Effects of hormones and protein kinase inhibitors on expression of steroidogenic enzyme promoters in electroporated primary rat granulosa cells

Orly, Joseph; Clemens, Jeffrey W.; Singer, Orna; Richards, JoAnne S.

doi:10.1095/biolreprod54.1.208

Cited by 29 publications

(19 citation statements)

References 52 publications

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“…Specifically, we have shown that LH rapidly, but transiently, induces PR mRNA and protein in FSH/Tdifferentiated (preovulatory) granulosa cells in culture (10). Although these differentiated cells provide the most physiological model in which to conduct transfection assays with PR promoter-reporter constructs, they do not transfect easily or efficiently (21). Therefore, to determine the efficacy of using immature granulosa cells as a model for analyzing PR promoterreporter constructs, it was necessary to determine whether the endogenous PR gene could be activated in these cells, if given the appropriate stimulus.…”

Section: Induction Of Pr Mrna In Cultured Granulosa Cellsmentioning

confidence: 99%

Transactivation of the Progesterone Receptor Gene in Granulosa Cells: Evidence that Sp1/Sp3 Binding Sites in the Proximal Promoter Play a Key Role in Luteinizing Hormone Inducibility

Sriraman

Sharma

Richards

2003

Molecular Endocrinology

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LH induction of the progesterone receptor (PR) in granulosa cells is a central event in ovulation. To identify critical regions of the mouse PR promoter that confer LH inducibility in granulosa cells, a mouse PR promoter (-384/+680) genomic fragment was ligated to a luciferase reporter construct and transfected into primary cultures of granulosa cells. Forskolin/phorbol myristate (PMA) induced PR promoter-luciferase reporter activity in granulosa cells greater than 15-fold. A deletion construct comprised only of the distal promoter alone (-348/+64) was inactive. Conversely, deletion constructs eliminating putative distal promoter-regulatory elements that bind Sp1, nuclear factor Y, and GATA-4 as well as the transcription start site (+1) failed to reduce forskolin/PMA activation of reporter activity. Additional 5'-deletions identified a minimal promoter region (+420/+680) sufficient to bestow cAMP responsiveness approximately 8- to 10-fold. Two GC-rich regions Sp1(A)[+440/+461] and Sp1(B) [+473/+490] bound Sp1/Sp3. Site-directed mutagenesis of Sp1(A) and Sp1(B) reduced activity of the proximal (+357/+680) promoter reporter construct approximately 50% and 99%, respectively. When the same Sp1(B) mutation was introduced into the intact promoter (-145/+680), forskolin/PMA induction of promoter activity was reduced by 70-80%. When the distal GC box as well as the proximal Sp1(B) site were both mutated in the context of the intact promoter, inducibility of the transgene was even more severely reduced. The importance of these Sp1/Sp3 binding regions was confirmed in human MCF-7 cells and Drosophila SL2 cells. Collectively, these results indicate that the Sp1/Sp3 binding sites within the mouse PR proximal promoter are essential for transactivation of the gene by agonists in granulosa cells. The molecular mechanisms by which LH activates Sp1/Sp3 at this region within the PR gene remain unknown but do not involve changes in the binding of Sp1/Sp3 to the critical GC boxes. Rather, Sp1/Sp3 appear to recruit other factors to the promoter.

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Section: Induction Of Pr Mrna In Cultured Granulosa Cellsmentioning

confidence: 99%

Transactivation of the Progesterone Receptor Gene in Granulosa Cells: Evidence that Sp1/Sp3 Binding Sites in the Proximal Promoter Play a Key Role in Luteinizing Hormone Inducibility

Sriraman

Sharma

Richards

2003

Molecular Endocrinology

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“…To understand the mechanism of the cAMP-PKA signal on the promoter activity of CYP11A1, the regulatory elements in its promoter have been analyzed in bovine CYP11A [1,23], rat CYP11A [28], mouse Cyp11a [2,21], and human CYP11A1 [3,16,39,40]. These investigations have identified certain cisacting elements conferring cAMP responsiveness via interactions with their specific transcription factors, using standard methods for the analysis of regulatory interacting proteins [29].…”

