Regulation of steroidogenesis and cholesterol synthesis by prostaglandin F-2  and lipoproteins in bovine luteal cells

Pate, Joy L.; Condon, W. A.

doi:10.1530/jrf.0.0870439

Cited by 32 publications

(23 citation statements)

References 22 publications

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“…PGF2ll had no effect on 25-hydroxycholesterol-stimulated (Pate & Condon, 1989). These results would also support those of Rajkumar et al (1985Rajkumar et al ( , 1988 (Jordan, 1981;Pate & Condon, 1984;Kenny & Robinson, 1986;Benhaim et al, 1987;Alila et al, 1988;Pate & Nephew, 1988).…”

Section: Cellular Uptake Of Lipoprotein-carried Cholesterolsupporting

confidence: 89%

“…PGF2u has been shown to suppress luteinizing hormone (LH)-stimulated, 3',5'-cyclic adenosine monophosphate (cAMP)-stimulated (Jordan, 1981;Pate & Condon, 1984;Benhaim et al, 1987) and lipoprotein-stimulated (Pate & Nephew, 1988;Pate & Condon, 1989) progesterone produc¬ tion. However, PGF-,U has no effect on low-density lipoprotein (LDL) or high-density lipoprotein (HDL) uptake in bovine luteal cells (Pate & Condon, 1989), or on HDL binding (Rajkumar et al, 1985) or LDL binding (Rajkumar et al, 1988) in rat luteal cells, and thus PGF2a may allow uptake of lipoprotein-carried cholesterol into the cell but inhibit the subsequent use of cholesterol for steroidogenesis.…”

Section: Introductionmentioning

confidence: 99%

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Localization of prostaglandin F2 inhibition of lipoprotein use by bovine luteal cells

Grusenmeyer¹,

Pate²

1992

Reproduction

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Summary. Prostaglandin F2\g=a\(PGF2\g=a\) inhibits lipoprotein-stimulated progesterone production by bovine luteal cells in vitro and the objective of this study was to localize the site of action of PGF2\g=a\. Cultured bovine luteal cells were treated with PGF2\g=a\ for seven days, and then with either lipoproteins or 25-hydroxycholesterol in the presence of aminoglutethimide (which inhibits cholesterol side-chain cleavage) for the final 48 h. The effects of PGF2\g=a\ on progesterone production, cellular cholesterol content, mitochondrial cholesterol content and cholesterol side-chain cleavage activity were determined. As expected, PGF2\g=a\ inhibited (P < 0\m=.\05)lipoprotein-stimulated progesterone production. However, PGF2\g=a\ did not inhibit low-density lipoprotein-stimulated, or high density lipoprotein-stimulated, increases in cellular cholesterol (P < 0\m=.\05) or inhibit lipoprotein-induced increases in mitochondrial cholesterol content (P < 0\m=.\05). Additionally, cholesterol content of mitochondria increased (P < 0\m=.\05) in the presence of PGF2\g=a\ alone. To determine if the PGF2\g=a\-induced inhibition of steroidogenesis occurred at, or after, the side-chain cleavage reaction, we treated cells with the readily diffusable sterol, 25-hydroxycholesterol. Prostaglandin F2\g=a\ did not inhibit 25\ x=r eq-\ hydroxycholesterol-stimulated progesterone production (P < 0\m=.\05).Prostaglandin F2\ g=a\ may therefore exert its luteolytic effect at a site after cholesterol transport to the mitochondria but before cholesterol side-chain cleavage.

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Section: Cellular Uptake Of Lipoprotein-carried Cholesterolsupporting

confidence: 89%

Section: Introductionmentioning

confidence: 99%

Localization of prostaglandin F2 inhibition of lipoprotein use by bovine luteal cells

Grusenmeyer¹,

Pate²

1992

Reproduction

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“…These treatment concentrations have been shown to affect bovine luteal cell function in vitro (Pate & Condon 1989, Benyo & Pate 1992, Townson & Pate 1996. After culture, media were removed and luteal cells were harvested to quantify SPP1 mRNA by quantitative PCR (qPCR) or to evaluate SPP1 protein expression via western blot.…”

Section: Cell Culturementioning

confidence: 99%

Expression and regulation of secreted phosphoprotein 1 in the bovine corpus luteum and effects on T lymphocyte chemotaxis

