Your search keyword '"Moncharmont B"' showing total 45 results

1. Interaction of Two Nonhistone Proteins with the Estradiol Response Element of the Avian Vitellogenin Gene Modulates the Binding of Estradiol-Receptor Complex

Author

Feavers, I. M., Jiricny, J., Moncharmont, B., Saluz, H. P., and Jost, J. P.

Published

1987

2. Formation and Identification of Cytoskeletal Components from Liver Cytosolic Precursors

Author

Sahyoun, N., Stenbuck, P., LeVine, H., Bronson, D., Moncharmont, B., Henderson, C., and Cuatrecasas, P.

Published

1982

3. «Après moi le déluge.» Strategie per la continuità nella gestione di un corso di laurea magistrale in Medicina

Author

Gallo, P, Barajon, I, Bellini, T, Familiari, G, Franzoni, L, Lui, F, Moncharmont, B, Perroteau, I, Riggio, O, Strepparava, M, Valli, M, Linda Vignozzi, E, Pietro Gallo, Isabella Barajon, Tiziana Bellini, Giuseppe Familiari, Lorella Franzoni, Fausta Lui, Bruno Moncharmont, Isabelle Perroteau, Oliviero Riggio, Maria Grazia Strepparava, Maurizia Valli, e Linda Vignozzi, Gallo, P, Barajon, I, Bellini, T, Familiari, G, Franzoni, L, Lui, F, Moncharmont, B, Perroteau, I, Riggio, O, Strepparava, M, Valli, M, Linda Vignozzi, E, Pietro Gallo, Isabella Barajon, Tiziana Bellini, Giuseppe Familiari, Lorella Franzoni, Fausta Lui, Bruno Moncharmont, Isabelle Perroteau, Oliviero Riggio, Maria Grazia Strepparava, Maurizia Valli, and e Linda Vignozzi

Abstract

The famous sentence “Après moi le déluge” (“After me the flood”), attributed to Louis XV, king of France, makes reference to the perception that one’s own successor is not going to be suitable to the task. The situation seems to apply to plenty of the Italian Presidents of the Undergraduate Curriculum in Medicine, who continually succeed one another, with the new President too often bound to restart from the beginning. The most obvious solution to this problem is to institutionalize the handover process. However, the presence of collegiate bodies, helping the President to manage the Curriculum, is another important tool to ensure continuity between the succeeding Presidents. Technical Committee for Planning teaching and education (TCP) was created in 2000 by the Permanent Conference of Presidents of the Undergraduate Curricula in Medicine and every Italian Undergraduate Curriculum should have such a structure. However, the functions attributed to TCP are changing because of the new tasks the President is nowadays facing, from faculty development, to the quality assurance, to the needs to second the paradigm shift from a teacher-based teaching to a student-centred learning. As a consequence, TCP requirements are changing and it is time to give birth to a 2.0 TCP to help Presidents to face nowadays challenges.

Published

2019

4. Analisi delle cause del ritardo studentesco nel CLM in Medicina

Author

Gallo, P, Bani, M, Bellini, T, Casacchia, M, della Rocca, C, Familiari, G, Mazzeo, A, Merli, M, Moncharmont, B, Montagna, L, Muraro, R, Riggio, O, Rosso, U, Strepparava, MG, Valli, M, Viola, F, Gallo, P, Bani, M, Bellini, T, Casacchia, M, della Rocca, C, Familiari, G, Mazzeo, A, Merli, M, Moncharmont, B, Montagna, L, Muraro, R, Riggio, O, Rosso, U, Strepparava, M, Valli, M, and Viola, F

Subjects

Medical Education, Tutoring, Counselling, Graduation Delay, M-PSI/08 - PSICOLOGIA CLINICA

Abstract

Although the number of inactive students is rather high in Italian University (35%), the figures are distinctively lower for medical students (14% of inactive students and 3-5% of renouncing). A recent survey among medical students at La Sapienza University of Rome has singled out the following as the main causes of graduation delay: difficulties in studying (43%); delayed matriculation (due to controversies in the application competition) (16%); psychological upset (13%); family (6%) or health (3%) problems; and economical difficulties (3%). The causes of graduation delay have been debated by the National Conference of the Undergraduate Curricula Presidents in a Forum held in Novara. Four types of causes and solutions have been discussed: i) teaching causes and active tutoring; ii) psychological upset and counselling; iii) social, cultural and economic hardships and counter window interventions; and iv) disproportion between didactic load and learning capabilities, and educational interventions. In conclusion, the need for monitoring student upset and for reducing disciplinary Learning objects (subject to quick obsolescence) in favour of methodological ones (that favour a lifelong learning) has been assessed.

Published

2017

5. Syllabus pedagogico. Esperienze di lavoro di gruppo

Author

Consorti, F, Familiari, G, Moncharmont, B, STREPPARAVA, MARIA GRAZIA, Consorti, F, Familiari, G, Moncharmont, B, and Strepparava, M

Subjects

small group activities - integrated course - interprofessional collaboration, M-PED/01 - PEDAGOGIA GENERALE E SOCIALE, lavoro a piccoli gruppi , corsi integrati , collaborazione interprofessionale, M-PSI/08 - PSICOLOGIA CLINICA, M-PSI/06 - PSICOLOGIA DEL LAVORO E DELLE ORGANIZZAZIONI

Abstract

This Forum is a part of the tetralogy of educational events devoted to “Training of teachers, supervisors and students to leadership and teamwork”. In a tetralogy the so called “Pedagogical pills” are mini-lectures, the workshops are based on experiential learning, forums are the privileged environment in which the Conference co-constructs its shared knowledge, since they are small group activities focused on sharing and discussion of real life experience. In this forum we identified some critical situations in which teamwork asks for a special attention, specially when the team is inter-professional. The following articles report on the most significant and common elements emerged from the discussion. The considered environments were the team of teachers of an integrated course, the relationship between teachers and administrative- technical personnel dn the inter-professional collaboration, probably the most challenging context in the near future.

Published

2016

6. Nuovi strumenti didattici. “Insegnamolo Strano” Atelier

Author

Strepparava, M, Barajon, I, Basili, S, Consorti, F, della Rocca, C, Familiari, G, Gallo, P, Lui, F, Merli, M, Moncharmont, B, Vignozzi, L, Maria Grazia Strepparava, Isabella Barajon, Stefania Basili, Fabrizio Consorti, Carlo della Rocca, Giuseppe Familiari, Pietro Gallo, Fausta Lui, Manuela Merli, Bruno Moncharmont, Linda Vignozzi, Strepparava, M, Barajon, I, Basili, S, Consorti, F, della Rocca, C, Familiari, G, Gallo, P, Lui, F, Merli, M, Moncharmont, B, Vignozzi, L, Maria Grazia Strepparava, Isabella Barajon, Stefania Basili, Fabrizio Consorti, Carlo della Rocca, Giuseppe Familiari, Pietro Gallo, Fausta Lui, Manuela Merli, Bruno Moncharmont, and Linda Vignozzi

Abstract

The article describes the ideas discussed during the labs organized by the Educational Team at the 131 CPPCLMMC Conference. The educational issues discussed during the three ateliers were: flipped classroom, video use in medical education and medical humanities. These three areas can be seen as prototypical examples of students centred teaching strategies. As result of the groups activities, the positive role of active and cooperative learning, the relevance of the faculty for identify the educational goals and related didactic strategies, the role of medical humanities in fostering a patient-centred doctor, was pointed out.

Published

2018

7. Strategie per far fronte al ritardo studentesco nel CLM in Medicina

Author

Gallo, P, Barajon, I, della Rocca, C, Mazzeo, A, Merli, M, Moncharmont, B, Strepparava, M, Pietro Gallo, Isabella Barajon, Carlo della Rocca, Adolfo Mazzeo, Manuela Merli, Bruno Moncharmont, Maria Grazia Strepparava, Gallo, P, Barajon, I, della Rocca, C, Mazzeo, A, Merli, M, Moncharmont, B, Strepparava, M, Pietro Gallo, Isabella Barajon, Carlo della Rocca, Adolfo Mazzeo, Manuela Merli, Bruno Moncharmont, and Maria Grazia Strepparava

Abstract

The Presidents of the Italian Undergraduate Curricula in Medicine have faced the problem of remediation in a workshop held in Udine on the 22nd September 2017. Presidents have been subdivided into small groups, have been given detailed data about a hypothetic undergraduate curriculum and have been asked to devise remediation strategies adequate to the case study proposed. Data included general information about the School of Medicine, its structure and scientific excellences, and amount and composition of teaching staff. Information has been given also on the region where the School is placed, its population and social-economical parameters, and on the number and origin of medical students. Entity of students’ graduation delay has been detailed. Undergraduate curriculum has been illustrated giving detailed information about the examinations: their number, weight in credits, deployment through the curriculum, and number of students passing them in due time, with minimum, maximum and average score. Rules for students entry blocks for the following year and information about the consistency of tutoringcounselling services and of teachers continuous education strategies have been finally given. The Presidents of Undergraduate Curricula in Medicine have reached the conclusions that they should obtain the necessary detailed information about entity and causes of their students’ graduation delay. Remediation strategies should include active and peer-to-peer tutoring and forms of flexibility in assessment design and curriculum re-modelling.

Published

2017

8. Il ruolo organizzativo e pedagogico del Presidente di Corso di Laurea Magistrale in Medicina

Author

Gallo, Pietro, Basili, Stefania, Caiaffa, Mf, Consorti, Fabrizio, DELLA ROCCA, Carlo, Demelia, L, Familiari, Giuseppe, Furlan, Pm, Moncharmont, B, Montagna, L, Scarone, S, and Valanzano, R.

Published

2013

9. In vitro secondary activation (memory effect) of avian vitellogenin II gene in isolated liver nuclei.

Author

Jost, J P, Moncharmont, B, Jiricny, J, Saluz, H, and Hertner, T

Abstract

The vitellogenin II gene is specifically reactivated in vitro (secondary stimulation, memory effect) in purified liver nuclei that had ceased to express the gene in vivo a month after the roosters had received a single injection of estradiol (primary stimulation). The in vitro reactivation depends on the addition to the nuclei of nuclear and cytoplasmic extracts from estradiol-stimulated livers, polyamines (0.1-1.0 mM), and calmodulin (0.1 mM). Under identical incubation conditions the vitellogenin gene could not be reactivated in oviduct, embryonic, and immature chicken liver nuclei. Two other genes, those for ovalbumin and lysozyme, which are regulated by estradiol in the oviduct, could not be activated in the liver nuclei. The correct initiation of vitellogenin gene transcription in the liver nuclei was tested by primer extension studies. Addition of the antiestrogen tamoxifen (0.1 microM) to the system decreased vitellogenin mRNA synthesis by about 45% without affecting total RNA synthesis. Addition of quercetin (0.1 mM) and trans-flupenthixol (0.2 mM), inhibitors of nuclear protein kinase II and calmodulin-dependent kinase, respectively, inhibited the synthesis of vitellogenin mRNA by about 55% without affecting total RNA synthesis. The inhibitory effects of the antiestrogen and the kinase inhibitors were not additive, suggesting that both classes of inhibitor act on the same target or related targets. Depleting the estradiol receptors from the cell and nuclear extracts by means of estradiol-receptor antibodies covalently bound to Matrex beads reduced the stimulation of the vitellogenin gene by 40%. We conclude that in addition to the estradiol receptor and phosphorylation of nuclear protein(s) there are additional factors responsible for the in vitro secondary activation of the avian vitellogenin II gene.

