Your search keyword '"R, Counis"' showing total 141 results

1. Tissue-specific pattern of variant transcripts of the human gonadotropin-releasing hormone receptor gene

Author

ML Kottler, F. Bergametti, S Morice, A. Starzec, R Counis, MC Carre, JP Lagarde, and E Decoret

Subjects

Adenoma, Male, medicine.medical_specialty, DNA, Complementary, RNA Splicing, Endocrinology, Diabetes and Metabolism, Molecular Sequence Data, Pituitary neoplasm, Biology, medicine.disease_cause, Exon, Endocrinology, Internal medicine, Complementary DNA, Testis, medicine, Humans, Pituitary Neoplasms, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Gene, Regulation of gene expression, Mutation, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, General Medicine, Molecular biology, Gene Expression Regulation, Hormone receptor, Pituitary Gland, RNA splicing, Receptors, LHRH

Abstract

The expression pattern of the GnRH receptor was investigated in a variety of normal and neoplastic human tissues by RT-PCR-Southern blotting. In addition to the full-length cDNA (sb1), we identified two other transcripts: the first (sb2) was characterized by a 128 bp deletion as previously described; the second was an unexpected finding composed of a shorter cDNA (sb3), the sequence of which revealed a 220 bp deletion corresponding in size to exon 2. These three transcripts were found in normal pituitary and pituitary adenomas, and in granulosa tumors, but not in testis, where sb2 was lacking. Only sb1 was expressed in normal, fibrocystic and malignant breast tissue. No transcript with a full-length region was found in endometrium, intestine or lymphocytes. This is the first report that shows that splicing of the gonadotropin-releasing hormone receptor gene is tissue dependent. We also determined the intron-exon nucleotide sequence of the gene and identified an MaeIII polymorphic site in exon 1 created by a silent C453T transition found in 10% of unrelated French whites.

Published

1999

2. International symposium on G Protein-Coupled Receptors

Author

D Hervé, D. Vergé, D.L Shi, R Counis, and J Cohen-Tannoudji

Subjects

Cell Biology, General Medicine, Biology, G protein-coupled receptor, Cell biology

Published

2004

3. Identification of Interacting Partners for the Mammalian GnRH Receptor. Impact on Receptor Signaling

Author

V Simon, G Garrel, C Denoyelle, C Avet, R Counis, and J Cohen-Tannoudji

Published

2010

4. Effects of Central Fatty Acids on Neuroendocrine and Endocrine Control of Reproduction

Author

G Garrel, V Simon, C Cruciani-Guglielmacci, S Migrenne, C Denoyelle, C Magnan, R Counis, and J Cohen-Tannoudji

Published

2010

5. Detection of HIV-1 infections by PCR: evaluation in a seropositive subject population

Author

A Akar, B Bournique, F Ajana, R Scholler, H Broly, and R Counis

Subjects

Molecular Sequence Data, Population, CD4-CD8 Ratio, Human immunodeficiency virus (HIV), HIV Infections, HIV Antibodies, Biology, medicine.disease_cause, Polymerase Chain Reaction, Sensitivity and Specificity, Virus, law.invention, Serology, law, HIV Seropositivity, medicine, Humans, education, Molecular Biology, Polymerase chain reaction, HIV Long Terminal Repeat, education.field_of_study, Base Sequence, virus diseases, Cell Biology, Genes, gag, Virology, DNA, Viral, Immunology, HIV-1, Primer (molecular biology), Oligonucleotide Probes

Abstract

To study the polymerase chain reaction (PCR) performance in detecting human immunodeficiency virus (HIV) infections, we tested 53 HIV-1 seropositive patients and 29 HIV-1 seronegative subjects for four different HIV-1 DNA regions. Fifty-one seropositive patients were found positive by PCR with at least one primer pair, but two were repeatedly negative for all primers. Weekly blood samples from 12 seropositive subjects all detected positive for at least one primer pair, but for three patients an irregular primer detection pattern was found. One additional HIV-1 seropositive sample, found negative for HIV DNA, was also negative for the beta-globin PCR control. The 29 seronegative specimens were HIV-1 DNA negative, as was a HIV-2 seropositive patient. This study demonstrates that PCR is almost as good as serological tests for detecting HIV infections, with a specificity of 100% and a sensitivity of 96% and that resampling the patients may improve detection performance.

Published

1992

6. Localization of luteinizing hormone β-mRNA by in situ hybridization in the sheep pars tuberalis

Author

J. Pelletier, Yves Tillet, R. Counis, and M. de Reviers

Subjects

Male, medicine.medical_specialty, Pituitary gland, Histology, In situ hybridization, Biology, Pathology and Forensic Medicine, Species Specificity, Pituitary Gland, Anterior, Internal medicine, medicine, Animals, RNA, Messenger, Northern blot, Cerebral Cortex, Sheep, Nucleic Acid Hybridization, DNA, Cell Biology, Luteinizing Hormone, Blotting, Northern, Molecular biology, Rats, Endocrinology, medicine.anatomical_structure, Gene Expression Regulation, Liver, Organ Specificity, Hypothalamus, Protein Biosynthesis, Median eminence, Pars tuberalis, Luteinizing hormone, Endocrine gland

Abstract

The localization of luteinizing hormone beta (LH beta)-mRNA was studied by in situ hybridization in the pars tuberalis of sheep using a homologous sheep double-stranded 32P- or 35S-cDNA. The labelled cDNA probe detected one mRNA sequence in the pars tuberalis by Northern blot analysis; this sequence was similar to that detected in the pituitary. In situ, the labelling of LH beta-mRNA in the horizontal and sagittal tissue sections was found throughout the pars tuberalis. This labelling was prevented by adding an excess of cold probe or treating the sections by ribonuclease before in situ hybridization. Controls showed a labelling in the pars distalis, but not in the median eminence, hypothalamus, cerebral cortex and liver sections. Double labelling by in situ hybridization followed by immunohistochemistry using a specific LH beta-antiserum indicated that the labelling of LH beta-mRNA appeared more intense in LH-containing cells that were found only in the ventral part of the pars tuberalis. These results suggest that the entire pars tuberalis is able to produce the LH beta subunit, but that the level of translation greatly varies according to the location of the cells.

Published

1992

7. Critical implication of transmembrane Phe310, possibly in conjunction with Trp279, in the rat gonadotropin-releasing hormone receptor activation

Author

S, Chauvin, M, Hibert, A, Bérault, and R, Counis

Subjects

Models, Molecular, Sequence Homology, Amino Acid, Protein Conformation, Phenylalanine, Molecular Sequence Data, Tryptophan, Membrane Proteins, CHO Cells, Rats, Cricetinae, Animals, Humans, Amino Acid Sequence, Receptors, LHRH

Abstract

The GnRH-R belongs to the superfamily of heptahelical GPCRs. A three-dimensional model of GnRH binding to its receptor predicted that Trp3 was the most deeply buried residue, potentially allowing it to interact with both Trp279, a highly conserved residue in the TMH 6 of GPCRs, and Phe310, present essentially in TMH 7 of GnRH-Rs. Replacement of Phe310 with Leu, the most common positional residue in GPCRs, induced a slightly decreased Bmax (1.6-fold) and affinity (3.8-fold); in addition, IP production was completely abolished. Similarly, replacement of Trp279 with Ser depressed the Bmax by 5.2-fold, the affinity by 2.3-fold, and totally abrogated IP production. The effect of the double mutation was not additive on binding, since the Bmax was reduced to the level of the Phe310Leu mutant, although the Kd was restored to a value not significantly different from that of the wild-type. The double mutant was also unable to induce IP production. Unexpectedly, no influence of any single or double substitution was noted on receptor internalization. These data provide evidence for the crucial role of Phe310, possibly in conjunction with Trp279, on GnRH transduction and suggest that the conformation for phospholipase C activation may not be required for GnRH-R internalization.

Published

2001

8. A new compound heterozygous mutation of the gonadotropin-releasing hormone receptor (L314X, Q106R) in a woman with complete hypogonadotropic hypogonadism: chronic estrogen administration amplifies the gonadotropin defect

Author

M L, Kottler, S, Chauvin, N, Lahlou, C E, Harris, C J, Johnston, J P, Lagarde, P, Bouchard, N R, Farid, and R, Counis

Subjects

Protein Conformation, Hypogonadism, Molecular Sequence Data, Estrogens, CHO Cells, Luteinizing Hormone, Phenotype, Haplotypes, Glycoprotein Hormones, alpha Subunit, Cricetinae, Mutation, Animals, Humans, Female, Amino Acid Sequence, RNA, Messenger, Follicle Stimulating Hormone, Child, Gonadotropins, Receptors, LHRH

Abstract

We describe a woman with complete hypogonadotropic hypogonadism and a new compound heterozygous mutation of the GnRH receptor (GnRHR) gene. A null mutation L314X leading to a partial deletion of the seventh transmembrane domain of the GnRHR is associated with a Q106R mutation previously described. L314X mutant receptor shows neither measurable binding nor inositol phosphate production when transfected in CHO-K1 cells compared to the wild-type receptor. The disease is transmitted as an autosomal recessive trait, as shown by pedigree analysis. Heterozygous patients with GnRHR mutations had normal pubertal development and fertility. The present study shows an absence of LH and FSH response to pulsatile GnRH administration (20 microg/pulse, sc, every 90 min). However, GnRH triggered free alpha-subunit (FAS) pulses of small amplitude, demonstrating partial resistance to pharmacological doses of GnRH. FSH, LH, and FAS concentrations were evaluated under chronic estrogen treatment and repeat administration of GnRH. Not only were plasma FSH, LH, and FAS concentrations decreased, but FAS responsiveness was reduced. This new case emphasizes the implication of the GnRH receptor mutations in the etiology of idiopathic hypogonadotropic hypogonadism. We also have evidence for a direct negative estrogen effect on gonadotropin secretion at the pituitary level, dependent on the GnRHR signaling pathway.

