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1. A Methodology for the Derivation and Verification of Use Cases for Product Lines

Author

Fantechi, A., Gnesi, S., Lami, G., Nesti, E., Hutchison, David, editor, Kanade, Takeo, editor, Kittler, Josef, editor, Kleinberg, Jon M., editor, Mattern, Friedemann, editor, Mitchell, John C., editor, Naor, Moni, editor, Nierstrasz, Oscar, editor, Pandu Rangan, C., editor, Steffen, Bernhard, editor, Sudan, Madhu, editor, Terzopoulos, Demetri, editor, Tygar, Dough, editor, Vardi, Moshe Y., editor, Weikum, Gerhard, editor, and Nord, Robert L., editor

Published
2004
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5. Thrombophilic syndrome associated to phenotypic resistance to activated protein C in postmenopausal women

Author

CASERTA L., CASERTA R., PERRICONE F., NESTI E., SESSA M., TAGLIAFERRI A., DE FRANCESCO F., DE LUCIA D., PANARIELLO S., TORELLA, Marco, Caserta, L., Caserta, R., Torella, Marco, Perricone, F., Nesti, E., Sessa, M., Tagliaferri, A., DE FRANCESCO, F., DE LUCIA, D., and Panariello, S.

Subjects
Thrombophilic syndrome, activated protein C, menopause
Abstract

HRT appears to be associated to a shift in the procoagulant-anticoagulant balance towards a procoagulant state. The changes in hemostatic system could explain the increased risk of VTE in healthy postmenopausal women during HRT, nevertheless this risk could be higher in women known to have a congenital or acquired thrombophilic state.

Published
2004

7. A methodology for the derivation and verification of use cases for product lines

Author

Fantechi A., Gnesi S., Lami G., and Nesti E.

Subjects
Product lines
Abstract

In this paper, we present a methodology to express, in a formal way, the requirements of products belonging to a product line. We relied on a formalism allowing the representation of variabilities at the family level and the instantiation of them in order to move to the requirements of a single product. The proposed methodology also allows the formalization of the family constraints to be taken into account for the construction of the products belonging to it, along with the verification of the compliance to those constraints of a single product requirements document. This approach is promising due to its simplicity and effectiveness for being supported by automatic tools.

Published
2004

8. New insights into the regulation of ion channels by integrins

Author

Becchetti, A, Pillozzi, S, Morini, R, Nesti, E, Arcangeli, A, Becchetti, A, Pillozzi, S, Morini, R, Nesti, E, and Arcangeli, A

Abstract

By controlling cell adhesion to the extracellular matrix, integrin receptors regulate processes as diverse as cell migration, proliferation, differentiation, apoptosis, and synaptic stability. Because the underlying mechanisms are generally accompanied by changes in transmembrane ion flow, a complex interplay occurs between integrins, ion channels, and other membrane transporters. This reciprocal interaction regulates bidirectional signal transduction across the cell surface and may take place at all levels of control, from transcription to direct conformational coupling. In particular, it is becoming increasingly clear that integrin receptors form macromolecular complexes with ion channels. Besides contributing to the membrane localization of the channel protein, the integrin/channel complex can regulate a variety of downstream signaling pathways, centered on regulatory proteins like tyrosine kinases and small GTPases. In turn, the channel protein usually controls integrin activation and expression. We review some recent advances in the field, with special emphasis on hematology and neuroscience. Some oncological implications are also discussed. © 2010 Elsevier Inc.

Published
2010

9. New insights into the regulation of ion channels by integrins

Author

Kwang Jeon, Becchetti, A, Pillozzi, S, Morini, R, Nesti, E, Arcangeli, A, Kwang Jeon, Becchetti, A, Pillozzi, S, Morini, R, Nesti, E, and Arcangeli, A

Abstract

By controlling cell adhesion to the extracellular matrix, integrin receptors regulate processes as diverse as cell migration, proliferation, differentiation, apoptosis, and synaptic stability. Because the underlying mechanisms are generally accompanied by changes in transmembrane ion flow, a complex interplay occurs between integrins, ion channels, and other membrane transporters. This reciprocal interaction regulates bidirectional signal transduction across the cell surface and may take place at all levels of control, from transcription to direct conformational coupling. In particular, it is becoming increasingly clear that integrin receptors form macromolecular complexes with ion channels. Besides contributing to the membrane localization of the channel protein, the integrin/channel complex can regulate a variety of downstream signaling pathways, centered on regulatory proteins like tyrosine kinases and small GTPases. In turn, the channel protein usually controls integrin activation and expression. We review some recent advances in the field, with special emphasis on hematology and neuroscience. Some oncological implications are also discussed. © 2010 Elsevier Inc.