Published

1986

10. Subunit composition of the molybdate-stabilized “8-9 S” nontransformed estradiol receptor purified from calf uterus.

Author

Redeuilh, G, Moncharmont, B, Secco, C, and Baulieu, E E

Abstract

The structure of the calf uterus nontransformed molybdate-stabilized estradiol receptor (ER) has been investigated using affinity labeling with tamoxifen aziridine and several monoclonal antibodies directed either against the steroid binding protein (Mr approximately 65,000) or against the heat shock protein of Mr approximately 90,000 (hsp 90). The purification was performed using affinity chromatography and a DEAE-Sephacel column. The [3H] estradiol-ER complex was obtained as a well-defined radioactive peak, the specific activity varying between 1,600 and 3,400 pmol/mg of protein. The purified ER sediments in glycerol gradients at 9.4 S +/- 0.2 (n = 5) and at 8.1 S +/- 0.2 (n = 15) in a 0.15 M KCl containing gradient (“8-9 S” ER). From a measured Stokes radius of 7.4 +/- 0.2 nm (n = 12), an Mr of approximately 300,000 has been calculated. Studies of the purified 8-9 S ER by glycerol gradient centrifugation and by “twin antibody” assay with the JS34/32 anti-ER monoclonal antibody suggest the presence of two binding subunits in the nontransformed molecular complex. Results of immunological analysis with polyclonal and several monoclonal antibodies against hsp 90 suggest the association of two molecules of this protein to the two steroid binding subunits. In high salt medium (0.4 M KCl), the purified ER sediments at 5.2 +/- 0.3 (n = 8), has a Stokes radius of 5.7 nm +/- 0.1 (n = 2) and the Mr is approximately 129,000, values expected for a homodimer consisting of two hormone-binding subunits (Mr approximately 65,000), a result confirmed by glycerol gradient centrifugation experiments, using the monoclonal antibody JS34/32. The relationship between the nontransformed 8-9 S ER and the transformed 5 S-ER forms are discussed, the simplest possibility being the release of the already formed homodimeric ER from 8-9 S ER during transformation.

Published

1987

11. Proteolytic activity of the purified hormone-binding subunit in the estrogen receptor.

Author

Molinari, A M, Abbondanza, C, Armetta, I, Medici, N, Minucci, S, Moncharmont, B, Nigro, V, and Puca, G A

Abstract

The hormone-binding subunit of the calf uterus estradiol receptor was purified as a hormone-free molecule. Immunoaffinity chromatography with a specific monoclonal antibody was used as the final step. The purified subunit was specifically labeled by radioactive diisopropyl fluorophosphate. The diisopropyl fluorophosphate-labeled amino acid was serine. The purified receptor was able to release the fluorogenic or chromogenic group from synthetic peptides containing phenylalanine at the carboxyl terminus. This occurred only in the presence of estradiol and was hampered by aprotinin and diisopropyl fluorophosphate. Estradiol-dependent hydrolytic activity was also found in the eluate from gel slices after SDS/PAGE of purified receptor. This activity comigrated with the renaturable estradiol-binding activity. The estradiol antagonists 4-hydroxytamoxifen and ICI 164,384 as well as other steroid hormones were unable to activate this hydrolytic activity.

Published

1991

12. Estradiol receptor of calf uterus: interactions with heparin-agarose and purification.

Author

Molinari, A M, Medici, N, Moncharmont, B, and Puca, G A

Abstract

Heparin attached covalently to agarose beads binds the "native" form of the estradiol receptor with very high affinity. Chondroitin sulfate does not bind to the receptor. When the receptor is complexed with hormone, the affinity is at least 10 times higher. Only the "native" and not the "nuclear" or the "derived" (i.e., after activation by a calcium-dependent enzyme) forms of the estradiol receptor interact with heparin. The "native" estradiol-receptor complex is purified to homogeneity after chromatography on columns of heparin-agarose, Sephadex G-200, and DEAE-cellulose, followed by two more Sephadex G-200 columns. The purified molecule is a single polypeptide of molecular weight 69,000 by polyacrylamide gel electrophoresis in sodium dodecyl sulphate. The sedimentation coefficient on sucrose gradients is 4.3 S, the Stokes radius from gel filtration is 36.5 A, and the isoelectric point is 6.4. The purified [3H]estradiol-receptor complex exchanges the radioactive hormone with estradiol or other estrogenic steroids, but not with testosterone, 5alpha-dihydrotestosterone, or progesterone.

Published

1977

13. Dual-specificity phosphatase (DUSP6) in human glioblastoma: epithelial-to-mesenchymal transition (EMT) involvement

Author

Erika Di Zazzo, Bruno Moncharmont, Candida Zuchegna, Samantha Messina, Zuchegna, Candida, Di Zazzo, Erika, Moncharmont, Bruno, Messina, Samantha, Zuchegna, C., Di Zazzo, E., Moncharmont, B., and Messina, S.

Subjects

Adult, 0301 basic medicine, Epithelial-Mesenchymal Transition, Epithelial-to-mesenchymal transition (EMT), lcsh:Medicine, DUSP6, Vimentin, medicine.disease_cause, General Biochemistry, Genetics and Molecular Biology, Brain Neoplasm, Dual-specificity phosphatase (DUSP6), 03 medical and health sciences, 0302 clinical medicine, Dual Specificity Phosphatase 6, Cell Line, Tumor, Dual-specificity phosphatase, medicine, Humans, 030212 general & internal medicine, Epithelial–mesenchymal transition, lcsh:Science (General), Dual-Specificity Phosphatase, lcsh:QH301-705.5, Cisplatin, biology, Brain Neoplasms, lcsh:R, Mesenchymal stem cell, General Medicine, nervous system diseases, Fibronectin, Research Note, 030104 developmental biology, lcsh:Biology (General), biology.protein, Cancer research, Dual-Specificity Phosphatases, Glioblastoma, Carcinogenesis, Human, lcsh:Q1-390, medicine.drug

Abstract

Objective Glioblastoma (GBM) is the most aggressive and common form of primary brain cancer. Survival is poor and improved treatment options are urgently needed. Dual specificity phosphatase-6 (DUSP6) is actively involved in oncogenesis showing unexpected tumor-promoting properties in human glioblastoma, contributing to the development and expression of the full malignant and invasive phenotype. The purpose of this study was to assess if DUSP6 activates epithelial-to-mesenchymal transition (EMT) in glioblastoma and its connection with the invasive capacity. Results We found high levels of transcripts mRNA by qPCR analysis in a panel of primary GBM compared to adult or fetal normal tissues. At translational levels, these data correlate with high protein expression and long half-life values by cycloheximide-chase assay in immunoblot experiments. Next, we demonstrate that DUSP6 gene is involved in epithelial-to-mesenchymal transition (EMT) in GBM by immunoblot characterization of the mesenchymal and epithelial markers. Vimentin, N-Cadherin, E-Cadherin and fibronectin were measured with and without DUSP6 over-expression, and in response to several stimuli such as chemotherapy treatment. In particular, the high levels of vimentin were blunted at increasing doses of cisplatin in condition of DUSP6 over-expression while N-Cadherin contextually increased. Finally, DUSP6 per se increased invasion capacity of GBM. Overall, our data unveil the DUSP6 involvement in invasive mesenchymal-like properties in GBM.

Published

2020

14. Multifaceted role of PRDM proteins in human cancer

Author

Erika Di Zazzo, Ciro Abbondanza, Maria Proto, Amelia Casamassimi, Bruno Moncharmont, Anna Sorrentino, Monica Rienzo, Donatella Fiore, Maurizio Bifulco, Patrizia Gazzerro, Casamassimi, A., Rienzo, M., Di Zazzo, E., Sorrentino, A., Fiore, D., Proto, M. C., Moncharmont, B., Gazzerro, P., Bifulco, M., Abbondanza, C., and Sorrentino, Anna.

Subjects

Review, Prognosis and therapy, lcsh:Chemistry, Neoplasms, Gene expression, Human malignancie, lcsh:QH301-705.5, Protein Interaction Domains and Motif, Spectroscopy, Nuclear Protein, Zinc finger, Nuclear Proteins, General Medicine, Prognosis, Computer Science Applications, Cell biology, The cancer genome atlas, DNA-Binding Proteins, Gene Expression Regulation, Neoplastic, Genetic alteration, Multigene Family, Histone methyltransferase, Disease Susceptibility, The cancer genome atla, Human, Protein Binding, Signal Transduction, Prognosi, DNA-Binding Protein, Human malignancies, Biology, Catalysis, Inorganic Chemistry, Genetic alterations, PRD-BF1 and RIZ homology domain containing gene family, medicine, Animals, Humans, Protein Interaction Domains and Motifs, Epigenetics, Physical and Theoretical Chemistry, Molecular Biology, Gene, Animal, Organic Chemistry, Alternative splicing, Cancer, Promoter, Histone-Lysine N-Methyltransferase, medicine.disease, lcsh:Biology (General), lcsh:QD1-999, Neoplasm, Positive Regulatory Domain I-Binding Factor 1, Transcription Factors

Abstract

The PR/SET domain family (PRDM) comprise a family of genes whose protein products share a conserved N-terminal PR [PRDI-BF1 (positive regulatory domain I-binding factor 1) and RIZ1 (retinoblastoma protein-interacting zinc finger gene 1)] homologous domain structurally and functionally similar to the catalytic SET [Su(var)3-9, enhancer-of-zeste and trithorax] domain of histone methyltransferases (HMTs). These genes are involved in epigenetic regulation of gene expression through their intrinsic HMTase activity or via interactions with other chromatin modifying enzymes. In this way they control a broad spectrum of biological processes, including proliferation and differentiation control, cell cycle progression, and maintenance of immune cell homeostasis. In cancer, tumor-specific dysfunctions of PRDM genes alter their expression by genetic and/or epigenetic modifications. A common characteristic of most PRDM genes is to encode for two main molecular variants with or without the PR domain. They are generated by either alternative splicing or alternative use of different promoters and play opposite roles, particularly in cancer where their imbalance can be often observed. In this scenario, PRDM proteins are involved in cancer onset, invasion, and metastasis and their altered expression is related to poor prognosis and clinical outcome. These functions strongly suggest their potential use in cancer management as diagnostic or prognostic tools and as new targets of therapeutic intervention.