Poole¹,

Ndiaye²,

Pate³

2013

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Secreted phosphoprotein 1 (SPP1) in the bovine corpus luteum (CL) regulates cell function during the transitional periods of luteinization and luteal regression. The objectives were to i) characterize SPP1 expression in the CL throughout the estrous cycle, ii) determine factors that regulate SPP1 expression in luteal cells, and iii) examine the role of SPP1 in lymphocyte chemotaxis, proliferation, and function. SPP1 mRNA was greater in fully functional (d10) CL and late cycle (d18) CL compared with developing (d4) CL. Additionally, SPP1 mRNA increased within 1 h and remained elevated 4 and 8 h following induction of luteolysis with prostaglandin (PG)F 2a . Expression of the SPP1 receptor, b 3 integrin, was not different throughout the estrous cycle but decreased following induction of luteolysis. Expression of CD44 increased during the estrous cycle but did not change during luteal regression. In cultured luteal cells, SPP1 mRNA was upregulated by PGF 2a and/or tumor necrosis factor a. Western blots revealed the presence of both full-length SPP1 and multiple cleavage products in cultured luteal cells and luteal tissue. Depletion of endogenous SPP1 did not hinder luteal cell-induced lymphocyte proliferation or lymphocyte phenotype but did inhibit lymphocyte migration toward luteal cells. Based on these data, it is concluded that SPP1 is initially activated to establish and maintain cellular interactions between steroidogenic and nonsteroidogenic cells during the development of the CL. Upon induction of luteolysis, SPP1 serves as a signaling molecule to recruit or activate immune cells to facilitate luteal regression and tissue degradation.

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“…The uptake of lipoprotein particle remnants and HDL is mediated via the scavenger receptor, class B, type I and LRP receptors (Acton et al 1996, Argov et al 2004. While intact LDL is known to stimulate luteal steroidogenesis (Pate & Condon 1989, Brannian et al 1995, oxidatively modified LDL (oxLDL) prepared in a laboratory setting has been reported to inhibit luteal progesterone production (Carroll et al 1992). Anti-steroidogenic and anti-gonadotrophic activities have been observed also for synthetic alkyl hydroperoxides (Kodaman et al 1994).…”

Section: Introductionmentioning

confidence: 99%

Polar phospholipids from bovine endogenously oxidized low density lipoprotein interfere with follicular thecal function

Löhrke¹,

Viergutz²,

Krüger³

2005

Journal of Molecular Endocrinology

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The role of endogenously oxidized low density lipoprotein (oxLDL) in follicular steroidogenic regulation is unknown. Information may be important in order to elucidate ovulatory dysregulation in disordered lipid metabolism. To obtain specific data, we studied the effect of polar phospholipids (PL) isolated from oxLDL with different endogenous levels of lipohydroperoxides (LHP) on the thecal expression of mRNA encoding steroidogenic enzymes and cyclooxygenase 2 (COX-2), and on the thecal production of superoxide and progesterone. Large (preovulatory) bovine follicles were used and analyses of thecal fragments from single follicles were performed by radioimmunoassays, chemiluminescence assays and quantitative RT-PCR. Basal concentration of mRNA for several lipoprotein receptors exceeded by about 10-times the basal level of mRNA encoding steroidogenic enzymes, suggesting that preovulatory theca receptors may favour uptake of oxLDL. PL (5-11 pmol phosphorus/ml) decreased (up to 0·5-times the control) progesterone synthesis, production of superoxide and levels of P450 cholesterol side chain cleavage (P450 scc), 3 -hydroxysteroid dehydrogenase and COX-2 mRNA. Abundance of COX-2 transcripts in thecal tissue incubated with forskolin depended on the progesterone/17 -oestradiol ratio of the follicle fluid, i.e. the previous microenvironment in vivo. PL effects were mimicked by the platelet-activating factor (PAF). WEB 2086, a PAF receptor blocker, did not always abolish these responses, suggesting that the effects were not mediated solely by this receptor. PAF interfered dose-dependently with LH-induced responses, indicating interference with LH signalling. PL from mildly oxidized LDL (0·5 nmol/ml LHP) tended to exert greater effects than PL from oxLDL containing 1·5 nmol/ml LHP. In consideration of the known physiologic role of progesterone, COX-2 and possibly superoxide, these results provide evidence for a potential of PL from oxLDL to induce ovulatory dysregulation and suggest that the extent of the LDL oxidation seems to be important for interfering with thecal responses to the preovulatory LH surge.

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Regulation of steroidogenesis and cholesterol synthesis by prostaglandin F-2 and lipoproteins in bovine luteal cells

Cited by 32 publications

References 22 publications

Localization of prostaglandin F2 inhibition of lipoprotein use by bovine luteal cells

Localization of prostaglandin F2 inhibition of lipoprotein use by bovine luteal cells

Expression and regulation of secreted phosphoprotein 1 in the bovine corpus luteum and effects on T lymphocyte chemotaxis

Polar phospholipids from bovine endogenously oxidized low density lipoprotein interfere with follicular thecal function

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