Published

2000

9. Mutations of the GnRH receptor gene: a new cause of autosomal-recessive hypogonadotropic hypogonadism

Author

M L, Kottler, R, Counis, and P, Bouchard

Subjects

Gonadotropin-Releasing Hormone, Hypogonadism, Molecular Sequence Data, Mutation, Animals, Humans, Genes, Recessive, Amino Acid Sequence, Receptors, LHRH

Abstract

Mutations in a few genes have been identified in hypogonadotropic hypogonadism (HH): the gene KAL-1 is involved in X-linked Kallmann syndrome associated with anosmia and mutations in transcription factors, namely, DAX-1 and Prop-1 were also evidenced when associated with other pituitary or endocrine defects. Recently, compound heterozygote mutations in the GnRH receptor gene were described both in males and females and hormonal resistance was confirmed in vitro. There is a wide spectrum of phenotype, ranging from complete HH with lack of pubertal development and cryptorchidism to partial hypogonadism with an arrest of pubertal development. In complete GnRH resistance, endogenous LH secretory patterns were abnormal, either apulsatile or characterized by a low-normal pulse frequency with small pulses or erratic pulses of low amplitude. In patients with partial resistance, basal LH plasma concentration was low, but FSH level was in the normal range. LH pulse analysis revealed normal frequency with decreased amplitude. Mutations are distributed along the coding sequence, as reported for other GPCRs. However, two hot-spots, Q106R and the R262Q, were observed, regardless of the geographic origin of the patients. In most cases, patients responded to GnRH administration, making the GnRH test inappropriate for screening GnRH resistance in IHH.

Published

2000

10. LH down-regulates gonadotropin-releasing hormone (GnRH) receptor, but not GnRH, mRNA levels in the rat testis

Author

Yannick Lerrant, Annette Bérault, MC Botte, ML Kottler, R Counis, and A Lozach

Subjects

Male, endocrine system, medicine.medical_specialty, medicine.drug_class, Endocrinology, Diabetes and Metabolism, Immunoblotting, Gonadotropin-releasing hormone, Biology, Testicle, Gonadotropic cell, Chorionic Gonadotropin, Gonadotropin-Releasing Hormone, Endocrinology, Internal medicine, Testis, medicine, Animals, Testosterone, RNA, Messenger, Rats, Wistar, Receptor, Analysis of Variance, Triptorelin Pamoate, Luteinizing Hormone, Triptorelin, Rats, medicine.anatomical_structure, Gonadotropin, Luteinizing hormone, Oligopeptides, hormones, hormone substitutes, and hormone antagonists, Receptors, LHRH, medicine.drug, Hormone

Abstract

The demonstration of an inhibitory effect of gonadotropin-releasing hormone (GnRH) agonists upon steroidogenesis in hypophysectomized rats and the presence of mRNA coding for GnRH and GnRH receptors (GnRH-R) in rat gonads suggests that GnRH can act locally in the gonads. To assess this hypothesis, we investigated the effects of GnRH analogs, gonadotropins and testosterone on the levels of both GnRH and GnRH-R mRNA in the rat testis. Using dot blot hybridization, we measured the mRNA levels 2 to 120 h after the administration of the GnRH agonist, triptorelin. We observed an acute reduction of both GnRH and GnRH-R mRNAs 24 h after the injection (about 38% of control). However, the kinetics for testis GnRH-R mRNA were different from those previously found for pituitary GnRH-R mRNA under the same conditions. Initially, the concentrations of serum LH and FSH peaked, then declined, probably due to the desensitization of the gonadotrope cells. In contrast, the GnRH antagonist, antarelix, after 8 h induced a 2.5-fold increase in GnRH-R mRNA, but not in GnRH mRNA, while gonadotropins levels were reduced. Human recombinant FSH had no significant effect on either GnRH or GnRH-R mRNA levels. Inversely, GnRH-R mRNA levels markedly decreased by 21% of that of control 24 h after hCG injection. Finally, 24 h after testosterone injection, a significant increase in GnRH-R mRNA levels (2.3 fold vs control) was found, but a reduction in the concentration of serum LH, probably by negative feedback on the pituitary, was observed. In contrast, GnRH mRNA levels were not significantly altered following testosterone treatment. Since LH receptors, GnRH-R and testosterone synthesis are colocalized in Leydig cells, our data suggest that LH could inhibit the GnRH-R gene expression or decrease the GnRH-R mRNA stability in the testis. However, this does not exclude the possibility that GnRH analogs could also affect the GnRH-R mRNA levels via direct binding to testicular GnRH-R. In contrast, the regulation of GnRH mRNA levels appeared to be independent of gonadotropins. Taken together, our results suggest a regulation of GnRH and GnRH-R mRNA specific for the testis.

Published

1999

11. Multiple elements in the distal part of the 1.2 kb 5'-flanking region of the rat GnRH receptor gene regulate gonadotrope-specific expression conferred by proximal domain

Author

H, Pincas, Z, Forraï, S, Chauvin, J N, Laverrière, and R, Counis

Subjects

Base Sequence, Models, Genetic, Transcription, Genetic, Molecular Sequence Data, Response Elements, Transfection, Polymerase Chain Reaction, Cell Line, Rats, Gene Expression Regulation, Genes, Reporter, Organ Specificity, Cricetinae, Animals, RNA, Messenger, Cloning, Molecular, Promoter Regions, Genetic, Sequence Alignment, Receptors, LHRH, Sequence Deletion

Abstract

Several lines of evidence indicate that the number of GnRH receptors (GnRH-R) and therefore, gonadotrope responsiveness to GnRH, is highly dependent upon the level of GnRH-R mRNA. To explore this aspect of regulation, we have isolated a 3.3 kb fragment encompassing the promoter region of the rat GnRH-R gene. Primer extension and RNase protection assays allowed the identification of five major transcriptional start sites located within the 110 bp region upstream of the translation start codon. Transfection experiments using the CAT reporter gene demonstrated that the 1261 bp 5' flanking region is required to direct high efficient expression in the gonadotrope-derived alphaT3-1 cell line thus contrasting with mouse in which the only 500 bp proximal sequence appeared to be sufficient. Another difference between rat and mouse was apparent in the 183 bp region of the rat promoter which induced a 3-fold stimulation of thymidine kinase promoter activity in both alphaT3-1 and CHO cells. Subsequent deletion analysis of the region residing between -1261 and -519 revealed the presence of multiple regulatory domains that contributed to the cell-specific activity. However, despite this efficiency in the context of the wild-type promoter, they failed to induce the activity of the minimal thymidine kinase (TK) promoter in the absence of the proximal 600 bp promoter region. Accordingly, a composite TK promoter containing the entire 1.2 kb promoter induced a 10-fold increase in the activity of the TK promoter in alphaT3-1 cells. Taken together these data suggest that distal regulatory regions are critical and require cooperation with proximal specific-promoter elements for activating basal R-GnRH gene expression in gonadotrope cells.

Published

1998

12. The GnRH receptor gene is preferentially expressed in functioning gonadotroph adenomas and displays a Mae III polymorphism site

Author

M L, Kottler, D, Seret-Bégué, N, Lahlou, M, Assayag, M C, Carré, J P, Lagarde, C, Ajzenberg, S, Christin-Maitre, P, Bouchard, J, Mikol, R, Counis, and A, Warnet

Subjects

Adenoma, Adult, Male, Heterozygote, Polymorphism, Genetic, Adolescent, Base Sequence, Molecular Sequence Data, Gene Expression, Middle Aged, Immunohistochemistry, Polymerase Chain Reaction, Gonadotropins, Pituitary, Humans, Female, Pituitary Neoplasms, Receptors, LHRH, Aged

Abstract

Given the central role of the GnRH receptor (GnRHR) in the regulation of the gonadotrophin secretion, it might be implicated directly or indirectly in the pathogenesis of gonadotroph tumours.We determined if GnRHR mRNA was expressed in gonadotroph tumours using RT-PCR and analysed the GnRHR gene for the presence of mutations in its coding region, using direct sequencing of PCR products. Results were analysed according to the pattern of expression of alpha, beta-FSH and beta-LH subunit (SU) genes.RNA was extracted from 20 gonadotroph tumours identified by immunohistochemistry (10% of stained cells): 9 adenomas were functioning (high serum gonadotrophin levels), 3 were associated with high alpha-SU levels and 8 were nonfunctioning. Genomic DNA was extracted from 64 normal subjects.We found GnRHR mRNA in 12 tumours (60%): 8/9 functioning (88%), 1/3 alpha-secreting (33%) and 3/8 nonfunctioning (37.5%) gonadotroph adenomas. There was a significant association between GnRHR expression and immunostaining for beta-FSH (P = 0.014). The nucleotide sequence of the amplified products was identical to that of human pituitary except for the presence, in 3 functioning adenomas, of a silent C to T transition at nucleotide 453 encoding for the serine residue situated in the second intracellular loop at position 151. Heterozygosity provided evidence that both alleles were transcribed in these tumours. This substitution creates a Mae III restriction site. Genomic DNA from normal subjects were then tested for the presence of this new polymorphism. The frequency of the heterozygosity (18.7%) was not significantly different from that found in gonadotroph tumours (25%) and this new Mae III polymorphism site cannot be used as a tumoural marker.The GnRHR gene is preferentially expressed in functioning rather than in nonfunctioning gonadotroph adenomas, but no mutations altering the coding region of the gene were found to further substantiate its role in the pathogenesis of gonadotroph tumours.

Published

1998

13. Fetal expression of GnRH and GnRH receptor genes in rat testis and ovary

Author

AM Chamagne, MC Carre, ML Kottler, R Counis, and MC Botte

Subjects

Male, endocrine system, medicine.medical_specialty, medicine.drug_class, Endocrinology, Diabetes and Metabolism, Gene Expression, Ovary, Testicle, Biology, Gonadotropin-Releasing Hormone, Rats, Sprague-Dawley, Embryonic and Fetal Development, Endocrinology, Internal medicine, Gene expression, Testis, medicine, Animals, RNA, Messenger, Receptor, Electrophoresis, Agar Gel, Messenger RNA, Reverse Transcriptase Polymerase Chain Reaction, Peptidylprolyl Isomerase, Gonadotropin secretion, Rats, Blotting, Southern, medicine.anatomical_structure, Hormone receptor, Female, Gonadotropin, hormones, hormone substitutes, and hormone antagonists, Receptors, LHRH, Densitometry

Abstract

The identification of gonadal gonadotropin-releasing hormone receptors (GnRH-R) and evidence of direct inhibitory effects of GnRH agonists upon steroidogenesis in adult rat gonads, lend credence to a putative intragonadal role of a locally secreted GnRH or GnRH-like peptide. Using reverse transcription-polymerase chain reaction followed by Southern blot hybridization and sequencing, we identified, both in the ovary and in the testis of fetal and adult rats, a fully processed GnRH messenger RNA (mRNA), the sequence of which, in adult testis, was identical to that found in the hypothalamus. We also detected in the testis, but not in the ovary, a transcript containing the first intron. The ontogeny of GnRH and GnRH-R gene expression was studied in rat gonads from 14.5 to 21.5 days post-coitum (dpc), using dot blot hybridization of total RNA. During this period, the levels of cyclophilin mRNA normalized to total RNA remained unchanged. Thus, we used cyclophilin as an internal standard. GnRH mRNA was detected in the ovary at 18.5 dpc, four days later than in the testis, and similar levels were found in both sexes at birth. GnRH-R mRNA was present at 14.5 dpc in the testis and at 15.5 dpc in the ovary, with the levels at 21.5 dpc being 2.4 times higher in the testis than in the ovary. GnRH and GnRH-R mRNA levels increased in both sexes in late fetal development, but this increase appeared two days sooner in the ovary compared with the testis, thus supporting the hypothesis that expression of the GnRH and GnRH-R genes is regulated in a sex-dependent manner during fetal development. In all cases, expression of GnRH and GnRH-R preceded gonadotropin receptors in the gonads and initiation of gonadotropin secretion by the pituitary.