Published

2020

15. «Après moi le déluge.» Strategie per la continuità nella gestione di un corso di laurea magistrale in Medicina

Author

Pietro Gallo, Isabella Barajon, Tiziana Bellini, Giuseppe Familiari, Lorella Franzoni, Fausta Lui, Bruno Moncharmont, Isabelle Perroteau, Oliviero Riggio, Maria Grazia Strepparava, Maurizia Valli, e Linda Vignozzi, Gallo, P, Barajon, I, Bellini, T, Familiari, G, Franzoni, L, Lui, F, Moncharmont, B, Perroteau, I, Riggio, O, Strepparava, M, Valli, M, and Linda Vignozzi, E

Subjects

Management Continuity, Organi Collegiali per il Corso di laurea, Medical Education, M-PED/03 - DIDATTICA E PEDAGOGIA SPECIALE, Collegiate Bodies for the Undergraduate Curriculum, MED/04 - PATOLOGIA GENERALE, M-PSI/08 - PSICOLOGIA CLINICA, Pedagogia Medica, Continuità di Gestione

Abstract

The famous sentence “Après moi le déluge” (“After me the flood”), attributed to Louis XV, king of France, makes reference to the perception that one’s own successor is not going to be suitable to the task. The situation seems to apply to plenty of the Italian Presidents of the Undergraduate Curriculum in Medicine, who continually succeed one another, with the new President too often bound to restart from the beginning. The most obvious solution to this problem is to institutionalize the handover process. However, the presence of collegiate bodies, helping the President to manage the Curriculum, is another important tool to ensure continuity between the succeeding Presidents. Technical Committee for Planning teaching and education (TCP) was created in 2000 by the Permanent Conference of Presidents of the Undergraduate Curricula in Medicine and every Italian Undergraduate Curriculum should have such a structure. However, the functions attributed to TCP are changing because of the new tasks the President is nowadays facing, from faculty development, to the quality assurance, to the needs to second the paradigm shift from a teacher-based teaching to a student-centred learning. As a consequence, TCP requirements are changing and it is time to give birth to a 2.0 TCP to help Presidents to face nowadays challenges.

Published

2019

16. Nuovi strumenti didattici. 'Insegnamolo Strano' Atelier

Author

Maria Grazia Strepparava, Isabella Barajon, Stefania Basili, Fabrizio Consorti, Carlo della Rocca, Giuseppe Familiari, Pietro Gallo, Fausta Lui, Manuela Merli, Bruno Moncharmont, Linda Vignozzi, Strepparava, M, Barajon, I, Basili, S, Consorti, F, della Rocca, C, Familiari, G, Gallo, P, Lui, F, Merli, M, Moncharmont, B, and Vignozzi, L

Subjects

M-PED/03 - DIDATTICA E PEDAGOGIA SPECIALE, FLIPPED CLASSROOM, VIDEO TECHNOLOGY ENHANCED LEARNING, MEDICAL HUMANITIES, ACTIVE LEARNING, M-PSI/08 - PSICOLOGIA CLINICA

Abstract

The article describes the ideas discussed during the labs organized by the Educational Team at the 131 CPPCLMMC Conference. The educational issues discussed during the three ateliers were: flipped classroom, video use in medical education and medical humanities. These three areas can be seen as prototypical examples of students centred teaching strategies. As result of the groups activities, the positive role of active and cooperative learning, the relevance of the faculty for identify the educational goals and related didactic strategies, the role of medical humanities in fostering a patient-centred doctor, was pointed out.

Published

2018

17. Prostate cancer stem cells: the role of androgen and estrogen receptors

Author

Antonio Agostino Sinisi, Giovanni Galasso, Erika Di Zazzo, Annalisa Di Santi, Gabriella Castoria, Ciro Abbondanza, Pia Giovannelli, Bruno Moncharmont, Gustavo Cernera, Antimo Migliaccio, Valentina Rossi, Marzia Di Donato, Zazzo, Erika Di, Galasso, Giovanni, Giovannelli, Pia, Donato, Marzia Di, Santi, Annalisa Di, Cernera, Gustavo, Rossi, Valentina, Abbondanza, Ciro, Moncharmont, Bruno, Sinisi, Antonio Agostino, Castoria, Gabriella, Migliaccio, Antimo, Di Zazzo, E., Galasso, G., Giovannelli, P., Di Donato, M., Di Santi, A., Cernera, G., Rossi, V., Abbondanza, C., Moncharmont, B., Sinisi, A. A., Castoria, G., and Migliaccio, A.

Subjects

Male, 0301 basic medicine, GPR30, medicine.medical_specialty, GPR30, stem cells, medicine.drug_class, Estrogen receptor, Review, Receptors, G-Protein-Coupled, estradiol receptors, Androgen deprivation therapy, 03 medical and health sciences, Prostate cancer, estradiol receptor, 0302 clinical medicine, stem cells, androgen receptor, Internal medicine, medicine, Humans, Androgen Receptor Antagonists, Models, Genetic, business.industry, Prostatic Neoplasms, prostate cancer, medicine.disease, Androgen, Gene Expression Regulation, Neoplastic, Androgen receptor, Estradiol receptors, Stem cells, 030104 developmental biology, Endocrinology, Receptors, Estrogen, Oncology, Receptors, Androgen, 030220 oncology & carcinogenesis, Androgens, Neoplastic Stem Cells, Cancer research, Stem cell, business, GPER

Abstract

Prostate cancer is one of the most commonly diagnosed cancers in men, and androgen deprivation therapy still represents the primary treatment for prostate cancer patients. This approach, however, frequently fails and patients develop castration-resistant prostate cancer, which is almost untreatable. Cancer cells are characterized by a hierarchical organization, and stem/progenitor cells are endowed with tumor-initiating activity. Accumulating evidence indicates that prostate cancer stem cells lack the androgen receptor and are, indeed, resistant to androgen deprivation therapy. In contrast, these cells express classical (α and/or ß) and novel (GPR30) estrogen receptors, which may represent new putative targets in prostate cancer treatment. In the present review, we discuss the still-debated mechanisms, both genomic and non-genomic, by which androgen and estradiol receptors (classical and novel) mediate the hormonal control of prostate cell stemness, transformation, and the continued growth of prostate cancer. Recent preclinical and clinical findings obtained using new androgen receptor antagonists, anti-estrogens, or compounds such as enhancers of androgen receptor degradation and peptides inhibiting non-genomic androgen functions are also presented. These new drugs will likely lead to significant advances in prostate cancer therapy.

Published

2015

18. Strategie per far fronte al ritardo studentesco nel CLM in Medicina

Author

Pietro Gallo, Isabella Barajon, Carlo della Rocca, Adolfo Mazzeo, Manuela Merli, Bruno Moncharmont, Maria Grazia Strepparava, Gallo, P, Barajon, I, della Rocca, C, Mazzeo, A, Merli, M, Moncharmont, B, and Strepparava, M

Subjects

Assessment Flexibility, Monitoraggio del Ritardo Studentesco, Medical Education, M-PED/03 - DIDATTICA E PEDAGOGIA SPECIALE, Tutoring, Flessibilità dell’Ordinamento, Remediation, M-PSI/08 - PSICOLOGIA CLINICA, Curriculum Flexibility, Pedagogia Medica, Tutoraggio, Valutazione dell’apprendimento

Abstract

The Presidents of the Italian Undergraduate Curricula in Medicine have faced the problem of remediation in a workshop held in Udine on the 22nd September 2017. Presidents have been subdivided into small groups, have been given detailed data about a hypothetic undergraduate curriculum and have been asked to devise remediation strategies adequate to the case study proposed. Data included general information about the School of Medicine, its structure and scientific excellences, and amount and composition of teaching staff. Information has been given also on the region where the School is placed, its population and social-economical parameters, and on the number and origin of medical students. Entity of students’ graduation delay has been detailed. Undergraduate curriculum has been illustrated giving detailed information about the examinations: their number, weight in credits, deployment through the curriculum, and number of students passing them in due time, with minimum, maximum and average score. Rules for students entry blocks for the following year and information about the consistency of tutoringcounselling services and of teachers continuous education strategies have been finally given. The Presidents of Undergraduate Curricula in Medicine have reached the conclusions that they should obtain the necessary detailed information about entity and causes of their students’ graduation delay. Remediation strategies should include active and peer-to-peer tutoring and forms of flexibility in assessment design and curriculum re-modelling.

Published

2017

19. Neuronal Differentiation Dictates Estrogen-Dependent Survival and ERK1/2 Kinetic by Means of Caveolin-1

Author

VOLPICELLI, FLORIANA, Massimiliano Caiazzo, Bruno Moncharmont, Umberto di Porzio, Luca Colucci D?Amato, CAIAZZO, MASSIMILIANO, Volpicelli, Floriana, Massimiliano, Caiazzo, Bruno, Moncharmont, Umberto di, Porzio, Luca Colucci, D?amato, Caiazzo, Massimiliano, Volpicelli, F, Caiazzo, M, Moncharmont, B, di Porzio, U, and COLUCCI D'AMATO, Generoso Luca

Subjects

Coated pits, Physiology, Cellular differentiation, Caveolin 1, Gene Expression, Estrogen receptor, lcsh:Medicine, Stimulation, Biochemistry, Mice, estrogen, Medicine and Health Sciences, Lipid Hormones, Phosphorylation, lcsh:Science, Mitogen-Activated Protein Kinase 1, Neurons, Mitogen-Activated Protein Kinase 3, Multidisciplinary, Estradiol, Organic Compounds, beta-Cyclodextrins, Cell Differentiation, Research Assessment, Cell biology, Protein Transport, Chemistry, ERK, Physical Sciences, Neuronal Differentiation, Protein Binding, Research Article, Neuronal differentiation, Estrogens, Cell differentiation, Cell type, Cell Survival, medicine.drug_class, Biology, Research and Analysis Methods, Cell Line, medicine, Animals, Gene Silencing, Molecular Biology, Cell Proliferation, Ethanol, Cell growth, Cell Membrane, Organic Chemistry, lcsh:R, Estrogen Receptor alpha, Chemical Compounds, Biology and Life Sciences, Cell Biology, Neuron, Hormones, Retraction, Estrogen, Alcohols, lcsh:Q, Estrogen receptor alpha, Developmental Biology, Neuroscience