Published
2010

10. Stable GM3 Lactone Mimetic Raises Antibodies Specific for the Antigens Expressed on Melanoma Cells

Author

Arcangeli, A, Toma, L, Contiero, L, Crociani, O, Legnani, L, Lunghi, C, Nesti, E, Moneti, G, Richichi, B, Nativi, C, Arcangeli Annarosa, TOMA, LUCIO, Contiero Luca, Crociani Olivia, LEGNANI, LAURA, Lunghi Carlotta, Nesti Elisa, Moneti Gloriano, Richichi Barbara, Nativi Cristina, Arcangeli, A, Toma, L, Contiero, L, Crociani, O, Legnani, L, Lunghi, C, Nesti, E, Moneti, G, Richichi, B, Nativi, C, Arcangeli Annarosa, TOMA, LUCIO, Contiero Luca, Crociani Olivia, LEGNANI, LAURA, Lunghi Carlotta, Nesti Elisa, Moneti Gloriano, Richichi Barbara, and Nativi Cristina

Abstract

Immunotherapy of tumors and of melanoma in particular has a long history, and recently this therapeutic approach found a reliable scientific rationale. This biological therapy aims to teach the patient’s immune system to recognize the antigens expressed on tumor cells and destroy them, leaving normal cells intact. The success of this therapy highly depends on the selection of target antigens that are essential for tumors growth and progression. The overexpression of GM3 ganglioside 1 and especially the expression of its metabolite GM3 lactone 2 characterize murine and human melanomas, playing an important role in tumor progression and making such self-antigens potential targets for the immunotherapy of these neoplasms. Although more immunogenic than its precursor, GM3 lactone 2 is unsuitable to be used in immunotherapy as a melanoma-associated antigen (MAA) because it is unstable under physiological conditions. We designed and synthesized the hydrolytically stable mimetic 3, which is remarkably simpler than the native lactone 2; after conjugation of 3 to the protein carrier keyhole-limpet hemocyanin (KLH), the obtained glycoprotein 5 was used as the immunogen in vivo to successfully elicit specific antimelanoma antibodies. In fact, no appreciable binding to GM1 was observed. Capitalizing on the stability and on the reduced structural complexity of mimetic 3, the immunostimulant 5 we report represents a new promising synthetic glycoconjugate for the immunotherapy of melanoma.

Published
2010

14. Stable GM3 Lactone Mimetic Raises Antibodies Specific for the Antigens Expressed on Melanoma Cells

Author

Carlotta Lunghi, Barbara Richichi, Luca Contiero, Annarosa Arcangeli, Cristina Nativi, Elisa Nesti, Gloriano Moneti, Olivia Crociani, Lucio Toma, Laura Legnani, Arcangeli, A, Toma, L, Contiero, L, Crociani, O, Legnani, L, Lunghi, C, Nesti, E, Moneti, G, Richichi, B, Nativi, C, Arcangeli A., Toma L., Contiero L., Crociani O., Legnani L., Lunghi C., Nesti E., Moneti G., Richichi B., and Nativi C.

Subjects
glycoprotein, Immunogen, medicine.medical_treatment, Pharmaceutical Science, Immunostimulant, Antigen-Antibody Reactions, Mice, Antibody Specificity, antibody, keyhole-limpet hemocyanin, GM3 lactone, Carbohydrate Conformation, Melanoma, biology, Chemistry, unclassified drug, Biochemistry, lactone, Immunotherapy, hemocyanin, Antibody, ganglioside GM3 lactone, Biotechnology, medicine.drug_class, Glycoconjugate, keyhole limpet hemocyanin, Biomedical Engineering, Bioengineering, Antibodies, antigen, Immune system, Antigen, medicine, Animals, G(M3) Ganglioside, Humans, lactone derivative, Computer Simulation, ganglioside GM3, Pharmacology, Molecular Mimicry, Organic Chemistry, Ganglioside mimetic, medicine.disease, Tumor progression, drug derivative, Hemocyanins, biology.protein
Abstract