Published

1998

14. GnRH and PACAP action in gonadotropes: cross-talk between phosphoinositidase C and adenylyl cyclase mediated signaling pathways

Author

C A, McArdle and R, Counis

Abstract

In order to respond appropriately to their environment, gonadotropes, like other cells, must integrate informational input from multiple ligands acting through multiple intracellular signaling pathways. In recent years, an increasing number of examples of functional interactions between the phosphoinositidase C (PIC) and adenylyl cyclase signaling pathways in gonadotropes have been described, and the discovery that these cells are targets for pituitary adenylyl cyclase activating peptide (PACAP) has provided a physiological context for earlier work on gonadotrope regulation by cAMP. It has become clear that gonadotropes possess multiple PIC-coupled receptor types, in addition to receptors activating adenylyl and guanylyl cyclases, so that the potential for both coincidence signaling and cross-talk in these cells is immense; examples of both are seen in the effects of PACAP and GnRH on Ca(2+) mobilization and adenylyl cyclase activation in alphaT3-1 cells. In these cells, GnRH, acting via PIC-coupled receptors, can dramatically inhibit adenylyl cyclase activated by PACAP, but can also alter cellular levels of protein kinase A subunits, providing a mechanism for coordinated regulation of both messenger and effector.

Published

1996

15. G Protein-Coupled Receptors: New insights into signaling and regulation

Author

D Hervé, R Counis, J Cohen-Tannoudji, D.L Shi, and D. Vergé

Subjects

G protein-coupled receptor kinase, GTPase-activating protein, Cell Biology, General Medicine, Biology, Receptor, Neuroscience, Cell biology, G protein-coupled receptor

Published

2004

16. Changes in LHbeta-gene and FSHbeta-gene expression in the ram pars tuberalis according to season and castration

Author

M. de Reviers, R. Counis, M. Moumni, Yves Tillet, and J. Pelletier

Subjects

Male, medicine.medical_specialty, Histology, medicine.drug_class, In situ hybridization, Biology, Pathology and Forensic Medicine, chemistry.chemical_compound, Follicle-stimulating hormone, Internal medicine, Gene expression, medicine, Animals, Castration, RNA, Messenger, Messenger RNA, Sheep, Brain, Cell Biology, Luteinizing Hormone, beta Subunit, Immunohistochemistry, Endocrinology, chemistry, Gene Expression Regulation, Follicle Stimulating Hormone, beta Subunit, Female, Pars tuberalis, Seasons, Gonadotropin, Luteinizing hormone

Abstract

Luteinizing hormone beta (LHβ) and follicle stimulating hormone beta (FSHβ) subunits and their mRNAs were studied in the ram pars tuberalis following different seasonal (winter vs summer) and experimental (intact vs castrated animals) conditions. Hormone-containing cells were identified by immunohistochemistry, and mRNAs for LHβ and FSHβ by in situ hybridization using homologous double-stranded 35S-cDNAs. The labelling was quantified by image analysis. Immunohistochemical staining showed that cells containing LHβ and FSHβ were localized mainly in the ventral part of the pars tuberalis but that, in the summer, additional LHβ-containing cells were present in the dorsal part in intact rams. On the other hand, LHβ-mRNA labelling was found in the whole pars tuberalis in wethers but only in the ventral part in intact rams. The magnitude of LHβ-mRNA labelling was significantly greater in summer than in winter rams, and in castrated than in intact animals (P

Published

1995

17. [Cyclic AMP: role in the synthesis and release of luteinizing hormone]

Author

A, Starzec, N, Bouamoud, M, Jutisz, and R, Counis

Subjects

Gonadotropin-Releasing Hormone, Male, Pituitary Gland, Anterior, Cyclic AMP, Dactinomycin, Radioimmunoassay, Animals, Rats, Inbred Strains, Cycloheximide, In Vitro Techniques, Luteinizing Hormone, Rats

Abstract

GnRH is capable of inducing an increase in cyclic AMP (AMPc) production in the anterior pituitary gland. However, this intracellular messenger is not involved in the mechanisms leading to acute release of gonadotropins. Using anterior pituitary cells in culture, we recently found that AMPc, like GnRH, stimulated the expression of genes encoding for LH and consequently increased the synthesis of LH subunits. To reevaluate the role of AMPc in the secretion of pituitary gonadotropins, we first studied the effects of 8-Br-AMPc, a permeant AMPc analog, on LH release during a 48-hour period. Direct activation of protein kinases A by 8-Br-AMPc substantially stimulated LH release, to values as high as those seen with GnRH under the optimal conditions used in this experiment. However, kinetics were different, with GnRH inducing a rapid rise in LH and 8-Br-AMPc causing a gradual increase after a five-hour lag. We also studied the effects of 8-Br-AMPc on the release of neosynthesized subunits. Pituitary cells were incubated with 35S-Met, and labeled alpha and LH beta polypeptides were recovered in parallel from the cells and medium. We observed that 8-Br-AMPc stimulated not only LH synthesis but also release of newly synthesized LH subunits, in this respect 8-Br-AMPc was more effective than GnRH. After five hours incubation with 1.5 mM 8-Br-AMPc, 95% of the alpha subunit and 40% of the LH beta subunit that had been newly synthesized were released into the medium, whereas the corresponding figures with exposure to 10 nM GnRH were 80% and 15% respectively.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1990

18. [Genes of pituitary gonadotropin hormones and their regulation]

Author

R, Counis

Subjects

Gene Expression Regulation, Genes, Molecular Structure, Protein Biosynthesis, Animals, Humans, RNA, Messenger, Follicle Stimulating Hormone, Luteinizing Hormone

Abstract

LH and FSH are produced in the pituitary gonadotropes; each contains two subunits, a common alpha and a unique LH beta- or FSH beta-subunit. All 3 subunits are synthesized as precursors, encoded by separate genes. Gonadotropin subunit messenger RNAs from different species have been isolated and characterized, their nucleotide sequence has been determined after synthesis and cloning of the complementary DNA. In this way, the primary structure of corresponding precursors has been obtained. The post-translational processing of the precursors which results in the formation of native glycosylated subunits has been studied in situ. Finally the gonadotropin subunit genes have been isolated and their structure elucidated, confirming the hypothesis that they evolved from a common ancestral gene. The different approaches used to study gonadotropin synthesis has allowed the demonstration of the hormonal regulation of the expression of the gonadotropin subunit genes. Hormones that affect gonadotropin release, such as gonadal steroids, GnRH, inhibin and thyroid hormones, also influence subunit gene expression, in a complex and varied manner, the mechanisms of which are still unclear. For example, at least part of the in vivo effects of oestradiol (inhibitory) or thyroid hormones (stimulatory at low doses) result from an indirect action via the hypothalamus, which probably affects GnRH secretion. It is now well established that GnRH stimulates gene expression and the synthesis of gonadotropin subunits. These effects are reproduced by direct activation of protein kinases A and C, in a manner which suggests a coordinate control of both synthesis and release of gonadotropins, through the mediation of intracellular signalling pathways (cyclic AMP, and phosphatidyl inositol hydrolysis). Gene transfer studies have demonstrated the presence of regulatory elements in the 5'-flanking regions of the (human) alpha gene that confer sensitivity to different factors including tri-iodothyronine, glucocorticoids, and cyclic AMP. The identification of regulatory domains of the genes in conjunction with studies using gonadotrope cells will help deepen our understanding or the cellular and molecular mechanisms involved in the multihormonal control of gonadotropin subunit synthesis.

Published

1990

19. Glycosylation process in gonadotrophs: a quantitative electron microscope autoradiographic study with labeled glucosamine

Author

I. Hurbain-Kosmath, Marian Jutisz, and R Counis

Subjects

Male, medicine.medical_specialty, Glycosylation, Golgi Apparatus, In Vitro Techniques, Biology, Cytoplasmic Granules, Endoplasmic Reticulum, law.invention, chemistry.chemical_compound, symbols.namesake, Anterior pituitary, Pituitary Gland, Anterior, Glucosamine, law, Internal medicine, Organelle, medicine, Animals, Tunicamycin, Endoplasmic reticulum, Biological Transport, Cell Biology, General Medicine, Golgi apparatus, Rats, Cell biology, Microscopy, Electron, Endocrinology, medicine.anatomical_structure, chemistry, Gonadotropins, Pituitary, symbols, Autoradiography, Electron microscope, Orchiectomy, Protein Processing, Post-Translational

Abstract

Incorporation of [3H]glucosamine into dispersed anterior pituitary cells was studied by electron microscope autoradiography. Gonadotrophs were examined to determine the intracellular route and kinetic patterns of glycosylation. Studies were performed with cells from; (a) normal adult male rats; (b) rats orchidectomized 3 wk earlier; and (c) orchidectomized rats treated with tunicamycin. Our results show that incorporation of [3H]glucosamine first occurs in the rough endoplasmic reticulum (RER), then proceeds in the Golgi elements (where peripheral carbohydrates are attached). Treatment with tunicamycin results in a decrease in labeling of these 2 organelles. Comparison of the kinetic patterns in normal and castrated male rats shows that the accumulation of labeled glycosylated proteins in granules reaches a plateau within 2 hr post-pulse in normal rats, and rises during a 6-hr chase in castrated rats. However, because of the necessity for a rather long 15 min pulse, we cannot exclude the possibility that incorporation of glucosamine during the pulse may occur concomitantly in the RER and the Golgi saccules, to be followed by rapid transfer to the secretory granules.