Abstract

Estrogens promote a plethora of effects in the CNS that profoundly affect both its development and mature functions and are able to influence proliferation, differentiation, survival and neurotransmission. The biological effects of estrogens are cell-context specific and also depend on differentiation and/or proliferation status in a given cell type. Furthermore, estrogens activate ERK1/2 in a variety of cellular types. Here, we investigated whether ERK1/2 activation might be influenced by estrogens stimulation according to the differentiation status and the molecular mechanisms underling this phenomenon. ERK1/2 exert an opposing role on survival and death, as well as on proliferation and differentiation depending on different kinetics of phosphorylation. Hence we report that mesencephalic primary cultures and the immortalized cell line mes-c-myc A1 express estrogen receptor a and activate ERK1/2 upon E-2 stimulation. Interestingly, following the arrest of proliferation and the onset of differentiation, we observe a change in the kinetic of ERKs phosphorylation induced by estrogens stimulation. Moreover, caveolin-1, a main constituent of caveolae, endogenously expressed and co-localized with ER-alpha on plasma membrane, is consistently up-regulated following differentiation and cell growth arrest. In addition, we demonstrate that siRNA-induced caveolin-1 down-regulation or disruption by means of beta-cyclodextrin treatment changes ERK1/2 phosphorylation in response to estrogens stimulation. Finally, caveolin-1 down-regulation abolishes estrogens-dependent survival of neurons. Thus, caveolin-1 appears to be an important player in mediating, at least, some of the non-genomic action of estrogens in neurons, in particular ERK1/2 kinetics of activation and survival.

Published

2014

20. The retinoblastoma-interacting zinc-finger protein RIZ is a downstream effector of estrogen action

Author

Ciro Abbondanza, Nicola Medici, Vincenzo Nigro, Valentina Rossi, Luigi Gallo, Giulio Piluso, Angela Belsito, Annarita Roscigno, Paola Bontempo, Annibale A. Puca, Anna Maria Molinari, Bruno Moncharmont, Giovanni A. Puca, Abbondanza, Ciro, Medici, Nicola, Nigro, Vincenzo, Rossi, V, Gallo, L, Piluso, Giulio, Belsito, Angela, Roscigno, A, Bontempo, Paola, Puca, Aa, Molinari, Anna Maria, Moncharmont, B, and Puca, Ga

Subjects

DNA-Binding Proteins, Multidisciplinary, Base Sequence, Receptors, Estrogen, Humans, Nuclear Proteins, Estrogens, Zinc Fingers, Histone-Lysine N-Methyltransferase, Biological Sciences, Cell Line, DNA Primers, Transcription Factors

Abstract

Co-immunoprecipitation experiments in cell extract from cultured cells or target tissues indicated that estrogen receptor was complexed with the retinoblastoma binding protein RIZ in a ligand-dependent manner. Mapping of interaction sites indicated that in both proteins the same regions and motifs responsible for the interaction of transcriptional co-activator and nuclear receptors were involved. In cultured cells, estradiol induced a redistribution of RIZ protein within the nucleus and in the cytoplasm. A similar effect was produced in vivo , in prepuberal rat endometrium, by administration of a physiological dose of estradiol. Therefore, RIZ protein could be a specific effector of estrogen action downstream of the hormone-receptor interaction, presumably involved in proliferation control.

Published

2000

21. PRDM Proteins: Molecular Mechanisms in Signal Transduction and Transcriptional Regulation

Author

Ciro Abbondanza, Bruno Moncharmont, Erika Di Zazzo, Caterina De Rosa, DI ZAZZO, E, De, Rosa, Abbondanza, Ciro, and Moncharmont, B.

Subjects

Regulation of gene expression, Genetics, General Immunology and Microbiology, Protein family, Review, Biology, General Biochemistry, Genetics and Molecular Biology, Chromatin remodeling, Chromatin, Transduction (genetics), lcsh:Biology (General), PRDM gene family, Transcriptional regulation, Neoplastic transformation, transcriptional regulation, Signal transduction, General Agricultural and Biological Sciences, lcsh:QH301-705.5, signal transduction

Abstract

PRDM (PRDI-BF1 and RIZ homology domain containing) protein family members are characterized by the presence of a PR domain and a variable number of Zn-finger repeats. Experimental evidence has shown that the PRDM proteins play an important role in gene expression regulation, modifying the chromatin structure either directly, through the intrinsic methyltransferase activity, or indirectly through the recruitment of chromatin remodeling complexes. PRDM proteins have a dual action: they mediate the effect induced by different cell signals like steroid hormones and control the expression of growth factors. PRDM proteins therefore have a pivotal role in the transduction of signals that control cell proliferation and differentiation and consequently neoplastic transformation. In this review, we describe pathways in which PRDM proteins are involved and the molecular mechanism of their transcriptional regulation.

Published

2012

22. patologia del metabolismo lipidico

Author

DI JESO, Bruno, moncharmont b, and DI JESO, Bruno

Subjects

lipoproteine, malattie del metabolismo lipidico, metabolismo

Abstract

Struttura e metabolismo delle lipoproteine plasmatiche, Enzimi e trasportatori chiave del metabolismo delle lipoproteine, Recettori delle lipoproteine, Metabolismo delle lipoproteine contenenti apoB, Biogenesi delle HDL e trasporto inverso del colesterolo, Principali malattie del metabolismo lipidico.

Published

2012

23. Highlighting chromosome loops in DNA-picked chromatin (DPC)

Author

Ciro Abbondanza, Fabiana Aceto, Nicola Medici, Bruno Perillo, Lucia Altucci, Giovanni Alfredo Puca, Maria Neve Ombra, Enrico V. Avvedimento, Bruno Moncharmont, Caterina De Rosa, Antonio Porcellini, Abbondanza, Ciro, De Rosa, C, Ombra, Mn, Aceto, F, Medici, Nicola, Altucci, Lucia, Moncharmontb, Puca, Ga, Porcellini, A, Avvedimento, Ev, Perillo, B., Abbondanza, C, Medici, N, Altucci, L, Moncharmont, B, Porcellini, Antonio, and Avvedimento, VITTORIO ENRICO

Subjects

Proteomics, Cancer Research, Transcription, Genetic, Computational biology, Biology, Response Elements, chemistry.chemical_compound, Transcription (biology), Cell Line, Tumor, Gene expression, Chromosomes, Human, Humans, DNA looping, Molecular Biology, Gene, Genetics, Histone Demethylases, Estradiol, epigenetics, Chromatin, Genes, bcl-2, nuclear architecture, chemistry, Nucleic Acid Conformation, chromatin, Female, transcription, DNA

Abstract

"Growing evidence supports the concept that dynamic intra-and inter-chromosomal links between specific loci contribute to the creation of cell type-specific gene expression profiles. Therefore, analysis of the establishment of peculiar functional correlations between sites, also distant on linear DNA, that govern the transcriptional process appears to be of fundamental relevance. We propose here an experimental approach showing that 17 beta-estradiol-induced transcription associates to formation of loops between the promoter and termination regions of hormone-responsive genes. This strategy reveals as a tool to be also suitably used, in conjunction with automated techniques, for an extensive analysis of sites shared by multiple genes for induced expression."

Published

2011

24. In VitroBinding of the Purified Hormone-Binding Subunit of the Estrogen Receptor to Oligonucleotides Containing Natural or Modified Sequences of an Estrogen-Responsive Element

Author

Vincenzo Nigro, Ciro Abbondanza, Nicola Medici, Anna Maria Molinari, Bruno Moncharmont, Giovanni Alfredo Puca, Medici, Nicola, Nigro, Vincenzo, Abbondanza, Ciro, Moncharmont, B, Molinari, Anna Maria, and Puca, Ga

Subjects

Protein subunit, Response element, Estrogen receptor, In Vitro Techniques, Biology, Endocrinology, Affinity chromatography, Animals, Electrophoretic mobility shift assay, Molecular Biology, Dyad symmetry, Hormone response element, Chromatography, Binding Sites, Base Sequence, Estradiol, Oligonucleotide, General Medicine, Molecular biology, Gene Expression Regulation, Receptors, Estrogen, Biochemistry, Cattle, Electrophoresis, Polyacrylamide Gel, Female, hormones, hormone substitutes, and hormone antagonists

Abstract

Estrogen receptor (ER) was purified from calf uterus by immunoaffinity chromatography in the absence of the ligand. The purified ER consists of a mixture of monomer and homodimer forms of 67-kDa hormone-binding subunit (no 90-kDa heat shock protein is present). The purified ER was incubated with a 32P-labeled 61-basepair oligonucleotide containing the sequence of the estrogen response element (ERE) of the Xenopus laevis A2 vitellogenin gene. DNA mobility shift assays showed formation of specific complexes of the ERE containing oligonucleotide with ER, formation which did not require and was not affected by estradiol or antiestrogenic molecules. Both the monomer and the dimer were equally able to interact with the ERE-containing oligonucleotide. Sucrose gradient experiments showed that only the ER monomer is able to interact with an oligonucleotide in which a single mutation destroyed the dyad symmetry of ERE. Multiple symmetric mutations which did not alter the dyad symmetry of ERE nevertheless totally destroyed the ability of the oligonucleotide to form complexes with either the monomeric or dimeric form of ER. These results suggest that ER is able to bind to ERE independently of the presence of estradiol or other proteins and, therefore, that estradiol does not act by modulating the ability of ER to bind to ERE on DNA.

Published

1991

25. Proteomic analysis of MCF-7 cell lines expressing the zinc-finger or the proline-rich domain of retinoblastoma-interacting-zinc-finger protein

Author

Livia Malorni, Annarita Farina, Bruno Moncharmont, Ciro Abbondanza, Gabriella Pocsfalvi, Antimo Di Maro, Augusto Parente, M. Rossi, and Antonio Malorni, Angela Chambery, Giuseppina Cacace, Chambery, A., Farina, A., DI MARO, A., Rossi, M., Abbondanza, C., Moncharmont, B., Malorni, L., Cacace, G., Pocsfalvi, G., Malorni, A., and Parente, A.