Immunotherapy of tumors and of melanoma in particular has a long history, and recently this therapeutic approach found a reliable scientific rationale. This biological therapy aims to teach the patients immune system to recognize the antigens expressed on tumor cells and destroy them, leaving normal cells intact. The success of this therapy highly depends on the selection of target antigens that are essential for tumors growth and progression. The overexpression of GM3 ganglioside 1 and especially the expression of its metabolite GM3 lactone 2 characterize murine and human melanomas, playing an important role in tumor progression and making such self-antigens potential targets for the immunotherapy of these neoplasms. Although more immunogenic than its precursor, GM3 lactone 2 is unsuitable to be used in immunotherapy as a melanoma-associated antigen (MAA) because it is unstable under physiological conditions. We designed and synthesized the hydrolytically stable mimetic 3, which is remarkably simpler than the native lactone 2; after conjugation of 3 to the protein carrier keyhole-limpet hemocyanin (KLH), the obtained glycoprotein 5 was used as the immunogen in vivo to successfully elicit specific antimelanoma antibodies. In fact, no appreciable binding to GM1 was observed. Capitalizing on the stability and on the reduced structural complexity of mimetic 3, the immunostimulant 5 we report represents a new promising synthetic glycoconjugate for the immunotherapy of melanoma. © 2010 American Chemical Society.

Published
2010

15. New insights into the regulation of ion channels by integrins

Author

Elisa Nesti, Serena Pillozzi, Raffaella Morini, Annarosa Arcangeli, Andrea Becchetti, Kwang Jeon, Becchetti, A, Pillozzi, S, Morini, R, Nesti, E, and Arcangeli, A

Subjects
Cell surface receptor, BIO/09 - FISIOLOGIA, Synaptic plasticity, Integrin, biology.protein, GTPase, Signal transduction, Biology, Cell adhesion, Transmembrane protein, Ion channel, cell adhesion, extracellular matrix, hERG, leukemia, lymphoma, migration, synaptic plasticity, Cell biology
Abstract

By controlling cell adhesion to the extracellular matrix, integrin receptors regulate processes as diverse as cell migration, proliferation, differentiation, apoptosis, and synaptic stability. Because the underlying mechanisms are generally accompanied by changes in transmembrane ion flow, a complex interplay occurs between integrins, ion channels, and other membrane transporters. This reciprocal interaction regulates bidirectional signal transduction across the cell surface and may take place at all levels of control, from transcription to direct conformational coupling. In particular, it is becoming increasingly clear that integrin receptors form macromolecular complexes with ion channels. Besides contributing to the membrane localization of the channel protein, the integrin/channel complex can regulate a variety of downstream signaling pathways, centered on regulatory proteins like tyrosine kinases and small GTPases. In turn, the channel protein usually controls integrin activation and expression. We review some recent advances in the field, with special emphasis on hematology and neuroscience. Some oncological implications are also discussed. © 2010 Elsevier Inc.

Published
2010

16. L’ANALGESIA SUBARACNOIDEA NEL TRAVAGLIO DI PARTO AVANZATO

Author

E. VILLANO, M. IANNOTTI, M. C. PACE, E. GRELLA, E. NESTI, C. PAROLISE, C. AURILIO, PASSAVANTI, Maria Beatrice, Villano, E., Iannotti, M., Pace, M. C., Passavanti, Maria Beatrice, Grella, E., Nesti, E., Parolise, C., and Aurilio, C.

Published
2001

17. Live rubella vectors can express native HIV envelope glycoproteins targeted by broadly neutralizing antibodies and prime the immune response to an envelope protein boost.

Author

Virnik K, Nesti E, Dail C, Scanlan A, Medvedev A, Vassell R, McGuire AT, Stamatatos L, and Berkower I

Subjects
Animals, Antibodies, Neutralizing blood, CD4-Positive T-Lymphocytes immunology, HIV Antibodies blood, HIV Infections immunology, HIV-1, Immunization, Secondary, Macaca mulatta, Recombinant Proteins immunology, Vaccines, Attenuated immunology, AIDS Vaccines immunology, Antibodies, Neutralizing immunology, HIV Envelope Protein gp120 immunology, HIV Infections prevention & control, Rubella virus
Abstract

Following HIV infection, most people make antibodies to gp120 and gp41, yet only a few make broadly neutralizing antibodies that target key antigenic sites on the envelope glycoproteins. The induction of broadly neutralizing antibodies by immunization remains a major challenge of HIV vaccine research. Difficulties include: variable protein sequence, epitopes that depend on the native conformation, glycosylation that conceals key antigenic determinants, and the assembly of Env trimers that mimic viral spikes. In addition, more potent immunogens may be needed to initiate the response of germline antibody precursors and drive B cell maturation toward antibodies with broad neutralizing activity. We have expressed HIV Env glycoproteins by incorporation into live attenuated rubella viral vectors. The rubella vaccine strain RA27/3 has demonstrated its safety and potency in millions of children. As a vector, it has elicited potent and durable immune responses in macaques to SIV Gag vaccine inserts. We now find that rubella/env vectors can stably express Env core derived glycoproteins ranging in size up to 363 amino acids from HIV clade C strain 426c. The expressed Env glycoproteins bind broadly neutralizing antibodies that target the native CD4 binding site. The vectors grew well in rhesus macaques, and they elicited a vaccine "take" in all animals, as measured by anti-rubella antibodies. By themselves, the vectors elicited modest antibody titers to the Env insert. But the combination of rubella/env prime followed by a homologous protein boost gave a strong response. Neutralizing antibodies appeared gradually after multiple vaccine doses. The vectors will be useful for testing new vaccine inserts and immunization strategies under optimized conditions of vector growth and protein expression., (Published by Elsevier Ltd.)