Published

1987

20. Functional importance of transmembrane helix 6 Trp(279) and exoloop 3 Val(299) of rat gonadotropin-releasing hormone receptor.

Author

S, Chauvin, A, Brault, Y, Lerrant, M, Hibert, and R, Counis

Abstract

Previous studies have established that the interaction of gonadotropin-releasing hormone (GnRH) with its receptor (GnRHR) would require partial entry of the N- and C-terminal regions of ligand into the transmembrane core. The functional significance of the conserved aromatic residue Trp(279) present in the transmembrane helix 6, and Val(299) located in exoloop 3 of the rat GnRHR was investigated by mutagenesis followed by expression in Chinese hamster ovary-K1 cells. Compared with wild-type, substitution of Trp(279) with Ser or Arg resulted in a marked reduction or total abolition, respectively, of ligand binding and, in both cases, abrogation of GnRH-induced inositol phosphate production. A total absence of functionality was observed when Val(299) was simply replaced with Ala. Mention should be made that an expression of all mutated and wild-type receptor proteins was observed. Interestingly, the double mutant [Trp(279)Arg/Val(299)Ala]GnRHR restored B(max) to wild type (504 +/- 43 versus 541 +/- 41 fmol/mg protein), but with a diminished affinity (4.95 +/- 1.05 versus 0.94 +/- 0.35 nM), and GnRH failed to induce inositol phosphate. No influence of the mutations was seen on internalization of the receptor. The three-dimensional model of GnRH binding to the rat GnRHR was built predicting that Trp(279) is buried at 20 A in the transmembrane core of the receptor, directly in contact with Trp(3) of GnRH. In contrast, Val(299) is located in a region that cannot be precisely defined at the extracellular end of transmembrane helix 7. Although models cannot provide any clue concerning the observed interactivity between the two distal residues, altogether these data reveal the functional importance of both GnRHR Trp(279) and Val(299) and suggest that Trp(279), interacting with GnRH Trp(3), represents the bottom of the binding pocket.

Published

2000

21. Demasquage presumé des récepteurs de la noradrénaline par enrichissement en acide linoléique des phospholipides membranaires de la cellule adipeuse

Author

R Counis

Subjects

medicine.medical_specialty, Linoleic acid, Biophysics, Phospholipid, Adipose tissue, Adenylate kinase, Stimulation, Biology, Biochemistry, Cyclase, In vitro, chemistry.chemical_compound, Endocrinology, chemistry, Internal medicine, medicine, heterocyclic compounds, Hormone

Abstract

Membrane phospholipid composition influences the noradrenaline reactivity of adipose cell ghosts in vitro. Basal and fluoride-stimulated adenylate cyclase activities and the phosphodiesterase activity were unchanged whether or not structural phospholipids were enriched in linoleic acid. However, the adenylate cyclase activation increased with increased proportion of essential fatty acids, under in vitro hormonal stimulation.

Published

1973

22. Démasquage des récepteurs de la noradrénaline par enrichissement en acide linoléique des phospholipides membranaires de la cellule adipeuse I. Act1vité lipase

Author

R. Counis, C. Loriette, J.P. Carreau, and P. Ketevi

Subjects

chemistry.chemical_classification, biology, Linoleic acid, Biophysics, Phospholipid, Adipose tissue, Stimulation, Biochemistry, In vitro, chemistry.chemical_compound, Endocrinology, chemistry, Essential fatty acid, biology.protein, Lipase

Abstract

The membrane phospholipid configuration, in relation to the essential fatty acid concentration, do not seem to have any influence on the basal lipolytic activity of adipose cells. However, under the stimulation of in vitro added noradrenaline, an obvious correlation exists between linoleic acid concentrations and hormone-sensitive lipase activities.

Published

1972

23. [Adenylate cyclase/Lipase. Hormone receptor induction]

Author

T, Cresteil, R, Counis, and J, Raulin

Subjects

Guinea Pigs, Age Factors, Gestational Age, Receptors, Cell Surface, DNA, Lipase, Glucagon, Fluorides, Norepinephrine, Fetus, Adipose Tissue, Brown, Adrenocorticotropic Hormone, Animals, Newborn, Animals, Adenylyl Cyclases

Abstract

An adenylate cyclase activity (AC) was found in guinea pig brown adipose tissue (BAT), since the tissue's apparition. This enzymatic activity increased during the development and showed high values at the end of gestation. An increase of AC units per cell was observed, in addition to the cell multiplication. A norepinephrine stimulation of AC activity was observed at the end of gestation : this regulating action disappeared in the first days of extrauterine life. Neither glucagon nor ACTH had any regulating role upon AC activity during fetal and newborn life. The basal lipolytic activity which was observed in BAT of fetuses (61rst day) and neonate dramatically around the 15th day. A potent lipolysis activation by norepinephrine was observed, but only after birth. The correlation observed between these enzymatic activities in presence of norepinephrine seems to indicate that the AC/lipase system was involved in the neonatal thermogenesis of guinea pigs.

Published

1975

24. [In situ biosynthesis of LH in cultured anterior pituitary cells: effects of GnRH]

Author

R, Counis, A, Starzec, and M, Jutisz

Subjects

Male, Threonine, Glycoprotein Hormones, alpha Subunit, Pituitary Gland, Anterior, Pituitary Hormones, Anterior, Tunicamycin, Animals, Rats, Inbred Strains, Luteinizing Hormone, Pituitary Hormone-Releasing Hormones, Cells, Cultured, Rats

Abstract

In order to investigate the biosynthetic pathway of LH subunits, anterior pituitary cells were cultured in the presence of [35S]Met and polypeptides immunologically-related (i.r.) to the alpha and LH beta subunits were isolated from cells and media using specific antisera. SDS-polyacrylamide gel electrophoresis allowed us to identify 3 forms of alpha polypeptide differing in their apparent Mr: 21 K, 23 K and 25 K. Pulse-chase experiments showed the 21 K peptide (partially glycosylated) being successively converted into 23 K (authentic alpha) and 25 K ("hyperglycosylated") peptides, with spontaneous release of the 2 larger forms into the medium. With regard to LH beta, a single polypeptide of Mr 19 K was resolved by electrophoresis from material immuno-precipitated with antiserum to LH beta. This LH beta-related polypeptide was primarily present in cells, and only in trace amounts in the medium. When the incubation of cells was performed in the presence of tunicamycin (an inhibitor of glycosylation), a 16 K i.r.-form of alpha was observed, corresponding to the apopeptide alpha. The use of hydroxynorvaline, which substitutes for threonine thereby blocking glycosylation sites, induced accumulation of the 21 K-form. In the presence of GnRH (10-40 nM), the rate of synthesis of the polypeptide chains of the LH subunits increased, whether or not glycosylation was blocked, suggesting that GnRH has no direct effect on glycosylation. GnRH also readily induced the release of the newly synthesized LH subunits. This stimulatory effect of GnRH was more pronounced for the highly glycosylated forms of alpha (23 and 25 K) compared to the 16 and 21 K forms.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1987

25. [Role of gonadal steroids in the regulation of messengers coding for pituitary gonadotropins]

Author

R, Counis, M, Corbani, A, Starzec, M, Schmitt-Ney, and M, Jutisz

Subjects

Gonadotropins, Pituitary, Animals, Nucleic Acid Hybridization, Steroids, DNA, RNA, Messenger, Gonads, Rats

Published

1984

26. Adenylate cyclase assay with [alpha-32P]ATP as substrate. A simple modification for lowering blanks

Author

R, Counis and S, Mongongu

Subjects

Male, Chemistry, Adenosine Triphosphate, Hot Temperature, Adipose Tissue, Chemical Phenomena, Cell Membrane, Aluminum Oxide, Animals, Hydrochloric Acid, Adenylyl Cyclases, Rats

Published

1978

27. [Focus on the biogenesis of hypophyseal gonadotropins]

Author

M, Jutisz, R, Counis, M, Corbani, A, Starzec, and Y, Lerrant

Subjects

Thyroxine, Pituitary Gland, Anterior, Protein Biosynthesis, Gonadotropins, Pituitary, Animals, Nucleic Acid Hybridization, Steroids, RNA, Messenger, Follicle Stimulating Hormone, Luteinizing Hormone, Gonads, Pituitary Hormone-Releasing Hormones, Rats

Abstract

We have studied the regulation of the biosynthesis of pituitary gonadotropins in the rat by gonadal steroids and a hypothalamic hormone, GnRH. The methodology used for studying the action of steroids, was either cell-free translation of pituitary messenger RNAs, or hybridization (Northern blot) with synthetic oligodeoxynucleotides (ODN), and for studying the effect of GnRH, primary anterior pituitary cell culture. Our results show that gonadectomy increases and injection of gonadal steroids into gonadectomized rats diminishes the rate of synthesis of the gonadotropin subunit precursors. Progesterone acts only after induction of its pituitary receptors in ovariectomized rats with estradiol benzoate. Thyroxine modulates the action of steroids. Hybridization experiments suggest that gonadal steroids act on the expression of genes encoding the precursors of gonadotropin subunits. GnRH significantly increases incorporation of the labeled amino acids into polypeptide chains of both alpha and LH beta subunits. Intracellular mediators of hormone action, such as cyclic AMP and diacylglycerols, mimic the stimulatory action of GnRH on the synthesis of LH subunits. However, we have no evidence that these products intervene in the effect of GnRH on the LH subunit synthesis. In conclusion, the synthesis of LH and FSH subunits is regulated, with opposite effects, by gonadal steroids which exert their negative control at the genomic level and by GnRH which proceeds via different, yet unknown mechanisms.