Subjects

Proteomics, Transcription Factors/analysis/genetics/metabolism, Biochemistry, Cathepsin D, Tumor Suppressor Proteins/metabolism, RNA/metabolism, Two-dimensional gel electrophoresi, Protein Isoforms, Electrophoresis, Gel, Two-Dimensional, Peptide mass fingerprint, Peptide-mass fingerprint, Nuclear Proteins/analysis/genetics/metabolism, Cytoskeleton, Zinc finger, RIZ domain, Retinoblastoma, Nuclear Proteins, DNA-Binding Proteins, Female, Proteomics/methods, Phosphopyruvate Hydratase/metabolism, Breast Neoplasms, Biology, Cell Line, Tumor, medicine, Biomarkers, Tumor, Humans, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization/methods, Gene, DNA-Binding Proteins/analysis/genetics/metabolism, Two-dimensional gel electrophoresis, Mass spectrometry, Tumor Suppressor Proteins, Proteomic, General Chemistry, Histone-Lysine N-Methyltransferase, Cathepsin D/metabolism, medicine.disease, Molecular biology, Breast Neoplasms/metabolism/pathology, Protein Structure, Tertiary, MCF-7, Cell culture, Biomarkers, Tumor/metabolism, Phosphopyruvate Hydratase, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Cytoskeleton/metabolism, RNA, Energy Metabolism, Transcription Factors

Abstract

To identify a growth-promoting activity related to retinoblastoma-interacting-zinc-finger (RIZ) protein, differential protein expression of MCF-7 cell lines expressing the zinc-finger or the proline-rich domain of RIZ protein was analyzed by a robust bottom-up mass-spectrometry proteomic approach. Spots corresponding to qualitative and quantitative differences in protein expression have been selected and identified. Some of these proteins have been previously reported as being associated with different types of carcinomas or involved in cell proliferation and differentiation. Knowledge of specific differentially expressed proteins by MCF-7-derived cell lines expressing RIZ different domains will provide the basis for identifying a growth-promoting activity related to RIZ gene products. To identify a growth-promoting activity related to retinoblastoma- interacting-zinc-finger (RIZ) protein, differential protein expression of MCF-7 cell lines expressing the zinc-finger or the proline-rich domain of RIZ protein was analyzed by a robust bottom-up mass-spectrometry proteomic approach. Spots corresponding to qualitative and quantitative differences in protein expression have been selected and identified. Some of these proteins have been previously reported as being associated with different types of carcinomas or involved in cell proliferation and differentiation. Knowledge of specific differentially expressed proteins by MCF-7-derived cell lines expressing RIZ different domains will provide the basis for identifying a growth-promoting activity related to RIZ gene products. © 2006 American Chemical Society.

Published

2006

26. Differentiation of myeloid cell lines correlates with a selective expression of RIZ protein

Author

Bruno Moncharmont, Paola Bontempo, Ignazio Armetta, M De Simone, Em Schiavone, Am Molinari, Nicola Medici, E. Nola, Patrizia Gazzerro, Ciro Abbondanza, Ga Puca, Gazzerro, P, Bontempo, Paola, Schiavone, Em, Abbondanza, Ciro, Moncharmont, B, Armetta, I, Medici, Nicola, DE SIMONE, M, Nola, Ernesto, Puca, Ga, and Molinari, Anna Maria

Subjects

Immunoblotting, Retinoic acid, Antineoplastic Agents, Tretinoin, Retinoic acid receptor beta, Biology, Benzoates, Retinoblastoma Protein, Adenoviridae, Retinoic acid-inducible orphan G protein-coupled receptor, Retinoids, chemistry.chemical_compound, Genetics, Humans, Myeloid Cells, Molecular Biology, Cells, Cultured, Genetics (clinical), Nuclear Proteins, Cell Differentiation, Zinc Fingers, Histone-Lysine N-Methyltransferase, Retinoic acid receptor gamma, Retinoid X receptor gamma, Immunohistochemistry, Molecular biology, Adenosine Monophosphate, DNA-Binding Proteins, Retinoic acid receptor, P19 cell, chemistry, Retinoic acid receptor alpha, Molecular Medicine, Research Article, Transcription Factors

Abstract

BACKGROUND: The retinoblastoma-interacting zinc-finger gene RIZ is expressed in two forms (RIZ1 and RIZ2) that differ for the presence near the N-terminus of RIZ1 of a conserved domain, defined PR (PRDI-BF1-RIZ homology), homologous to a similar domain present in other proteins recognized as tumor suppressor gene products. The RIZ1 form is usually absent or expressed at low levels in tumor cells, whereas RIZ2 is frequently expressed. We investigated a possible involvement of RIZ1 in differentiation control using a myeloid cell maturation model that is easily modulated by retinoids and other agents. MATERIALS AND METHODS: HL60 or NB4 cell lines or patients' leukemic promyelocytes were treated with all- trans -retinoic acid or other agents to induce differentiation. RIZ gene expression was determined with reverse transcriptase polymerase chain reaction (RT-PCR) and RNase protection assay. Immunocytochemistry was performed to assess variation of the intracellular distribution of RIZ protein on all- trans-retinoic acid treatment. Forced expression of RIZ1 protein was obtained with a recombinant adenovirus containing RIZ1 cDNA. RESULTS: Treatment with retinoic acid induced a selective expression of RIZ1 in HL60 cell line. Retinoic acid effect was maximal at 7 days and correlated to the granulocytic differentiation of cells. A similar effect was obtained in retinoic acid-sensitive NB4 cell line or in patients' leukemic promyelocytes, but not in the retinoic acid-resistant cell line NB4.007/6 or in the U937 cell line. Selective expression of RIZ1 was also induced by 12-O-tetradecanoyl-phorbol-13-acetate in the U937 and HL60 cell lines and by 1,25-dihydroxyvitamin D(3) only in HL60 cells. In HL60 cells, RIZ1 was also induced by activation of a retinoid alpha receptor-independent maturation pathway based on retinoid X receptor agonist and protein kinase A synergism. In addition, retinoic acid produced a redistribution of the antigen within the nucleus in these cells. Forced expression of RIZ1 protein induced growth arrest and death of HL60 cells. CONCLUSIONS: The correlation between the selective expression of RIZ1 induced by retinoic acid, 12-O-tetradecanoyl-phorbol-13-acetate, or 1,25-dihydroxyvitamin D(3) and differentiation suggested that RIZ protein was involved in myeloid cell differentiation induced by these agents.

Published

2001

27. Interaction of vault particles with estrogen receptor in the MCF-7 breast cancer cell

Author

Vincenzo Nigro, Ciro Abbondanza, Angela Belsito, Nicola Medici, Giulio Piluso, Anna Maria Molinari, Giovanni Alfredo Puca, Bruno Moncharmont, Valentina Rossi, Luigi Gallo, Annarita Roscigno, Abbondanza, Ciro, Rossi, V, Roscigno, A, Gallo, L, Belsito, Angela, Piluso, Giulio, Medici, Nicola, Nigro, Vincenzo, Molinari, Anna Maria, Moncharmont, B, and Puca, Ga

Subjects

Vault RNA, Recombinant Fusion Proteins, Receptors, Cytoplasmic and Nuclear, Estrogen receptor, Breast Neoplasms, Mice, Major vault protein, Tumor Cells, Cultured, Animals, Humans, Receptor, Vault (organelle), Estrogen receptor beta, Vault Ribonucleoprotein Particles, Ribonucleoprotein, Mice, Inbred BALB C, Estradiol, biology, Estrogens, Articles, Cell Biology, Precipitin Tests, Molecular biology, Neoplasm Proteins, Receptors, Estrogen, Ribonucleoproteins, Nuclear receptor, biology.protein, RNA, Female, HeLa Cells

Abstract

A 104-kD protein was coimmunoprecipitated with the estrogen receptor from the flowtrough of a phosphocellulose chromatography of MCF-7 cell nuclear extract. mAbs to this protein identified several cDNA clones coding for the human 104-kD major vault protein. Vaults are large ribonucleoprotein particles of unknown function present in all eukaryotic cells. They have a complex morphology, including several small molecules of RNA, but a single protein species, the major vault protein, accounts for >70% of their mass. Their shape is reminiscent of the nucleopore central plug, but no proteins of known function have been described to interact with them. Western blot analysis of vaults purified on sucrose gradient showed the presence of estrogen receptor co-migrating with the vault peak. The AER317 antibody to estrogen receptor coimmunoprecipitated the major vault protein and the vault RNA also in the 20,000 g supernatant fraction. Reconstitution experiments of estrogen receptor fragments with the major vault protein mapped the site of the interaction between amino acids 241 and 280 of human estrogen receptor, where the nuclear localization signal sequences are located. Estradiol treatment of cells increased the amount of major vault protein present in the nuclear extract and coimmunoprecipitated with estrogen receptor, whereas the anti-estrogen ICI182,780 had no effect. The hormone-dependent interaction of vaults with estrogen receptor was reproducible in vitro and was prevented by sodium molybdate. Antibodies to progesterone and glucocorticoid receptors were able to coimmunoprecipitate the major vault protein. The association of nuclear receptors with vaults could be related to their intracellular traffic.

Published

1998

28. Proteolytic activity of the purified hormone-binding subunit in the estrogen receptor

Author

Ciro Abbondanza, Ignazio Armetta, Nicola Medici, Bruno Moncharmont, Anna Maria Molinari, Giovanni Alfredo Puca, Vincenzo Nigro, Saverio Minucci, Molinari, Anna Maria, Abbondanza, Ciro, Armetta, I., Medici, Nicola, Minucci, Sergio, Moncharmont, B., Nigro, Vincenzo, and Puca, Ga

Subjects

Isoflurophate, Estradiol Antagonists, medicine.drug_class, Polyunsaturated Alkamides, Molecular Sequence Data, Phenylalanine, Biology, Serine, Aprotinin, Affinity chromatography, Endopeptidases, medicine, Animals, Amino Acid Sequence, Receptor, chemistry.chemical_classification, Multidisciplinary, Estradiol, Hydrolysis, Uterus, Estrogen Antagonists, Molecular biology, Amino acid, Tamoxifen, Biochemistry, chemistry, Chromogenic Compounds, Receptors, Estrogen, Estrogen, Diisopropyl fluorophosphate, Cattle, Electrophoresis, Polyacrylamide Gel, Female, hormones, hormone substitutes, and hormone antagonists, medicine.drug, Research Article

Abstract

The hormone-binding subunit of the calf uterus estradiol receptor was purified as a hormone-free molecule. Immunoaffinity chromatography with a specific monoclonal antibody was used as the final step. The purified subunit was specifically labeled by radioactive diisopropyl fluorophosphate. The diisopropyl fluorophosphate-labeled amino acid was serine. The purified receptor was able to release the fluorogenic or chromogenic group from synthetic peptides containing phenylalanine at the carboxyl terminus. This occurred only in the presence of estradiol and was hampered by aprotinin and diisopropyl fluorophosphate. Estradiol-dependent hydrolytic activity was also found in the eluate from gel slices after SDS/PAGE of purified receptor. This activity comigrated with the renaturable estradiol-binding activity. The estradiol antagonists 4-hydroxytamoxifen and ICI 164,384 as well as other steroid hormones were unable to activate this hydrolytic activity.

