Literature DB >> 10446906

Functional and subcellular changes in the A-kinase-signaling pathway: relation to aromatase and Sgk expression during the transition of granulosa cells to luteal cells.

I J Gonzalez-Robayna1, T N Alliston, P Buse, G L Firestone, J S Richards.   

Abstract

The responsiveness of granulosa cells to FSH (cAMP) changes as these cells switch from the proliferative stage in growing follicles to the terminally differentiated, nonproliferating stage after LH-induced luteinization. To analyze this transition, two well characterized culture systems were used. 1) Granulosa cells isolated from immature rats were cultured in serum-free medium, a system that permits analysis of dynamic, short-term responses to hormones/cAMP. 2) Granulosa cells from preovulatory (PO) follicles that have been exposed in vivo to surge concentrations of hCG (PO/ hCG) were cultured in medium containing 1% FBS, a system that permits analyses of cells that have undergo irreversible, long-term changes associated with luteinization. To analyze the biochemical basis for the switch in cAMP responsiveness, the localization of A-kinase pathway components was related to the expression of two cAMP target genes, aromatase (CYP19) and serum-and glucocorticoid-induced kinase (Sgk). Components of the A-kinase pathway were analyzed by Western blotting and indirect immunofluorescence using specific antibodies to the C subunit, RIIalpha/beta subunits, CREB (cAMP-regulatory element binding protein), phospho-CREB, CBP (CREB binding protein), and Sgk. Cellular levels of C subunit and CREB were similar in all cell types and hormone treatments. CREB and CBP were nuclear; RIIalpha/beta was restricted to a cytoplasmic basket-like structure. Addition of FSH to immature granulosa cells caused rapid nuclear import of C subunit within 1 h. Nuclear C subunit decreased by 6 h after FSH but could be rapidly reimported to the nucleus by the addition of forskolin at 6, 24, or 48 h. Nuclear C subunit was associated with the rapid but transient increases in phospho-CREB. FSH induced Sgk in a biphasic manner in which the protein was nuclear at 1 h and cytoplasmic at 48 h. Aromatase mRNA was only expressed at 24-48 h after FSH, a pattern that was not altered by phosphodiesterases or phosphatases. In the luteinized (PO/hCG) granulosa cells, immunoreactive C subunit was localized in a punctate pattern in the nucleus as well as to a cytoplasmic basket-like structure, a distribution pattern not altered by forskolin. Aromatase, Sgk, and phospho-CREB were expressed at elevated levels in a non-forskolin-responsive manner. Most notable, both phospho-CREB and Sgk were preferentially localized in a punctate pattern within the cytoplasm and not altered by forskolin. Collectively, these data indicate that when granulosa cells differentiate to luteal cells the subcellular localization (nuclear vs. cytoplasmic) of A-kinase pathway components changes markedly. Thus, either the mechanisms of nuclear import and export or the presence of distinct docking sites (and functions ?) dictate where A-kinase, phospho-CREB and Sgk are localized in granulosa cells compared with the terminally differentiated luteal cells.

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Year:  1999        PMID: 10446906     DOI: 10.1210/mend.13.8.0334

Source DB:  PubMed          Journal:  Mol Endocrinol        ISSN: 0888-8809


  22 in total

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2.  DNA methylation and histone modifications are associated with repression of the inhibin α promoter in the rat corpus luteum.

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3.  Defective gonadotropin-dependent ovarian folliculogenesis and granulosa cell gene expression in inhibin-deficient mice.

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4.  Gene expression profiling reveals Cyp26b1 to be an activin regulated gene involved in ovarian granulosa cell proliferation.

Authors:  Jingjing L Kipp; Ann Golebiowski; Guadalupe Rodriguez; Michael Demczuk; Signe M Kilen; Kelly E Mayo
Journal:  Endocrinology       Date:  2010-11-17       Impact factor: 4.736

5.  Follicle-stimulating hormone and estradiol interact to stimulate glutathione synthesis in rat ovarian follicles and granulosa cells.

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Journal:  Biol Reprod       Date:  2009-06-10       Impact factor: 4.285

6.  Mitogen-activated protein kinase regulates FSH-induced expression of tissue-type plasminogen activator through an activator protein 1 response element.

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Authors:  Joshua Cottom; Lisa M Salvador; Evelyn T Maizels; Scott Reierstad; Youngkyu Park; Daniel W Carr; Monika A Davare; Johannes W Hell; Stephen S Palmer; Paul Dent; Hisaaki Kawakatsu; Masato Ogata; Mary Hunzicker-Dunn
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8.  Negative regulation of SEK1 signaling by serum- and glucocorticoid-inducible protein kinase 1.

Authors:  Myung Jin Kim; Ji Soo Chae; Kwang Je Kim; Sang Gil Hwang; Kyoung Wan Yoon; Eun Kyung Kim; Hee Jae Yun; Jun-Ho Cho; Jeehyun Kim; Bong-Woo Kim; Hyung-Chul Kim; Sang Sun Kang; Florian Lang; Ssang-Goo Cho; Eui-Ju Choi
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9.  Transcription of steroidogenic acute regulatory protein in the rodent ovary and placenta: alternative modes of cyclic adenosine 3', 5'-monophosphate dependent and independent regulation.

Authors:  Natalie Yivgi-Ohana; Noa Sher; Naomi Melamed-Book; Sarah Eimerl; Moriah Koler; Pulak R Manna; Douglas M Stocco; Joseph Orly
Journal:  Endocrinology       Date:  2008-10-09       Impact factor: 4.736

10.  Mutations of the lutropin/choriogonadotropin receptor that do not activate the phosphoinositide cascade allow hCG to induce aromatase expression in immature rat granulosa cells.

Authors:  Nebojsa Andric; Mario Ascoli
Journal:  Mol Cell Endocrinol       Date:  2008-02-03       Impact factor: 4.102

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