Published

1989

28. Molecular mechanisms involved in the hormonal regulation of prolactin and gonadotropins biosynthesis in the pituitary gland

Author

M, Jutisz and R, Counis

Subjects

Sheep, Models, Genetic, Transcription, Genetic, DNA, Recombinant, Estrogens, Prolactin, Rats, Pituitary Gland, Anterior, Genes, Regulator, Gonadotropins, Pituitary, Animals, Female, RNA, Messenger, Cloning, Molecular

Published

1985

29. [Possible unmasking of noradrenaline receptors by linoleic acid-rich phospholipids in fat cell membranes. II. Adenylate cyclase and phosphodiesterase activities]

Author

R, Counis

Subjects

Epididymis, Male, Phosphoric Diester Hydrolases, Cell Membrane, Phosphorus Isotopes, Receptors, Cell Surface, Rats, Enzyme Activation, Fluorides, Norepinephrine, Adipose Tissue, Linoleic Acids, Animals, Adenylyl Cyclases

Published

1973

30. [Antilipolytic role of tetracycline. Inhibition of adenylate cyclase in vitro]

Author

R, Counis, K, Koumanov, J, Raulin, and R, Infante

Subjects

Male, Norepinephrine, Adipose Tissue, Phosphoric Diester Hydrolases, Animals, Tetracycline, Glucagon, Adenylyl Cyclases, Rats

Published

1973

31. [Relative non-masking of noradrenaline receptors by linoleic acid-rich phospholipids in fat cell membranes. I. Lipase activity]

Author

J P, Carreau, C, Loriette, R, Counis, and P, Ketevi

Subjects

Glycerol, Male, Cell Membrane, Fatty Acids, Proteins, Rats, Inbred Strains, Lipase, In Vitro Techniques, Rats, Receptors, Adrenergic, Norepinephrine, Adipose Tissue, Linoleic Acids, Spectrophotometry, Animals, Phospholipids

Published

1972

32. [Adenylcyclase activity during fetal and neonatal development of brown adipose tissue. Drawback and criticism of measurement methods]

Author

R, Counis and J, Raulin

Subjects

Chromatography, Adenine Nucleotides, Radioimmunoassay, Phosphorus Isotopes, Tritium, Enzymes, Rats, Adenosine Triphosphate, Fetus, Adipose Tissue, Adipose Tissue, Brown, Animals, Newborn, Glucosyltransferases, Methods, Animals, Adenylyl Cyclases

Published

1970

33. [Fetal and neonatal adenylcyclase of adipose tissue. Relation to the essential fatty acid proportion of exogenous lipids]

Author

J P, Carreau, R, Counis, and J, Raulin

Subjects

Norepinephrine, Fetus, Adipose Tissue, Adipose Tissue, Brown, Animals, Newborn, Fatty Acids, Essential, Pregnancy, Animals, Female, Dietary Fats, Maternal-Fetal Exchange, Adenylyl Cyclases, Rats

Published

1971

34. Rat Gnrhr promoter directs species-specific gene expression in the pituitary and testes of transgenic mice.

Author

Ishaq M, Schang AL, Magre S, Laverrière JN, Guillou A, Coudouel N, Wargnier R, Cohen-Tannoudji J, and Counis R

Subjects

Animals, Leydig Cells metabolism, Male, Mice, Mice, Transgenic, Promoter Regions, Genetic genetics, Rats, Rats, Transgenic, Receptors, LHRH genetics, Pituitary Gland metabolism, Receptors, LHRH metabolism, Testis metabolism

Abstract

The GnRH receptor (GnRHR) is expressed in several non-pituitary tissues, notably in gonads. However, mechanisms underlying the gonad-specific expression of Gnrhr are not well understood. Here, Gnrhr expression was analysed in the developing testes and pituitaries of rats and transgenic mice bearing the human placental alkaline phosphatase reporter gene (ALPP) under the control of the rat Gnrhr promoter. We showed that the 3.3 kb, but not the pituitary-specific 1.1 kb promoter, directs ALPP expression exclusively to testis Leydig cells from embryonic day 12 onwards. Real-time PCR analysis revealed that promoter activity displayed the same biphasic profile as marker genes in Leydig cells, i.e. abrupt declines after birth followed by progressive rises after a latency phase, in coherence with the differentiation and evolution of foetal and adult Leydig cell lineages. Interestingly, the developmental profile of transgene expression showed high similarity with the endogenous Gnrhr profile in the rat testis, while mouse Gnrhr was only poorly expressed in the mouse testis. In the pituitary, both transgene and Gnrhr were co-expressed at measurable levels with similar ontogenetic profiles, which were markedly distinct from those in the testis. Castration that induced pituitary Gnrhr up-regulation in rats did not affect the mouse Gnrhr. However, it duly up-regulated the transgene. In addition, in LβT2 cells, the rat, but not mouse, Gnrhr promoter was sensitive to GnRH agonist stimulation. Collectively, our data highlight inter-species variations in the expression and regulation of Gnrhr in two different organs and reveal that the rat promoter sequence contains relevant genetic information that dictates rat-specific gene expression in the mouse context.

Published

2013

35. Mechanisms of action of hormone-sensitive lipase in mouse Leydig cells: its role in the regulation of the steroidogenic acute regulatory protein.

Author

Manna PR, Cohen-Tannoudji J, Counis R, Garner CW, Huhtaniemi I, Kraemer FB, and Stocco DM

Subjects

3-Hydroxysteroid Dehydrogenases genetics, 3-Hydroxysteroid Dehydrogenases metabolism, ATP Binding Cassette Transporter 1, ATP-Binding Cassette Transporters genetics, ATP-Binding Cassette Transporters metabolism, Animals, Bucladesine pharmacology, Carbamates pharmacology, Carrier Proteins genetics, Carrier Proteins metabolism, Cells, Cultured, Cholesterol blood, Cholesterol Esters blood, Cholesterol Side-Chain Cleavage Enzyme genetics, Cholesterol Side-Chain Cleavage Enzyme metabolism, Cyclic AMP metabolism, Cyclic AMP physiology, Cyclic AMP-Dependent Protein Kinases metabolism, Gene Expression Regulation, Gene Knockdown Techniques, Leydig Cells metabolism, Liver X Receptors, Male, Mice, Nicotinic Acids pharmacology, Orphan Nuclear Receptors agonists, Orphan Nuclear Receptors genetics, Orphan Nuclear Receptors metabolism, Oxadiazoles pharmacology, Perilipin-1, Phosphoproteins metabolism, Promoter Regions, Genetic, RNA, Small Interfering genetics, Retinoid X Receptors agonists, Retinoid X Receptors metabolism, Scavenger Receptors, Class B genetics, Scavenger Receptors, Class B metabolism, Second Messenger Systems, Sterol Esterase genetics, Sterol Esterase metabolism, Sterol Regulatory Element Binding Protein 1 genetics, Sterol Regulatory Element Binding Protein 1 metabolism, Tetrahydronaphthalenes pharmacology, Leydig Cells enzymology, Phosphoproteins genetics, Progesterone biosynthesis, Sterol Esterase physiology

Abstract

Hormone-sensitive lipase (HSL) catalyzes the hydrolysis of cholesteryl esters in steroidogenic tissues and, thus, facilitates cholesterol availability for steroidogenesis. The steroidogenic acute regulatory protein (StAR) controls the rate-limiting step in steroid biosynthesis. However, the modes of action of HSL in the regulation of StAR expression remain obscure. We demonstrate in MA-10 mouse Leydig cells that activation of the protein kinase A (PKA) pathway, by a cAMP analog Bt2cAMP, enhanced expression of HSL and its phosphorylation (P) at Ser-660 and Ser-563, but not at Ser-565, concomitant with increased HSL activity. Phosphorylation and activation of HSL coincided with increases in StAR, P-StAR (Ser-194), and progesterone levels. Inhibition of HSL activity by CAY10499 effectively suppressed Bt2cAMP-induced StAR expression and progesterone synthesis. Targeted silencing of endogenous HSL, with siRNAs, resulted in increased cholesteryl ester levels and decreased cholesterol content in MA-10 cells. Depletion of HSL affected lipoprotein-derived cellular cholesterol influx, diminished the supply of cholesterol to the mitochondria, and resulted in the repression of StAR and P-StAR levels. Cells overexpressing HSL increased the efficacy of liver X receptor (LXR) ligands on StAR expression and steroid synthesis, suggesting HSL-mediated steroidogenesis entails enhanced oxysterol production. Conversely, cells deficient in LXRs exhibited decreased HSL responsiveness. Furthermore, an increase in HSL was correlated with the LXR target genes, steroid receptor element-binding protein 1c and ATP binding cassette transporter A1, demonstrating HSL-dependent regulation of steroidogenesis predominantly involves LXR signaling. LXRs interact/cooperate with RXRs and result in the activation of StAR gene transcription. These findings provide novel insight and demonstrate the molecular events by which HSL acts to drive cAMP/PKA-mediated regulation of StAR expression and steroidogenesis in mouse Leydig cells.

Published

2013

36. SET protein interacts with intracellular domains of the gonadotropin-releasing hormone receptor and differentially regulates receptor signaling to cAMP and calcium in gonadotrope cells.

Author

Avet C, Garrel G, Denoyelle C, Laverrière JN, Counis R, Cohen-Tannoudji J, and Simon V

Subjects

Animals, Calcium Signaling, GTP-Binding Proteins metabolism, Humans, Kinetics, Mutagenesis, Site-Directed, Promoter Regions, Genetic, Protein Binding, Protein Structure, Tertiary, RNA, Small Interfering metabolism, Rats, Receptors, LHRH metabolism, Recombinant Proteins metabolism, Signal Transduction, Calcium metabolism, Cyclic AMP metabolism, Gene Expression Regulation, Gonadotrophs metabolism, Receptors, LHRH chemistry

Abstract

In mammals, the receptor of the neuropeptide gonadotropin-releasing hormone (GnRHR) is unique among the G protein-coupled receptor (GPCR) family because it lacks the carboxyl-terminal tail involved in GPCR desensitization. Therefore, mechanisms involved in the regulation of GnRHR signaling are currently poorly known. Here, using immunoprecipitation and GST pull-down experiments, we demonstrated that SET interacts with GnRHR and targets the first and third intracellular loops. We delineated, by site-directed mutagenesis, SET binding sites to the basic amino acids (66)KRKK(69) and (246)RK(247), located next to sequences required for receptor signaling. The impact of SET on GnRHR signaling was assessed by decreasing endogenous expression of SET with siRNA in gonadotrope cells. Using cAMP and calcium biosensors in gonadotrope living cells, we showed that SET knockdown specifically decreases GnRHR-mediated mobilization of intracellular cAMP, whereas it increases its intracellular calcium signaling. This suggests that SET influences signal transfer between GnRHR and G proteins to enhance GnRHR signaling to cAMP. Accordingly, complexing endogenous SET by introduction of the first intracellular loop of GnRHR in αT3-1 cells significantly reduced GnRHR activation of the cAMP pathway. Furthermore, decreasing SET expression prevented cAMP-mediated GnRH stimulation of Gnrhr promoter activity, highlighting a role of SET in gonadotropin-releasing hormone regulation of gene expression. In conclusion, we identified SET as the first direct interacting partner of mammalian GnRHR and showed that SET contributes to a switch of GnRHR signaling toward the cAMP pathway.