Published

1991

29. Estradiol receptor of calf uterus: interactions with heparin-agarose and purification

Author

Nicola Medici, Giovanni Alfredo Puca, Anna Maria Molinari, Bruno Moncharmont, Molinari, Anna Maria, Medici, Nicola, Moncharmont, B, and Puca, Ga

Subjects

Size-exclusion chromatography, In Vitro Techniques, Chromatography, DEAE-Cellulose, chemistry.chemical_compound, Polysaccharides, Centrifugation, Density Gradient, Animals, Chondroitin sulfate, Receptor, Polyacrylamide gel electrophoresis, Cell Nucleus, Multidisciplinary, Chromatography, Estradiol, Chemistry, Heparin, Sepharose, Chondroitin Sulfates, Uterus, Sedimentation coefficient, Molecular Weight, Isoelectric point, Biochemistry, Receptors, Estrogen, Sephadex, Chromatography, Gel, Agarose, Cattle, Electrophoresis, Polyacrylamide Gel, Female, Research Article

Abstract

Heparin attached covalently to agarose beads binds the "native" form of the estradiol receptor with very high affinity. Chondroitin sulfate does not bind to the receptor. When the receptor is complexed with hormone, the affinity is at least 10 times higher. Only the "native" and not the "nuclear" or the "derived" (i.e., after activation by a calcium-dependent enzyme) forms of the estradiol receptor interact with heparin. The "native" estradiol-receptor complex is purified to homogeneity after chromatography on columns of heparin-agarose, Sephadex G-200, and DEAE-cellulose, followed by two more Sephadex G-200 columns. The purified molecule is a single polypeptide of molecular weight 69,000 by polyacrylamide gel electrophoresis in sodium dodecyl sulphate. The sedimentation coefficient on sucrose gradients is 4.3 S, the Stokes radius from gel filtration is 36.5 A, and the isoelectric point is 6.4. The purified [3H]estradiol-receptor complex exchanges the radioactive hormone with estradiol or other estrogenic steroids, but not with testosterone, 5alpha-dihydrotestosterone, or progesterone.

Published

1977

30. Dual-specificity phosphatase (DUSP6) in human glioblastoma: epithelial-to-mesenchymal transition (EMT) involvement.

Author

Zuchegna C, Di Zazzo E, Moncharmont B, and Messina S

Subjects

Adult, Cell Line, Tumor, Dual Specificity Phosphatase 6, Dual-Specificity Phosphatases, Epithelial-Mesenchymal Transition genetics, Humans, Brain Neoplasms genetics, Glioblastoma genetics

Abstract

Objective: Glioblastoma (GBM) is the most aggressive and common form of primary brain cancer. Survival is poor and improved treatment options are urgently needed. Dual specificity phosphatase-6 (DUSP6) is actively involved in oncogenesis showing unexpected tumor-promoting properties in human glioblastoma, contributing to the development and expression of the full malignant and invasive phenotype. The purpose of this study was to assess if DUSP6 activates epithelial-to-mesenchymal transition (EMT) in glioblastoma and its connection with the invasive capacity., Results: We found high levels of transcripts mRNA by qPCR analysis in a panel of primary GBM compared to adult or fetal normal tissues. At translational levels, these data correlate with high protein expression and long half-life values by cycloheximide-chase assay in immunoblot experiments. Next, we demonstrate that DUSP6 gene is involved in epithelial-to-mesenchymal transition (EMT) in GBM by immunoblot characterization of the mesenchymal and epithelial markers. Vimentin, N-Cadherin, E-Cadherin and fibronectin were measured with and without DUSP6 over-expression, and in response to several stimuli such as chemotherapy treatment. In particular, the high levels of vimentin were blunted at increasing doses of cisplatin in condition of DUSP6 over-expression while N-Cadherin contextually increased. Finally, DUSP6 per se increased invasion capacity of GBM. Overall, our data unveil the DUSP6 involvement in invasive mesenchymal-like properties in GBM.

Published

2020

31. Multifaceted Role of PRDM Proteins in Human Cancer.

Author

Casamassimi A, Rienzo M, Di Zazzo E, Sorrentino A, Fiore D, Proto MC, Moncharmont B, Gazzerro P, Bifulco M, and Abbondanza C

Subjects

Animals, DNA-Binding Proteins metabolism, Disease Susceptibility, Gene Expression Regulation, Neoplastic, Histone-Lysine N-Methyltransferase metabolism, Humans, Multigene Family, Neoplasms mortality, Neoplasms pathology, Nuclear Proteins metabolism, Prognosis, Protein Binding, Protein Interaction Domains and Motifs, Signal Transduction, Transcription Factors metabolism, DNA-Binding Proteins genetics, Histone-Lysine N-Methyltransferase genetics, Neoplasms etiology, Neoplasms metabolism, Nuclear Proteins genetics, Positive Regulatory Domain I-Binding Factor 1 genetics, Positive Regulatory Domain I-Binding Factor 1 metabolism, Transcription Factors genetics

Abstract

The PR/SET domain family (PRDM) comprise a family of genes whose protein products share a conserved N-terminal PR [PRDI-BF1 (positive regulatory domain I-binding factor 1) and RIZ1 (retinoblastoma protein-interacting zinc finger gene 1)] homologous domain structurally and functionally similar to the catalytic SET [Su(var)3-9, enhancer-of-zeste and trithorax] domain of histone methyltransferases (HMTs). These genes are involved in epigenetic regulation of gene expression through their intrinsic HMTase activity or via interactions with other chromatin modifying enzymes. In this way they control a broad spectrum of biological processes, including proliferation and differentiation control, cell cycle progression, and maintenance of immune cell homeostasis. In cancer, tumor-specific dysfunctions of PRDM genes alter their expression by genetic and/or epigenetic modifications. A common characteristic of most PRDM genes is to encode for two main molecular variants with or without the PR domain. They are generated by either alternative splicing or alternative use of different promoters and play opposite roles, particularly in cancer where their imbalance can be often observed. In this scenario, PRDM proteins are involved in cancer onset, invasion, and metastasis and their altered expression is related to poor prognosis and clinical outcome. These functions strongly suggest their potential use in cancer management as diagnostic or prognostic tools and as new targets of therapeutic intervention.

Published

2020

32. Adiponectin as Link Factor between Adipose Tissue and Cancer.

Author

Di Zazzo E, Polito R, Bartollino S, Nigro E, Porcile C, Bianco A, Daniele A, and Moncharmont B

Subjects

Adiponectin chemistry, Animals, Humans, Inflammation metabolism, Models, Biological, Signal Transduction, Adiponectin metabolism, Adipose Tissue metabolism, Neoplasms metabolism

Abstract

Adipose tissue is a key regulator of energy balance playing an active role in lipid storage as well as in synthesizing several hormones directly involved in the pathogenesis of obesity. Obesity represents a peculiar risk factor for a growing list of cancers and is frequently associated to poor clinical outcome. The mechanism linking obesity and cancer is not completely understood, but, amongst the major players, there are both chronic low-grade inflammation and deregulation of adipokines secretion. In obesity, the adipose tissue is pervaded by an abnormal number of immune cells that create an inflammatory environment supporting tumor cell proliferation and invasion. Adiponectin (APN), the most abundant adipokine, shows anti-inflammatory, anti-proliferative and pro-apoptotic properties. Circulating levels of APN are drastically decreased in obesity, suggesting that APN may represent the link factor between obesity and cancer risk. The present review describes the recent advances on the involvement of APN and its receptors in the etiology of different types of cancer.

Published

2019

33. Early and Late Induction of KRAS and HRAS Proto-Oncogenes by Reactive Oxygen Species in Primary Astrocytes.

Author

Messina S, Di Zazzo E, and Moncharmont B

Abstract

Astrocytes, one of the predominant types of glial cells, function as both supportive and metabolic cells for the brain. Among mammalian tissues, the highest levels of p21 Ras protein are detected in the brain. Here, we investigated the expression of KRAS and HRAS proto-oncogenes in primary astrocytes following acute oxidative stimulation. Reactive oxygen species (ROS) changed the expression of proto-oncogenes at both transcriptional and translational levels. De novo protein synthesis analysis measured approximate values of proteins half-life, ranging from 1-4 h, of the different H- and K- isoforms by western blot analysis. Quantitative gene expression analysis of KRAS and HRAS revealed an unexpected short-term induction of KRAS mRNA in primary astrocytes in response to acute stimulation. Indeed, cultured astrocytes responded to proteasomal inhibition by preventing the reduction of c-K-Ras. A fraction of K-Ras protein accumulated in the presence of ROS and cycloheximide, while a substantial proportion was continuously synthesized. These data indicate that ROS regulate in a complementary fashion p21 Ras isoforms in primary astrocytes: K-Ras is rapidly and transiently induced by post-translational and post-transcriptional mechanisms, while H-Ras is stably induced by mRNA accumulation. We suggest that K-Ras and H-Ras are ROS sensors that adapt cells to metabolic needs and oxidative stress., Competing Interests: The authors declare that they have no conflicts of interest.

Published

2017

34. Critical Function of PRDM2 in the Neoplastic Growth of Testicular Germ Cell Tumors.

Author

Di Zazzo E, Porcile C, Bartollino S, and Moncharmont B

Abstract

Testicular germ cell tumors (TGCTs) derive from primordial germ cells. Their maturation is blocked at different stages, reflecting histological tumor subtypes. A common genetic alteration in TGCT is a deletion of the chromosome 1 short arm, where the PRDM2 gene, belonging to the P ositive R egulatory domain gene ( PRDM ) family, is located. Expression of PRDM2 gene is shifted in different human tumors, where the expression of the two principal protein forms coded by PRDM2 gene, RIZ1 and RIZ2, is frequently unbalanced. Therefore, PRDM2 is actually considered a candidate tumor suppressor gene in different types of cancer. Although recent studies have demonstrated that PRDM gene family members have a pivotal role during the early stages of testicular development, no information are actually available on the involvement of these genes in TGCTs. In this article we show by qRT-PCR analysis that PRDM2 expression level is modulated by proliferation and differentiation agents such as estradiol, whose exposure during fetal life is probably an important risk factor for TGCTs development in adulthood. Furthermore in normal and cancer germ cell lines, PRDM2 binds estradiol receptor α (ERα) and influences proliferation, survival and apoptosis, as previously reported using MCF-7 breast cancer cell line, suggesting a potential tumor-suppressor role in TGCT formation., Competing Interests: The authors declare that they have no conflicts of interest.

