Expression of AhR and ARNT mRNA in Cultured Human Endometrial Explants Exposed to TCDD

doi:10.1093/toxsci/62.2.289

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Toxicological Sciences 62, 289-298 (2001)
Copyright © 2001 by the Society of Toxicology

REPRODUCTIVE AND DEVELOPMENTAL TOXICOLOGY

Expression of AhR and ARNT mRNA in Cultured Human Endometrial Explants Exposed to TCDD

Jeff A. Pitt^*^,1, Li Feng, Barbara D. Abbott^,2, Judy Schmid, Ronald E. Batt^¶, Theodore G. Costich^¶, Stephen T. Koury and Diane P. Bofinger

^* Curriculum in Toxicology, University of North Carolina, Chapel Hill, North Carolina 27599; Department of Biotechnical and Clinical Laboratory Science, State University of New York at Buffalo, Buffalo, New York 14214; Developmental Biology Branch, RTD, and Office of the Associate Director for Health/Biostatistics and Research Support Staff, NHEERL, U.S. EPA, Research Triangle Park, North Carolina 27711; and ^¶ Department of Gynecology-Obstetrics, State University of New York at Buffalo, Buffalo, New York 14214

Endometriosis is a debilitating disease found in 10–15%of reproductive-age women and is characterized by the presenceof endometrial tissue outside of the uterus. The present studycharacterizes the expression of AhR and ARNT mRNA in a humanendometrial explant culture model in the absence and presenceof TCDD exposure. In a parallel, companion study using thismodel, TCDD exposure was shown to induce CYP1A1 mRNA, CYP1B1mRNA, EROD (7-ethoxyresorufin-O-deethylase) activity, and CYP1B1protein in human endometrial explants. Explants were preparedfrom specimens obtained at laparoscopy or laparotomy from womenundergoing surgery for tubal ligation, endometriosis, or pelvicpain unrelated to endometriosis. These specimens were a subsetof the specimens used in the parallel study. The explants werecultured in medium containing 10 nM estradiol (E₂) or 1 nM estradiolplus 500 nM progesterone (E₂ + P₄) with or without TCDD (first24 h). After culture, AhR and ARNT mRNA expression were quantifiedby RT-PCR. TCDD treatment significantly increased the expressionof AhR mRNA, but not ARNT mRNA. The expression of both geneswas similar for all individual explants and the ratio of AhR:ARNTmRNA expression across all samples was 1.7 to 1.8. ConstitutiveAhR mRNA expression was donor age dependent (increasing withage), while ARNT mRNA expression was donor age and tissue phasedependent (increased in older and proliferative phase specimens).Similar to results in the parallel study on expression of CYP1A1mRNA, CYP1B1 mRNA, EROD activity, and CYP1B1 protein, the presenceof endometriosis did not affect the expression of AhR or ARNTmRNA, either constitutively or following TCDD exposure. However,the detection of disease-specific change was limited by smallsample size and variability in tissue cycle phase. The humanendometrial explant culture model will be useful for futurestudies of the effects of dioxin-like compounds on human endometriumin relationship to cycle phase, hormonal exposure, and donorage.

Key Words: endometrium; endometriosis; TCDD; AhR; ARNT.

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