigure 4. Effect of extracts of newspaper and rubber on human skin CYP1A1 mRNA, embryonic zebrafish CYP1A-dependent EROD activity and zebrafish development. (A) Human skin was incubated with the indicated extract (newsprint (NP) or rubber stopper (RUB) at 1 final concentration) overnight at 37uC, mRNA was isolated and transcribed into cDNA and quantitated by real time PCR. Values are expressed as the mean 6 SD of 4 (TCDD) or 6 (extract) individual skin samples. All values were significantly different from those of DMSO controls (set to 1) at p,0.05 as determined by one-way ANOVA using Stata/SE9.2 software for Windows with Bonferroni corrections. (B) Newly fertilized zebrafish embryos were exposed for 96 h to DMSO (0.02 v/v), newspaper (.Arly estrogen) responsiveness [1,20,34]. Since some of these commercial and consumer product extracts contain substantial AhR agonist activity, it is possible that they can also contain chemicals that can produce endocrine disrupting effects in exposed animals. Since these extracts are likely complex mixtures of chemicals, and numerous structurally diverse xenobiotics have been shown to bind to and activate steroid hormone receptor signaling pathways [35?8], it is likely that these extracts also contain steroid hormone receptor agonists. In fact, DMSO and ETOH extracts of the rubber products produce a substantial estrogenic induction response in a recombinant human ovarian carcinoma (BG1) cell line (BG1Luc4E2) containing a stably transfected estrogen receptor responsive luciferase reporter gene [38], demonstrating that they contain estrogen receptor agonists (Figure 5). While endocrine disrupting chemicals (EDCs) have been identified in extracts of environmental and food matrices, personal care products, sunscreens and a limited number of commercial and consumer products [39?2], most studies have focused on identification of known EDCs, rather than assessing the overall EDC activity of a sample extract and then identifying the responsible chemicals. Using hormone receptor based screening approaches, like that described here for the AhR, extracts of a very limited number of paper, rubber and plastic materials have been previously shown to contain estrogenic, antiestrogenic, androgenic, and/or antiprogesteronic activity [43?5]. Thus, in addition to AhR agonists, commercial and consumer products also contain extractable estrogenic EDCs. The effect of these extracts on other nuclear receptor signaling pathways remains to be determined. While the identities of the AhR- and ER-active chemicals described here and their toxicological impacts remain to beCommercial/Consumer Products Contain AhR AgonistsFigure 3. Induction of AhR-dependent luciferase reporter gene activity in stably transfected mouse, rat and human hepatoma cells by extracts of commercial and consumer products. Recombinant mouse (H1L1.1c2), rat (H4L1.1c4) and human (HG21.1c3) 23727046 hepatoma cell lines were incubated with the indicated extract (10 ml/ml) for 4 hr and luciferase activity determined as described in Material and methods. Values are expressed as a percentage of the maximal luciferase induction by TCDD and represent the mean 6 SD of triplicate determinations. The results shown are representative of duplicate experiments and those values significantly greater than that of solvent alone (p#0.05 as determined by the students T-test) are indicated by an asterisk. doi:10.1371/journal.pone.0056860.gCommercial/Consumer Products Contain AhR AgonistsFigure 4. Effect of extracts of newspaper and rubber on human skin CYP1A1 mRNA, embryonic zebrafish CYP1A-dependent EROD activity and zebrafish development. (A) Human skin was incubated with the indicated extract (newsprint (NP) or rubber stopper (RUB) at 1 final concentration) overnight at 37uC, mRNA was isolated and transcribed into cDNA and quantitated by real time PCR. Values are expressed as the mean 6 SD of 4 (TCDD) or 6 (extract) individual skin samples. All values were significantly different from those of DMSO controls (set to 1) at p,0.05 as determined by one-way ANOVA using Stata/SE9.2 software for Windows with Bonferroni corrections. (B) Newly fertilized zebrafish embryos were exposed for 96 h to DMSO (0.02 v/v), newspaper (.