Published

2016

35. Prostate cancer stem cells: the role of androgen and estrogen receptors.

Author

Di Zazzo E, Galasso G, Giovannelli P, Di Donato M, Di Santi A, Cernera G, Rossi V, Abbondanza C, Moncharmont B, Sinisi AA, Castoria G, and Migliaccio A

Subjects

Androgens pharmacology, Gene Expression Regulation, Neoplastic drug effects, Humans, Male, Models, Genetic, Neoplastic Stem Cells pathology, Prostatic Neoplasms metabolism, Prostatic Neoplasms pathology, Receptors, Androgen metabolism, Receptors, Estrogen metabolism, Receptors, G-Protein-Coupled genetics, Receptors, G-Protein-Coupled metabolism, Neoplastic Stem Cells metabolism, Prostatic Neoplasms genetics, Receptors, Androgen genetics, Receptors, Estrogen genetics

Abstract

Prostate cancer is one of the most commonly diagnosed cancers in men, and androgen deprivation therapy still represents the primary treatment for prostate cancer patients. This approach, however, frequently fails and patients develop castration-resistant prostate cancer, which is almost untreatable.Cancer cells are characterized by a hierarchical organization, and stem/progenitor cells are endowed with tumor-initiating activity. Accumulating evidence indicates that prostate cancer stem cells lack the androgen receptor and are, indeed, resistant to androgen deprivation therapy. In contrast, these cells express classical (α and/or β) and novel (GPR30) estrogen receptors, which may represent new putative targets in prostate cancer treatment.In the present review, we discuss the still-debated mechanisms, both genomic and non-genomic, by which androgen and estradiol receptors (classical and novel) mediate the hormonal control of prostate cell stemness, transformation, and the continued growth of prostate cancer. Recent preclinical and clinical findings obtained using new androgen receptor antagonists, anti-estrogens, or compounds such as enhancers of androgen receptor degradation and peptides inhibiting non-genomic androgen functions are also presented. These new drugs will likely lead to significant advances in prostate cancer therapy.

Published

2016

36. Neuronal differentiation dictates estrogen-dependent survival and ERK1/2 kinetic by means of caveolin-1.

Author

Volpicelli F, Caiazzo M, Moncharmont B, di Porzio U, and Colucci-D'Amato L

Subjects

Animals, Caveolin 1 genetics, Cell Line, Cell Membrane metabolism, Cell Proliferation drug effects, Cell Survival drug effects, Cell Survival genetics, Estrogen Receptor alpha metabolism, Estrogens pharmacology, Gene Expression, Gene Silencing, Mice, Neurons drug effects, Phosphorylation, Protein Binding, Protein Transport, beta-Cyclodextrins pharmacology, Caveolin 1 metabolism, Cell Differentiation, Estrogens metabolism, Mitogen-Activated Protein Kinase 1 metabolism, Mitogen-Activated Protein Kinase 3 metabolism, Neurons cytology, Neurons metabolism

Abstract

Estrogens promote a plethora of effects in the CNS that profoundly affect both its development and mature functions and are able to influence proliferation, differentiation, survival and neurotransmission. The biological effects of estrogens are cell-context specific and also depend on differentiation and/or proliferation status in a given cell type. Furthermore, estrogens activate ERK1/2 in a variety of cellular types. Here, we investigated whether ERK1/2 activation might be influenced by estrogens stimulation according to the differentiation status and the molecular mechanisms underling this phenomenon. ERK1/2 exert an opposing role on survival and death, as well as on proliferation and differentiation depending on different kinetics of phosphorylation. Hence we report that mesencephalic primary cultures and the immortalized cell line mes-c-myc A1 express estrogen receptor α and activate ERK1/2 upon E2 stimulation. Interestingly, following the arrest of proliferation and the onset of differentiation, we observe a change in the kinetic of ERKs phosphorylation induced by estrogens stimulation. Moreover, caveolin-1, a main constituent of caveolae, endogenously expressed and co-localized with ER-α on plasma membrane, is consistently up-regulated following differentiation and cell growth arrest. In addition, we demonstrate that siRNA-induced caveolin-1 down-regulation or disruption by means of ß-cyclodextrin treatment changes ERK1/2 phosphorylation in response to estrogens stimulation. Finally, caveolin-1 down-regulation abolishes estrogens-dependent survival of neurons. Thus, caveolin-1 appears to be an important player in mediating, at least, some of the non-genomic action of estrogens in neurons, in particular ERK1/2 kinetics of activation and survival.

Published

2014

37. PRDM Proteins: Molecular Mechanisms in Signal Transduction and Transcriptional Regulation.

Author

Di Zazzo E, De Rosa C, Abbondanza C, and Moncharmont B

Abstract

PRDM (PRDI-BF1 and RIZ homology domain containing) protein family members are characterized by the presence of a PR domain and a variable number of Zn-finger repeats. Experimental evidence has shown that the PRDM proteins play an important role in gene expression regulation, modifying the chromatin structure either directly, through the intrinsic methyltransferase activity, or indirectly through the recruitment of chromatin remodeling complexes. PRDM proteins have a dual action: they mediate the effect induced by different cell signals like steroid hormones and control the expression of growth factors. PRDM proteins therefore have a pivotal role in the transduction of signals that control cell proliferation and differentiation and consequently neoplastic transformation. In this review, we describe pathways in which PRDM proteins are involved and the molecular mechanism of their transcriptional regulation.

Published

2013

38. Highlighting chromosome loops in DNA-picked chromatin (DPC).

Author

Abbondanza C, De Rosa C, Ombra MN, Aceto F, Medici N, Altucci L, Moncharmont B, Puca GA, Porcellini A, Avvedimento EV, and Perillo B

Subjects

Cell Line, Tumor, Chromatin metabolism, Chromosomes, Human genetics, Estradiol pharmacology, Female, Genes, bcl-2 genetics, Histone Demethylases metabolism, Humans, Chromatin chemistry, Chromosomes, Human chemistry, Estradiol metabolism, Nucleic Acid Conformation, Proteomics methods, Response Elements genetics, Transcription, Genetic

Abstract

Growing evidence supports the concept that dynamic intra- and inter-chromosomal links between specific loci contribute to the creation of cell-type specific gene expression profiles. Therefore, analysis of the establishment of peculiar functional correlations between sites, also distant on linear DNA, that govern the transcriptional process appears to be of fundamental relevance. We propose here an experimental approach showing that 17β-estradiol-induced transcription associates to formation of loops between the promoter and termination regions of hormone-responsive genes. This strategy reveals as a tool to be also suitably used, in conjunction with automated techniques, for an extensive analysis of sites shared by multiple genes for induced expression.

Published

2011

39. Differentiation of myeloid cell lines correlates with a selective expression of RIZ protein.

Author

Gazzerro P, Bontempo P, Schiavone EM, Abbondanza C, Moncharmont B, Armetta I, Medici N, De Simone M, Nola E, Puca GA, and Molinari AM

Subjects

Adenosine Monophosphate analogs & derivatives, Adenoviridae metabolism, Antineoplastic Agents pharmacology, Benzoates pharmacology, Cells, Cultured, Histone-Lysine N-Methyltransferase, Humans, Immunoblotting, Immunohistochemistry, Myeloid Cells cytology, Myeloid Cells drug effects, Nuclear Proteins genetics, Retinoblastoma Protein genetics, Retinoblastoma Protein metabolism, Retinoids pharmacology, Tretinoin pharmacology, Zinc Fingers genetics, Cell Differentiation physiology, DNA-Binding Proteins, Myeloid Cells physiology, Nuclear Proteins metabolism, Transcription Factors

Abstract

Background: The retinoblastoma-interacting zinc-finger gene RIZ is expressed in two forms (RIZ1 and RIZ2) that differ for the presence near the N-terminus of RIZ1 of a conserved domain, defined PR (PRDI-BF1-RIZ homology), homologous to a similar domain present in other proteins recognized as tumor suppressor gene products. The RIZ1 form is usually absent or expressed at low levels in tumor cells, whereas RIZ2 is frequently expressed. We investigated a possible involvement of RIZ1 in differentiation control using a myeloid cell maturation model that is easily modulated by retinoids and other agents., Materials and Methods: HL60 or NB4 cell lines or patients' leukemic promyelocytes were treated with all- trans -retinoic acid or other agents to induce differentiation. RIZ gene expression was determined with reverse transcriptase polymerase chain reaction (RT-PCR) and RNase protection assay. Immunocytochemistry was performed to assess variation of the intracellular distribution of RIZ protein on all- trans-retinoic acid treatment. Forced expression of RIZ1 protein was obtained with a recombinant adenovirus containing RIZ1 cDNA., Results: Treatment with retinoic acid induced a selective expression of RIZ1 in HL60 cell line. Retinoic acid effect was maximal at 7 days and correlated to the granulocytic differentiation of cells. A similar effect was obtained in retinoic acid-sensitive NB4 cell line or in patients' leukemic promyelocytes, but not in the retinoic acid-resistant cell line NB4.007/6 or in the U937 cell line. Selective expression of RIZ1 was also induced by 12-O-tetradecanoyl-phorbol-13-acetate in the U937 and HL60 cell lines and by 1,25-dihydroxyvitamin D(3) only in HL60 cells. In HL60 cells, RIZ1 was also induced by activation of a retinoid alpha receptor-independent maturation pathway based on retinoid X receptor agonist and protein kinase A synergism. In addition, retinoic acid produced a redistribution of the antigen within the nucleus in these cells. Forced expression of RIZ1 protein induced growth arrest and death of HL60 cells., Conclusions: The correlation between the selective expression of RIZ1 induced by retinoic acid, 12-O-tetradecanoyl-phorbol-13-acetate, or 1,25-dihydroxyvitamin D(3) and differentiation suggested that RIZ protein was involved in myeloid cell differentiation induced by these agents.