Published

2013

37. Identification and analysis of two novel sites of rat GnRH receptor gene promoter activity: the pineal gland and retina.

Author

Schang AL, Bleux C, Chenut MC, Ngô-Muller V, Quérat B, Jeanny JC, Counis R, Cohen-Tannoudji J, and Laverrière JN

Subjects

Animals, CHO Cells, Cells, Cultured, Cricetinae, Cricetulus, Embryo, Mammalian, Gene Expression Profiling, Gene Expression Regulation, Developmental, Humans, Male, Mice, Mice, Transgenic, Organ Specificity genetics, Pineal Gland embryology, Rats, Rats, Sprague-Dawley, Retina embryology, Pineal Gland metabolism, Promoter Regions, Genetic genetics, Receptors, LHRH genetics, Retina metabolism

Abstract

Background and Aims: In mammals, activation of pituitary GnRH receptor (GnRHR) by hypothalamic GnRH increases the synthesis and secretion of LH and FSH, which, in turn, regulate gonadal functions. However, GnRHR gene (Gnrhr) expression is not restricted to the pituitary., Methods: To gain insight into the extrapituitary expression of Gnrhr, a transgenic mouse model that expresses the human placental alkaline phosphatase reporter gene driven by the rat Gnrhr promoter was created., Results: This study shows that the rat Gnrhr promoter is operative in two functionally related organs, the pineal gland, as early as embryonic day (E) 13.5, and the retina where activity was only detected at E17.5. Accordingly, Gnrhr mRNA were present in both tissues. Transcription factors known to regulate Gnrhr promoter activity such as the LIM homeodomain factors LHX3 and ISL1 were also detected in the retina. Furthermore, transient transfection studies in CHO and gonadotrope cells revealed that OTX2, a major transcription factor in both pineal and retina cell differentiation, is able to activate the Gnrhr promoter together with either CREB or PROP1, depending on the cell context., Conclusion: Rather than using alternate promoters, Gnrhr expression is directed to diverse cell lineages through specific associations of transcription factors acting on distinct response elements along the same promoter. These data open new avenues regarding GnRH-mediated control of seasonal and circadian rhythms in reproductive physiology., (Copyright © 2012 S. Karger AG, Basel.)

Published

2013

38. Mechanisms underlying the tissue-specific and regulated activity of the Gnrhr promoter in mammals.

Author

Schang AL, Quérat B, Simon V, Garrel G, Bleux C, Counis R, Cohen-Tannoudji J, and Laverrière JN

Abstract

The GnRH receptor (GnRHR) plays a central role in the development and maintenance of reproductive function in mammals. Following stimulation by GnRH originating from the hypothalamus, GnRHR triggers multiple signaling events that ultimately stimulate the synthesis and the periodic release of the gonadotropins, luteinizing-stimulating hormone (LH) and follicle-stimulating hormones (FSH) which, in turn, regulate gonadal functions including steroidogenesis and gametogenesis. The concentration of GnRHR at the cell surface is essential for the amplitude and the specificity of gonadotrope responsiveness. The number of GnRHR is submitted to strong regulatory control during pituitary development, estrous cycle, pregnancy, lactation, or after gonadectomy. These modulations take place, at least in part, at the transcriptional level. To analyze this facet of the reproductive function, the 5' regulatory sequences of the gene encoding the GnRHR have been isolated and characterized through in vitro and in vivo approaches. This review summarizes results obtained with the mouse, rat, human, and ovine promoters either by transient transfection assays or by means of transgenic mice.

Published

2012

39. Decoding high Gonadotropin-releasing hormone pulsatility: a role for GnRH receptor coupling to the cAMP pathway?

Author

Cohen-Tannoudji J, Avet C, Garrel G, Counis R, and Simon V

Abstract

The gonadotropin-releasing hormone (GnRH) pulsatile pattern is critical for appropriate regulation of gonadotrope activity but only little is known about the signaling mechanisms by which gonadotrope cells decode such pulsatile pattern. Here, we review recent lines of evidence showing that the GnRH receptor (GnRH-R) activates the cyclic AMP (cAMP) pathway in gonadotrope cells, thus ending a long-lasting controversy. Interestingly, coupling of GnRH-R to the cAMP pathway as well as induction of nitric oxide synthase 1 (NOS1) or follistatin through this signaling pathway take place preferentially under high GnRH pulsatility. The preovulatory surge of GnRH in vivo is indeed associated with an important increase of pituitary cAMP and NOS1 expression levels, both being markedly inhibited by treatment with a GnRH antagonist. Altogether, this suggests that due to its atypical structure and desensitization properties, the GnRH-R may continue to signal through the cAMP pathway under conditions inducing desensitization for most other receptors. Such a mechanism may contribute to decode high GnRH pulsatile pattern and enable gonadotrope cell plasticity during the estrus cycle.

Published

2012

40. Unsaturated fatty acids stimulate LH secretion via novel PKCepsilon and -theta in gonadotrope cells and inhibit GnRH-induced LH release.

Author

Garrel G, Simon V, Denoyelle C, Cruciani-Guglielmacci C, Migrenne S, Counis R, Magnan C, and Cohen-Tannoudji J

Subjects

Animals, Cells, Cultured, Gonadotrophs metabolism, Male, Protein Kinase C-theta, Rats, Fatty Acids, Unsaturated pharmacology, Gonadotrophs drug effects, Gonadotropin-Releasing Hormone pharmacology, Isoenzymes physiology, Luteinizing Hormone metabolism, Protein Kinase C physiology, Protein Kinase C-epsilon physiology

Abstract

The activity of pituitary gonadotrope cells, crucial for reproductive function, is regulated by numerous factors including signals related to nutritional status. In this work, we demonstrated, for the first time, that in vivo central exposure of rats to lipids intracarotid infusion of a heparinized triglyceride emulsion selectively increases the expression of pituitary LH subunit genes without any alteration of pituitary GnRH receptor and hypothalamic GnRH or Kiss-1 transcript levels. Furthermore, we showed that unsaturated fatty acids (UFA), oleate and linoleate, increase LH release in a dose-dependent manner as well as LHβ mRNA levels in both immortalized LβT2 gonadotrope cell line and rat primary cell cultures. In contrast, the saturated palmitate was ineffective. ACTH or TSH secretion was unaffected by UFA treatment. We demonstrated in LβT2 cells that linoleate effect is mediated neither by activation of membrane fatty acid (FA) receptors GPR40 or GPR120 although we characterized these receptors in LβT2 cells, nor through nuclear peroxisome proliferator-activated receptors. Furthermore, linoleate β-oxidation is not required for its action on LH secretion. In contrast, pharmacological inhibition of protein kinase C (PKC) or ERK pathways significantly prevented linoleate-stimulated LH release. Accordingly, linoleate was shown to activate novel PKC isoforms, PKCε and -θ, as well as ERK1/2 in LβT2 cells. Lastly, unsaturated, but not saturated, FA inhibited GnRH-induced LH secretion in LβT2 cells as well as in pituitary cell cultures. Altogether, these results suggest that the pituitary is a relevant site of FA action and that UFA may influence reproduction by directly interfering with basal and GnRH-dependent gonadotrope activity.

Published

2011

41. Reporter transgenic mouse models highlight the dual endocrine and neural facet of GnRH receptor function.

Author

Schang AL, Counis R, Magre S, Bleux C, Granger A, Ngô-Muller V, Chenut MC, Ishaq M, Cohen-Tannoudji J, and Laverrière JN

Subjects

Animals, Mice, Mice, Transgenic, Models, Animal, Endocrine Glands physiology, Receptors, LHRH physiology

Abstract

In the pituitary of mammals, the GnRH receptor (GnRHR) plays crucial roles in the neuroendocrine control of reproductive function. This receptor is specifically expressed by the gonadotrope cells scattered among the five other endocrine cell types constituting the anterior pituitary; it is also expressed in other organs, such as the gonads and brain where its function is not well defined. To gain insight into GnRHR function, distribution, and regulation, several transgenic approaches have been developed using a range of reporter genes under the control of the mouse, rat, or ovine GnRHR gene (Gnrhr) promoters. Comprehensive reviews of the literature, together with recent results obtained in our laboratory, illustrate how these transgenic models highlight the endocrine as well as the neural facet of GnRHR function. In this review, the endocrine aspect will be discussed with regard to the pituitary and gonad function, whereas the neural aspect will be discussed with regard to hippocampal formation and the oculomotor pathway, the latter constituting an unpreviously described site of Gnrhr promoter activity. These approaches should help elucidate the properties of the mammalian GnRH system., (© 2011 New York Academy of Sciences.)

Published

2011

42. GnRH receptor gene expression in the developing rat hippocampus: transcriptional regulation and potential roles in neuronal plasticity.

Author

Schang AL, Ngô-Muller V, Bleux C, Granger A, Chenut MC, Loudes C, Magre S, Counis R, Cohen-Tannoudji J, and Laverrière JN

Subjects

Alkaline Phosphatase metabolism, Animals, Cells, Cultured, Early Growth Response Protein 1 genetics, Early Growth Response Protein 1 metabolism, Gene Expression Regulation, Developmental genetics, Gene Expression Regulation, Developmental physiology, Humans, Immunohistochemistry, Microfilament Proteins genetics, Microfilament Proteins metabolism, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Neuronal Plasticity genetics, Promoter Regions, Genetic genetics, Rats, Receptors, LHRH genetics, Reverse Transcriptase Polymerase Chain Reaction, Synaptophysin genetics, Synaptophysin metabolism, Hippocampus metabolism, Neuronal Plasticity physiology, Receptors, LHRH metabolism

Abstract

In the pituitary of mammals, the GnRH receptor (GnRHR) plays a primary role in the control of reproductive function. It is further expressed in the hippocampus, where its function, however, is not well defined. By quantitative RT-PCR analyses, we demonstrate herein that the onset of GnRHR gene (Gnrhr) expression in the rat hippocampus was unexpectedly delayed as compared to the pituitary and only occurred after birth. Using a previously described transgenic mouse model bearing the human placental alkaline phosphatase reporter gene under the control of the rat Gnrhr promoter, we established a positive correlation between the temporal pattern of Gnrhr mRNA levels and promoter activity in the hippocampal formation. The gradual appearance of human placental alkaline phosphatase transgene expression occurred simultaneously in the hippocampus and interconnected structures such as the lateral septum and the amygdala, coinciding with the establishment of hippocampo-septal projections. Analysis of transcription factors together with transient transfection assays in hippocampal neurons indicated that the combinatorial code governing the hippocampus-specific expression of the Gnrhr is distinct from the pituitary, likely involving transactivating factors such as NUR77, cyclic AMP response element binding protein, and Finkel-Biskis-Jinkins murine osteosarcoma virus oncogene homolog. A silencing transcription factor acting via the -3255/-1135 promoter region of the Gnrhr may be responsible for the transcriptional repression observed around birth. Finally, GnRH directly stimulated via activation of its receptor the expression of several marker genes of neuronal plasticity such as Egr1, synaptophysin, and spinophilin in hippocampal primary cultures, suggesting a role for GnRHR in neuronal plasticity. Further characterization of these mechanisms may help unravel important functions of GnRH/GnRHR signaling in the brain.