Section: Cyp11a1 Promoter Activity Regulated By Camp Signalingmentioning

confidence: 99%

Transcriptional Regulation of <i>CYP11A1</i>

Guo¹,

Hu²,

Chung³

2003

J Biomed Sci

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Steroid hormones are important physiological regulators that control our glucose and salt balance, as well as sexual characteristics. The synthesis of steroid hormones is under tight control; disturbed secretion of steroids often leads to diseases. The mechanism controlling the secretion of steroids, namely steroidogenesis, has been the focus of intensive studies. CYP11A1 controls the first and rate-limiting step of steroid biosynthesis. It is expressed in the adrenal cortex and gonads, under the control of pituitary hormones, through the cAMP-signaling pathway. The promoter of the CYP11A1 gene contains sequences that bind to transcription factor SF-1, which plays an important role in the tissue-specific and hormonally regulated expression of steroidogenic genes. Detailed transcriptional analysis documents the importance of SF-1 in activating CYP11A1 in vitro and in vivo. Other factors like c-Jun are also involved. The assembly of various transcription factors forming protein-DNA complexes appears to be the key step in CYP11A1 transcription.

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“…Various reports have directly implicated tyrosine kinase pathways in ovarian steroidogenesis. Addition of specific tyrosine kinase inhibitors to cultured rat granulosa cells results in inhibition of LH-stimulated progesterone production and Cyp11a1 mRNA expression [57][58][59]. Other studies have shown synergistic effects of insulin or IGF1 on gonadotropin-stimulated progesterone production and expression of Cyp11a1 and Hsd3b mRNAs by rat and human granulosa cells [3,4,8].…”

Section: Discussionmentioning

confidence: 96%

Protein Kinase A-Independent cAMP Stimulation of Progesterone in a Luteal Cell Model Is Tyrosine Kinase Dependent but Phosphatidylinositol-3-Kinase and Mitogen-Activated Protein Kinase Independent1

Needle

Piparo

Cole

et al. 2007

Biology of Reproduction

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Comprehensive understanding of the cellular mechanisms utilized by luteal cells in response to extracellular hormonal signals resulting in the normal synthesis and secretion of their steroid and peptide products has yet to be achieved. Previous studies have established that cAMP functions as a second messenger in mediating gonadotropin stimulated luteal progesterone secretion. Classically, increased intracellular concentrations of cAMP result in activation of protein kinase A (PKA), which in turn phosphorylates gene regulatory transcription factors. Recent studies demonstrate that non-PKA mediated actions of cAMP exist, yet the mechanisms are not well understood. In addition to gonadotropic hormones, such growth factors as insulin, insulin-like growth factor 1, and epidermal growth factor have been shown to modulate luteal steroid hormone synthesis and steroidogenic enzyme expression as either independent effects or via amplification or modulation of the action of gonadotropic hormones or cAMP. Thus, mechanisms independent of cAMP and also downstream to cAMP that do not involve PKA are likely to be important in steroidogenesis in mammalian cells. The present studies were performed to help define the cellular mediators involved in cAMP-stimulated progesterone expression. Our data demonstrate that, in an in vitro steroidogenic cell model, 1) cAMP-stimulated progesterone occurs in a manner that is independent of PKA, 2) neither phosphatidylinositol-3-kinase nor mitogen-activated protein kinase are involved in PKA-independent cAMP-stimulated progesterone production, 3) tyrosine kinase activity does mediate cAMP-stimulated progesterone production, and 4) cAMP directly activates the Ras protein. These data suggest novel mediators of cAMP-stimulated progesterone production.

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Effects of hormones and protein kinase inhibitors on expression of steroidogenic enzyme promoters in electroporated primary rat granulosa cells

Cited by 29 publications

References 52 publications

Transactivation of the Progesterone Receptor Gene in Granulosa Cells: Evidence that Sp1/Sp3 Binding Sites in the Proximal Promoter Play a Key Role in Luteinizing Hormone Inducibility

Transactivation of the Progesterone Receptor Gene in Granulosa Cells: Evidence that Sp1/Sp3 Binding Sites in the Proximal Promoter Play a Key Role in Luteinizing Hormone Inducibility

Transcriptional Regulation of <i>CYP11A1</i>

Protein Kinase A-Independent cAMP Stimulation of Progesterone in a Luteal Cell Model Is Tyrosine Kinase Dependent but Phosphatidylinositol-3-Kinase and Mitogen-Activated Protein Kinase Independent1

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