Published

2001

40. Estradiol induces functional inactivation of p53 by intracellular redistribution.

Author

Molinari AM, Bontempo P, Schiavone EM, Tortora V, Verdicchio MA, Napolitano M, Nola E, Moncharmont B, Medici N, Nigro V, Armetta I, Abbondanza C, and Puca GA

Subjects

Blotting, Western, Cyclin-Dependent Kinase Inhibitor p21, Cyclins biosynthesis, DNA Damage, Electrophoresis, Polyacrylamide Gel, Estradiol analogs & derivatives, Estradiol pharmacology, Estrogen Antagonists pharmacology, Female, Fulvestrant, G1 Phase, Humans, Immunohistochemistry, S Phase, Transfection, Tumor Cells, Cultured, Breast Neoplasms metabolism, Estradiol metabolism, Tumor Suppressor Protein p53 antagonists & inhibitors

Abstract

Estrogen treatment of MCF-7 cells grown in serum-free medium induced a modification of the intracellular distribution of p53 protein. Western blot analysis and immunofluorescence staining showed that p53 was localized in the nucleus of untreated cell and that after 48 h of hormone treatment, it was mostly localized in the cytoplasm. This effect was blocked by the antiestrogen ICI182,780. Intracellular redistribution of p53 was correlated to a reduced expression of the WAF1/CIP1 gene product and to the presence of degradation fragments of p53 in the cytosol. Estradiol treatment prevented the growth inhibition induced by oligonucleotide transfection, simulating DNA damage. This observation indicated that the wild-type p53 gene product present in the MCF-7 cell could be inactivated by estradiol through nuclear exclusion to permit the cyclin-dependent phosphorylation events leading to the G1-S transition. In addition, the estradiol-induced inactivation of p53 could be involved in the tumorigenesis of estrogen-dependent neoplasm.

Published

2000

41. The retinoblastoma-interacting zinc-finger protein RIZ is a downstream effector of estrogen action.

Author

Abbondanza C, Medici N, Nigro V, Rossi V, Gallo L, Piluso G, Belsito A, Roscigno A, Bontempo P, Puca AA, Molinari AM, Moncharmont B, and Puca GA

Subjects

Base Sequence, Cell Line, DNA Primers, Histone-Lysine N-Methyltransferase, Humans, Receptors, Estrogen metabolism, DNA-Binding Proteins, Estrogens physiology, Nuclear Proteins metabolism, Transcription Factors, Zinc Fingers

Abstract

Co-immunoprecipitation experiments in cell extract from cultured cells or target tissues indicated that estrogen receptor was complexed with the retinoblastoma binding protein RIZ in a ligand-dependent manner. Mapping of interaction sites indicated that in both proteins the same regions and motifs responsible for the interaction of transcriptional co-activator and nuclear receptors were involved. In cultured cells, estradiol induced a redistribution of RIZ protein within the nucleus and in the cytoplasm. A similar effect was produced in vivo, in prepuberal rat endometrium, by administration of a physiological dose of estradiol. Therefore, RIZ protein could be a specific effector of estrogen action downstream of the hormone-receptor interaction, presumably involved in proliferation control.

Published

2000

42. Interaction of vault particles with estrogen receptor in the MCF-7 breast cancer cell.

Author

Abbondanza C, Rossi V, Roscigno A, Gallo L, Belsito A, Piluso G, Medici N, Nigro V, Molinari AM, Moncharmont B, and Puca GA

Subjects

Animals, Estradiol pharmacology, Estrogens metabolism, Estrogens pharmacology, Female, HeLa Cells, Humans, Mice, Mice, Inbred BALB C, Neoplasm Proteins genetics, Precipitin Tests, RNA, Receptors, Cytoplasmic and Nuclear metabolism, Receptors, Estrogen genetics, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Ribonucleoproteins genetics, Tumor Cells, Cultured, Breast Neoplasms metabolism, Neoplasm Proteins metabolism, Receptors, Estrogen metabolism, Ribonucleoproteins metabolism, Vault Ribonucleoprotein Particles

Abstract

A 104-kD protein was coimmunoprecipitated with the estrogen receptor from the flowtrough of a phosphocellulose chromatography of MCF-7 cell nuclear extract. mAbs to this protein identified several cDNA clones coding for the human 104-kD major vault protein. Vaults are large ribonucleoprotein particles of unknown function present in all eukaryotic cells. They have a complex morphology, including several small molecules of RNA, but a single protein species, the major vault protein, accounts for >70% of their mass. Their shape is reminiscent of the nucleopore central plug, but no proteins of known function have been described to interact with them. Western blot analysis of vaults purified on sucrose gradient showed the presence of estrogen receptor co-migrating with the vault peak. The AER317 antibody to estrogen receptor coimmunoprecipitated the major vault protein and the vault RNA also in the 20,000 g supernatant fraction. Reconstitution experiments of estrogen receptor fragments with the major vault protein mapped the site of the interaction between amino acids 241 and 280 of human estrogen receptor, where the nuclear localization signal sequences are located. Estradiol treatment of cells increased the amount of major vault protein present in the nuclear extract and coimmunoprecipitated with estrogen receptor, whereas the anti-estrogen ICI182,780 had no effect. The hormone-dependent interaction of vaults with estrogen receptor was reproducible in vitro and was prevented by sodium molybdate. Antibodies to progesterone and glucocorticoid receptors were able to coimmunoprecipitate the major vault protein. The association of nuclear receptors with vaults could be related to their intracellular traffic.

Published

1998

43. 17 beta-hydroxysteroid dehydrogenase gene expression in human breast cancer cells: regulation of expression by a progestin.

Author

Poutanen M, Moncharmont B, and Vihko R

Subjects

17-Hydroxysteroid Dehydrogenases metabolism, Breast Neoplasms enzymology, Gene Expression Regulation, Neoplastic drug effects, Humans, Isoenzymes genetics, Placenta enzymology, Progesterone Congeners pharmacology, RNA, Messenger genetics, RNA, Neoplasm genetics, Receptors, Estrogen metabolism, Receptors, Progesterone metabolism, Tumor Cells, Cultured, 17-Hydroxysteroid Dehydrogenases genetics, Breast Neoplasms genetics, Pregnenediones pharmacology

Abstract

The expression of the 17 beta-hydroxysteroid dehydrogenase (17-HSD) gene in a series of human breast cancer cell lines was studied by Northern blot hybridization with a cDNA probe and by a time-resolved immunofluorometric assay using polyclonal antibodies against the enzyme protein. The 17-HSD enzyme protein concentration was measured in the 800 x g cell extract. A high concentration was measured in the BT-20 cell line, corresponding to one-fourth of the average concentration in placental tissue. Western blot analysis indicated that the antigen corresponded to a single Mr 35,000 band. In 2 other cell lines (MDA-MB-361 and T-47D), the 17-HSD protein concentration was much lower, but still measurable, whereas in the remaining 5 cell lines (HBL-100, MCF-7, MDA-MB-231, MDA-MB-468, and ZR-75-1) it was below the detection limit of the assay. Treatment of the cells for 5 days with the synthetic progestin, ORG2058, resulted in an increase of the 17-HSD protein concentration only in the T-47D cell line. By Northern blot analysis, a low level of 2.3-kilobase mRNA transcripts was detected in all 8 cell lines. In addition, a 1.3-kilobase 17-HSD mRNA was present in the samples from the 3 cell lines containing measurable amounts of 17-HSD protein in the cell extract, and the band intensities were proportional to the amount of protein measured with the immunofluorometric assay. Only in the T-47D cell line did progestin treatment correspond to an increased amount of the 17-HSD 1.3-kilobase mRNA. These results suggest that the 1.3-kilobase mRNA for 17-HSD is the form most closely associated with protein expression and is also the only form responding to the progestin induction of the 17-HSD gene.

Published

1992

44. Comparison of estrogen receptors in hormone-dependent and hormone-independent Grunder strain mouse mammary tumors.

Author

Moncharmont B, Ramp G, De Goeij CC, and Sluyser M

Subjects

Animals, Centrifugation, Density Gradient, Cytosol enzymology, Cytosol metabolism, Electrophoresis, Polyacrylamide Gel, Endopeptidases metabolism, Estradiol metabolism, Female, Mammary Neoplasms, Experimental pathology, Mice, Mice, Inbred Strains, Neoplasm Transplantation, Neoplasms, Hormone-Dependent pathology, Mammary Neoplasms, Experimental metabolism, Neoplasms, Hormone-Dependent metabolism, Receptors, Estrogen metabolism

Abstract

Hormone-dependent (HD) Grunder strain mouse mammary carcinomas contain a 65-kDa estrogen receptor (ER) with minor amounts of 50- and 35-kDa components which apparently still contain the intact hormone-binding (COOH-terminal) domain. When the HD tumors lose their hormonal dependence during serial transplantation, the hormone-independent (HI) transplants show an increase in 50- and 35-kDa components relative to 65-kDa ER. In HI transplants of three of five tumor lines studied (TSl 85, 86, and 106), the 65-kDa receptor was entirely replaced by 50- and 35-kDa receptors, whereas in the two other lines (TSl 101 and 104) there usually were about equal amounts of 65- and 50-kDa ERs. No difference was found between ERs of HD and HI tumors in affinity for estradiol, steroid specificity, or immunoreactivity for the monoclonal antibody JS34/32. Estrogen stimulation of HI tumors did not increase the concentration of progesterone receptor in the tumor tissue, indicating that ER in these tumors was not functional in enhancing progesterone receptor. Incubation of 65-kDa ER with HI tumor cytosol or combined homogenization of HD and HI tumor tissue did not cause degradation of 65-kDa ER. alpha-Chymotrypsin-like protease activity generally was lower in HI than in HD tumor cytosols, indicating that the lower molecular size of ER in HI tumors cannot be attributed to the increased level of this protease activity.

Published

1991

45. Immunocytochemical demonstration of estrogen receptors by monoclonal antibodies in human breast cancer: correlation with estrogen receptor assay by dextran-coated charcoal method.

Author

Marchetti E, Querzoli P, Moncharmont B, Parikh I, Bagni A, Marzola A, Fabris G, and Nenci I

Subjects

Charcoal, Dextrans, Female, Histocytochemistry, Humans, Immunologic Techniques, Methods, Antibodies, Monoclonal, Breast Neoplasms analysis, Receptors, Estrogen analysis

Abstract

Immunocytochemical demonstration of estrogen receptors in 115 human breast cancer specimens was performed using mouse monoclonal antibodies against estrogen receptor and avidin-biotin as the displaying system. The antibody indicated a highly heterogeneous endowment of neoplastic cells with estrogen receptor at both nuclear and cytoplasmic levels. The percentage of labeled cells within each tumor specimen was recorded to compare this immunocytochemical assay with the biochemical assay of estrogen receptors by the dextran-coated charcoal method. A significant correlation was observed between these two assays. The present results show that estrogen receptors can be confidently demonstrated at the single cell level, thus providing additional information to quantitative biochemical assays. Their prognostic and therapeutic predictive powers may be usefully integrated, particularly in view of the heterogeneous distribution of receptors among cancer cells.

Published

1987