Published

2011

43. Sustained gonadotropin-releasing hormone stimulation mobilizes the cAMP/PKA pathway to induce nitric oxide synthase type 1 expression in rat pituitary cells in vitro and in vivo at proestrus.

Author

Garrel G, Simon V, Thieulant ML, Cayla X, Garcia A, Counis R, and Cohen-Tannoudji J

Subjects

Animals, Cell Culture Techniques, Cyclic AMP analysis, Cyclic AMP-Dependent Protein Kinases antagonists & inhibitors, Female, Gonadotropin-Releasing Hormone pharmacology, Nitric Oxide Synthase analysis, Nitric Oxide Synthase Type I, Nitric Oxide Synthase Type II analysis, Nitric Oxide Synthase Type II metabolism, Nitric Oxide Synthase Type III analysis, Nitric Oxide Synthase Type III metabolism, Proestrus drug effects, Rats, Rats, Wistar, Cyclic AMP metabolism, Cyclic AMP-Dependent Protein Kinases metabolism, Gonadotropin-Releasing Hormone metabolism, Nitric Oxide Synthase metabolism, Pituitary Gland enzymology, Proestrus metabolism

Abstract

Previous in vivo studies have established that pituitary nitric oxide synthase type 1 (NOS1) is regulated by gonadotropin-releasing hormone (GnRH). The aim of our study was to elucidate the mechanisms of NOS1 regulation by GnRH in rat pituitary cells. Using a perifused cell system, we demonstrated that NOS1 induction was sensitive to GnRH pulse frequency and was maximally induced under continuous GnRH stimulation. In primary cultures of rat pituitary cells, sustained stimulation with the GnRH agonist triptorelin (GnRHa) increased NOS1 protein levels, whereas NOS2 and NOS3 levels were unaffected. NOS1 up-regulation occurred in gonadotroph cells only, in a time-dependent and concentration-dependent manner (maximum increase, 2.5-fold; half-maximal concentration, 0.17 nM). GnRHa effect was mimicked by cAMP pathway activators and, most importantly, was blocked by disruption of the protein kinase A (PKA) pathway using pharmacological inhibitors such as Rp-cAMP or drug phosphatase technology-protein kinase inhibitor (DPT-PKI), a cell-permeant PKI peptide. In contrast, modulation of the PKC pathway and inhibition of the MAPK cascade were ineffective. Overall, these experiments demonstrated that GnRH-induced up-regulation of pituitary NOS1 is mediated notably by the cAMP/PKA pathway. Last, in vivo administration of a GnRH antagonist markedly inhibited the pituitary cAMP rise at proestrus in addition to suppressing NOS1 increase. Altogether, our data suggest that the cAMP/PKA signaling pathway is preferentially recruited under sustained GnRH stimulation in vivo during proestrus, allowing the expression of a specific set of PKA-regulated proteins, including NOS1, in gonadotroph cells.

Published

2010

44. The GnRH receptor and the response of gonadotrope cells to GnRH pulse frequency code. A story of an atypical adaptation of cell function relying on a lack of receptor homologous desensitization.

Author

Counis R, Garrel G, Laverriere JN, Simon V, Bleux C, Magre S, and Cohen-Tannoudji J

Subjects

Animals, Follicle Stimulating Hormone, Gene Expression Regulation, Gonadotropin-Releasing Hormone metabolism, Pituitary Gland metabolism, Luteinizing Hormone, Receptors, LHRH

Abstract

Brain control of the reproductive system is mediated through hypothalamic gonadotropin-releasing hormone (GnRH) which activates specific receptors (GnRHR) present at the surface of the pituitary gonadotropes to trigger secretion of the two gonadotropins LH and FSH. A unique feature of this system is the high dependence on the secretion mode of GnRH, which is basically pulsatile but undergoes considerable fluctuations in pulse frequency pattern in response to endogenous or external factors. How the physiological fluctuations of GnRH secretion that orchestrate normal reproduction are decoded by the gonadotrope cell machinery to ultimately control gonadotropin release and/or subunit gene transcription has been the subject of intensive studies during the past decades. Surprisingly, the mammalian GnRHR is unique among G protein-coupled receptor family as it lacks the carboxy-terminal tail usually involved in classical endocytotic process. Accordingly, it does not desensitize properly and internalizes very poorly. Both this atypical intrinsic property and post-receptor events may thus contribute to decode the GnRH signal. This includes the participation of a network of signaling pathways that differently respond to GnRH together with a growing amount of genes differentially sensitive to pulse frequency. Among these are two pairs of genes, the transcription factors EGR-1 and NAB, and the regulatory factors activin and follistatin, that function as intracellular autoregulatory feedback loops controlling respectively LHbeta and FSHbeta gene expression and hence, LH and FSH synthesis. Pituitary gonadotropes thus represent a unique model of cells functionally adapted to respond to a considerably fluctuating neuroendocrine stimulation, from short individual pulses to sustained GnRH as observed at the proestrus of ovarian cycle. Altogether, the data emphasize the adaptative reciprocal complementarity of hypothalamic GnRH neurones and pituitary gonadotropes to function as an original unit.

Published

2009

45. Gonadotropin-releasing hormone inhibits pituitary adenylyl cyclase-activating polypeptide coupling to 3',5'-cyclic adenosine-5'-monophosphate pathway in LbetaT2 gonadotrope cells through novel protein kinase C isoforms and phosphorylation of pituitary adenylyl cyclase-activating polypeptide type I receptor.

Author

Larivière S, Garrel-Lazayres G, Simon V, Shintani N, Baba A, Counis R, and Cohen-Tannoudji J

Subjects

Animals, Blotting, Western, Calcium metabolism, Cell Line, Gonadotrophs cytology, Gonadotrophs metabolism, Gonadotropin-Releasing Hormone agonists, Mice, Phosphorylation drug effects, Pituitary Adenylate Cyclase-Activating Polypeptide genetics, Protein Binding drug effects, Protein Isoforms genetics, Protein Isoforms metabolism, Receptors, Pituitary Adenylate Cyclase-Activating Polypeptide genetics, Reverse Transcriptase Polymerase Chain Reaction, Triptorelin Pamoate pharmacology, Cyclic AMP metabolism, Gonadotrophs drug effects, Gonadotropin-Releasing Hormone pharmacology, Pituitary Adenylate Cyclase-Activating Polypeptide metabolism, Protein Kinase C metabolism, Receptors, Pituitary Adenylate Cyclase-Activating Polypeptide metabolism

Abstract

Gonadotrope cells are primarily regulated by GnRH but are also targets of the pituitary adenylyl cyclase-activating polypeptide (PACAP). Although it has been reported that reciprocal interactions between both neuropeptides contribute to regulation of gonadotrope function, the underlying mechanisms remain poorly understood. In this study, we reevaluated PACAP coupling to the cAMP pathway in LbetaT2 gonadotrope cells and analyzed GnRH effect on PACAP signaling. We established that PACAP38 markedly increases intracellular cAMP levels (EC50 of 4.7 +/- 1.3 nm) through the PACAP type 1 receptor (PAC1-R), as evidenced by pharmacological and RT-PCR studies. Interestingly, although GnRH couples to cAMP pathway in LbetaT2 cells, the effects of both neuropeptides were not synergistic. Instead, the GnRH agonist (GnRHa) triptorelin rapidly and strongly inhibited (70% inhibition as early as 5 min) PACAP38-induced cAMP production. Inhibition was calcium independent, mimicked by the phorbol ester phorbol 12-myristate 13-acetate, and blocked by the protein kinase C (PKC) inhibitor bisindoylmaleimide, indicating that GnRHa inhibitory action relies on PKC. Selective down-regulation of both conventional and novel PKC prevented a GnRHa effect, whereas pharmacological inhibition of conventional PKC only was ineffective, strongly suggesting the involvement of novel PKC isoforms. GnRHa did not inhibit forskolin- or cholera toxin-stimulated cAMP accumulation, suggesting that PAC1-R is the predominant target of GnRH. Accordingly, we demonstrated for the first time that GnRH increases PAC1-R phosphorylation through PKC, providing a potential molecular mechanism which may account for GnRH inhibitory effect.

Published

2008

46. What is the role of PACAP in gonadotrope function?

Author

Counis R, Laverrière JN, Garrel-Lazayres G, Cohen-Tannoudji J, Larivière S, Bleux C, and Magre S

Subjects

Animals, Cyclic AMP metabolism, Female, Gonadotrophs cytology, Gonadotrophs metabolism, Gonadotropin-Releasing Hormone metabolism, Models, Biological, Pituitary Gland cytology, Pituitary Gland drug effects, Pituitary Gland metabolism, Rats, Signal Transduction drug effects, Gonadotrophs drug effects, Pituitary Adenylate Cyclase-Activating Polypeptide pharmacology

Abstract

Strong evidence in favor of a direct action of hypothalamic PACAP at the pituitary to modulate gonadotrope function has been acquired mainly by in vitro studies using cultured pituitary cells or gonadotrope cell lines. In particular, PACAP has been shown to cooperate with GnRH, the primary regulator of gonadotropes, to regulate/modulate gonadotropin subunit gene expression, gonadotropin release as well as gonadotrope responsiveness. These effects of PACAP appear to be due essentially to its high potent stimulatory action on the cAMP/protein kinase pathway. Ensuing mechanisms include signaling cross-talk and/or enhanced gene expression within gonadotropes. PACAP may also indirectly operate on these cells through paracrine mechanisms. While PACAP has long been viewed as a hypophysiotropic factor, a locally produced PACAP has also been described. Interestingly, both appear similarly up-regulated at proestrus of the reproductive cycle in female rats. Further in vivo investigation is now necessary to ascertain the physiological relevance of the observed pituitary PACAP effects and especially to evaluate the respective contribution of hypothalamic and pituitary PACAP in the dynamic control of gonadotrope function.

