The long-range goal of this project is to define the molecular mechanisms that regulate the expression of the enzymes required for the synthesis of progesterone and estradiol-17beta (E20 in the human and sheep placenta and fetal adrenal. These steroidal secretions are important in effecting the maintenance of uterine quiescence; but the rates of secretion or bioaction must be altered to initiate the preparatory and active phases of labor. The molecular basis of regulation of 3beta-hydroxysteroid dehydrogenase/delta 5->4-isomerase (3beta-HSD) type I in human trophoblast will be determined: (i) The levels of 3beta-HSD MRNA and protein in cultured trophoblast, choriocarcinoma, chorion laeve, and amnion cells will be evaluated after treatments with agonists of protein kinases A and C, and Ca2+-dependent signal transduction; (ii) with selected placental-derived growth factors [insulin-like growth factors (IGFs) I and II, and transforming growth of factor-betas(TGF-betas)]. The nature of the cis- regulatory and trans-acting elements in the 5'-untranscribed flanking sequence, which account for the high expression of this gene in trophoblast, will be established using transfection assays of chimeric gene constructs and gel-shift assays. The level of 3 beta-HSD expression in human fetal adrenal (HFA) is low compared with that in placenta throughout most of pregnancy; but increased of the adrenal enzyme must occur near the time of parturition. The HFA 3beta-HSD is postulated to be the product of a gene distinct from that which encodes the placental (type I) isoform and regulated separately. The action of ACTH, TGF-betas, parathyroid hormone- related protein (PTH-rP), IGFs, and E2 on the level of MRNA encoding HFA 3beta-HSD and the cellular content and activity of this enzyme will be defined. By immunohistochemistry and in situ hybridization, the cell types that express 3beta-HSD and 17alpha-hydroxylase cytochrome P450 (P45017alpha) in the ovine placentome during dexamethasone-induced parturition will be determined. The in vitro action of potential regulators (e.g., IGF-1/II, TGF-betas, glucocorticosteroids) of 3beta-HSD and P450alpha expression in ovine trophoblast cells will be evaluated. Glucocorticosteroid-induced expression of P45017alpha in ovine placenta near the time of parturition may involve alternative, tissue-specific promoters. Unique, untranslated exonic sequences, obtained from amplification of full-length placental and adrenal CDNAS, will be sought to identify placental- and adrenal-specific P45017alpha transcripts and promoters in the CYP17 gene; by means of """"""""foot-printing"""""""" studies, the role of putative steroid enhancer and TGF-beta-inhibitory sequences in the 5'- flanking sequence will be investigated. We will determine whether the enhanced placental expression of this gene involves a trans-acting factor that interacts with a steroid enhancer-like consensus sequence. We will ascertain if differences in 5'-regulatory elements in the human an sheep CYP17 genes account for differences in placental P45017alpha expression.

Project Start
Project End
Budget Start
Budget End
Support Year
19
Fiscal Year
1996
Total Cost
Indirect Cost
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