Published

2007

47. Gonadotropin-releasing hormone couples to 3',5'-cyclic adenosine-5'-monophosphate pathway through novel protein kinase Cdelta and -epsilon in LbetaT2 gonadotrope cells.

Author

Larivière S, Garrel G, Simon V, Soh JW, Laverrière JN, Counis R, and Cohen-Tannoudji J

Subjects

Adenylyl Cyclases metabolism, Animals, Calcium physiology, Cell Line, Gonadotropin-Releasing Hormone agonists, Isoenzymes physiology, Mice, Protein Kinase C-delta metabolism, Protein Kinase C-epsilon metabolism, Receptors, LHRH metabolism, Signal Transduction drug effects, Cyclic AMP metabolism, Gonadotrophs drug effects, Gonadotrophs metabolism, Gonadotropin-Releasing Hormone physiology, Protein Kinase C-delta physiology, Protein Kinase C-epsilon physiology

Abstract

GnRH regulates the reproductive system by stimulating synthesis and release of gonadotropins. GnRH acts through a receptor coupled to multiple intracellular events including a rapid phosphoinositide turnover. Although the cAMP pathway is essential for gonadotrope function, the ability of GnRH to induce cAMP, as well as the coupling mechanisms involved, remain controversial. In this study, we established that GnRH increases intracellular cAMP levels in a concentration-dependent manner in LbetaT2 gonadotrope cells (maximal increase, 2.5-fold; EC(50), 0.30 nm), and this was further evidenced by GnRH activation of a cAMP-sensitive reporter gene. The GnRH effect was Ca(2+) independent, mimicked by the phorbol ester phorbol 12-myristate 13-acetate, and blocked by the protein kinase C (PKC) inhibitor bisindolylmaleimide, indicating that the GnRH effect was mediated by PKC. Pharmacological inhibition of conventional PKC isoforms with Gö6976 did not prevent GnRH-induced cAMP production, whereas down-regulation of novel PKCdelta, -epsilon, and -theta by a long-term treatment with GnRH markedly reduced it. Expression of dominant-negative (DN) mutants of PKCdelta or -epsilon but not PKCtheta impaired GnRH activation of a cAMP-sensitive promoter, demonstrating that PKCdelta and -epsilon are the two endogenous isoforms mediating GnRH activation of the adenylyl cyclase (AC) pathway in LbetaT2 cells. Accordingly, we identified by RT-PCR and immunocytochemical analysis, two PKC-sensitive AC isoforms, i.e. AC5 and AC7 as potential targets for GnRH. Lastly, we showed that only sustained stimulation of GnRH receptor significantly increased cAMP, suggesting that in vivo, the cAMP signaling pathway may be selectively recruited under intense GnRH release such as the preovulatory GnRH surge.

Published

2007

48. The LIM-homeodomain proteins Isl-1 and Lhx3 act with steroidogenic factor 1 to enhance gonadotrope-specific activity of the gonadotropin-releasing hormone receptor gene promoter.

Author

Granger A, Bleux C, Kottler ML, Rhodes SJ, Counis R, and Laverrière JN

Subjects

Animals, Base Sequence, Cell Line, Cricetinae, DNA genetics, DNA metabolism, Homeodomain Proteins genetics, Humans, Mice, Organ Specificity, Protein Binding, Rats, Receptors, Cytoplasmic and Nuclear genetics, Response Elements genetics, Steroidogenic Factor 1, Transcription Factors genetics, Transcriptional Activation, Gene Expression Regulation, Homeodomain Proteins metabolism, Pituitary Gland metabolism, Promoter Regions, Genetic genetics, Receptors, Cytoplasmic and Nuclear metabolism, Receptors, LHRH genetics, Transcription Factors metabolism

Abstract

The GnRH receptor (GnRH-R) plays a central role in mammalian reproductive function throughout adulthood. It also appears as an early marker gene of the presumptive gonadotrope lineage in developing pituitary. Here, using transient transfections combined with DNA/protein interaction assays, we have delineated cis-acting elements within the rat GnRH-R gene promoter that represent targets for the LIM-homeodomain (LIM-HD) proteins, Isl-1 and Lhx3. These factors, critical in early pituitary development, are thus also crucial for gonadotrope-specific expression of the GnRH-R gene. In heterologous cells, the expression of Isl-1 and Lhx3, together with steroidogenic factor 1 (SF-1), culminates in the activation of both the rat as well as human GnRH-R promoter, suggesting that this combination is evolutionarily conserved among mammals. The specificity of these LIM-HD factors is attested by the inefficiency of related proteins, including Lhx5 and Lhx9, to activate the GnRH-R gene promoter, as well as by the repressive capacity of a dominant-negative derivative of Lhx3. Accordingly, targeted deletion of the LIM response element decreases promoter activity. In addition, experiments with Gal4-SF-1 fusion proteins suggest that LIM-HD protein activity in gonadotrope cells is dependent upon SF-1 binding. Finally, using a transgenic model that allows monitoring of in vivo promoter activity, we show that the overlapping expression of Isl-1 and Lhx3 in the developing pituitary correlates with promoter activity. Collectively, these data suggest the occurrence of a specific LIM-HD pituitary code and designate the GnRH-R gene as the first identified transcriptional target of Isl-1 in the anterior pituitary.

Published

2006

49. Differential mechanisms for PACAP and GnRH cAMP induction contribute to cross-talk between both hormones in the gonadotrope LbetaT2 cell line.

Author

Larivière S, Garrel G, Robin MT, Counis R, and Cohen-Tannoudji J

Subjects

Animals, Cell Line, Female, Mice, Cyclic AMP biosynthesis, Gonadotropin-Releasing Hormone pharmacology, Granulosa Cells drug effects, Granulosa Cells metabolism, Pituitary Adenylate Cyclase-Activating Polypeptide pharmacology

Abstract

The effects and respective influence of pituitary adenylate cyclase-activating polypeptide (PACAP) and gonadotropin-releasing hormone (GnRH) on cyclic AMP (cAMP) production in pituitary gonadotropes were analyzed using the LbetaT2 cell line. Both hormones induced cAMP with, however, different intensity and time course. In addition, the GnRH effect was markedly reduced by PKC inhibitors. Despite its positive coupling to cAMP pathway, GnRH counteracted PACAP induction of cAMP and this effect was mimicked by the PKC activator phorbol 12-myristate 13-acetate (PMA). The data reveal major differences in the mechanisms by which PACAP and GnRH activate cAMP/PKA pathway in LbetaT2 cells and suggest that PKC activation serves GnRH not only to increase cAMP but also to counteract the PACAP stimulation of this signaling pathway.

Published

2006

50. Molecular mechanisms of insulin-like growth factor-I mediated regulation of the steroidogenic acute regulatory protein in mouse leydig cells.

Author

Manna PR, Chandrala SP, King SR, Jo Y, Counis R, Huhtaniemi IT, and Stocco DM

Subjects

3-Hydroxysteroid Dehydrogenases metabolism, Animals, Bucladesine pharmacology, Cells, Cultured, Cyclic AMP metabolism, Cyclic AMP Response Element-Binding Protein metabolism, Cyclic AMP-Dependent Protein Kinases pharmacology, Gene Expression Regulation, Insulin physiology, Male, Mice, Mitogen-Activated Protein Kinase 1 antagonists & inhibitors, Mitogen-Activated Protein Kinase 1 physiology, Mitogen-Activated Protein Kinase 3 antagonists & inhibitors, Mitogen-Activated Protein Kinase 3 physiology, Phosphorylation, Protein Kinase C pharmacology, Proto-Oncogene Proteins c-jun metabolism, Transcription, Genetic, Insulin-Like Growth Factor I physiology, Leydig Cells metabolism, Phosphoproteins genetics, Phosphoproteins metabolism, Steroids biosynthesis, Transcriptional Activation

Abstract

Growth factors are known to play diverse roles in steroidogenesis, a process regulated by the mitochondrial steroidogenic acute regulatory (StAR) protein. The mechanism of action of one such growth factor, IGF-I, was investigated in mouse Leydig tumor (mLTC-1) cells to determine its potential role in the regulation of StAR expression. mLTC-1 cells treated with IGF-I demonstrated temporal and concentration-dependent increases in StAR expression and steroid synthesis. However, IGF-I had no effect on cytochrome P450 side-chain cleavage or 3beta-hydroxysteroid dehydrogenase protein levels. IGF-I was capable of augmenting N,O'-dibutyrl-cAMP-stimulated steroidogenic responsiveness in these cells. The steroidogenic potential of IGF-I was also confirmed in primary cultures of isolated mouse Leydig cells. IGF-I increased phosphorylation of ERK1/2, an event inhibited by the MAPK/ERK inhibitors, PD98059 and U0126. Interestingly, inhibition of ERK activity enhanced IGF-I-mediated StAR protein expression, but phosphorylation of StAR was undetectable, an observation in contrast to that seen with N,O'-dibutyrl-cAMP signaling. Further studies demonstrated that these events were tightly correlated with the expression of dosage-sensitive sex reversal, adrenal hypoplasia congenita, critical region on the X chromosome, gene 1 and scavenger receptor class B type 1. Whereas both protein kinase A and protein kinase C signaling were involved in the IGF-I-mediated steroidogenic response, the majority of the effects of IGF-I were found to be mediated by the protein kinase C pathway. Transcriptional activation of the StAR gene by IGF-I was influenced by several transcription factors, its up-regulation being dependent on phosphorylation of the cAMP response element-binding protein (CREB) and the activator protein 1 family member, c-Jun. Conversely, StAR gene transcription was markedly inhibited by expression of nonphosphorylatable CREB (Ser(133)Ala), dominant negative A-CREB, and dominant negative c-Jun (TAM-67) mutants. Collectively, the present studies identify molecular events in IGF-I signaling that may influence testicular growth, development, and the Leydig cell steroidogenic machinery through autocrine/paracrine regulation.

Published

2006