Published
2018
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18. Expression of complete SIV p27 Gag and HIV gp120 engineered outer domains targeted by broadly neutralizing antibodies in live rubella vectors.

Author

Virnik K, Nesti E, Dail C, Hockenbury M, Ni Y, Felber BK, Schief WR, and Berkower I

Subjects
AIDS Vaccines genetics, AIDS Vaccines immunology, Animals, Antibodies, Viral immunology, Gene Products, gag genetics, Genetic Vectors, HIV Envelope Protein gp120 genetics, HIV Infections immunology, HIV Infections prevention & control, Immunization, Immunogenicity, Vaccine, Macaca mulatta, Rubella Vaccine genetics, Rubella Vaccine immunology, Rubella virus immunology, SAIDS Vaccines genetics, SAIDS Vaccines immunology, Simian Immunodeficiency Virus immunology, Vaccines, Attenuated administration & dosage, Vaccines, Attenuated immunology, Antibodies, Neutralizing immunology, Gene Products, gag immunology, HIV Envelope Protein gp120 immunology, Rubella virus genetics, Simian Immunodeficiency Virus genetics
Abstract

Infection with HIV or SIV often elicits a potent immune response to viral antigens. This includes T cells and antibodies specific for Gag and Env antigens. In contrast, when given as a vaccine, the same antigens have been weak immunogens, unable to elicit antibodies with comparable titer, durability, or neutralizing activity. We have used the live attenuated rubella vaccine strain RA27/3 as a viral vector to express HIV and SIV antigens. By mimicking an HIV infection, these vectors could elicit stronger and more durable immunity to HIV antigens. The vectors are based on the licensed rubella vaccine strain, which has demonstrated safety and potency in millions of children. One or two doses protect for life against rubella infection. The question was whether rubella vectors could similarly enhance the immunogenicity of a foreign vaccine insert. We have previously reported that rubella vectors can express small protein antigens in vitro and in vivo, where they elicit a strong immune response to the vaccine insert. The vectors have now expressed larger vaccine inserts that include epitope-rich fragments of the Gag matrix and capsid proteins (aa 41-211) or the complete p27 capsid protein with p2 (aa 136-381). These vectors have elicited a robust and durable immune response to Gag in rhesus macaques. This size range also encompasses the engineered outer domain (eOD) of HIV envelope gp120 (172 amino acids). The rubella/eOD-GT6 and GT8 vectors stably expressed glycoproteins that bind germline precursors and mature forms of VRC01-class broadly neutralizing antibodies. These vectors potentially could be used as part of a sequential immunization strategy to initiate the production of broadly neutralizing antibodies., (Published by Elsevier Ltd.)

Published
2017
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19. Harnessing the master transcriptional repressor REST to reciprocally regulate neurogenesis.

Author

Nesti E

Abstract

Neurogenesis begins in embryonic development and continues at a reduced rate into adulthood in vertebrate species, yet the signaling cascades regulating this process remain poorly understood. Plasma membrane-initiated signaling cascades regulate neurogenesis via downstream pathways including components of the transcriptional machinery. A nuclear factor that temporally regulates neurogenesis by repressing neuronal differentiation is the repressor element 1 (RE1) silencing transcription (REST) factor. We have recently discovered a regulatory site on REST that serves as a molecular switch for neuronal differentiation. Specifically, C-terminal domain small phosphatase 1, CTDSP1, present in non-neuronal cells, maintains REST activity by dephosphorylating this site. Reciprocally, extracellular signal-regulated kinase, ERK, activated by growth factor signaling in neural progenitors, and peptidylprolyl cis/trans isomerase Pin1, decrease REST activity through phosphorylation-dependent degradation. Our findings further resolve the mechanism for temporal regulation of REST and terminal neuronal differentiation. They also provide new potential therapeutic targets to enhance neuronal regeneration after injury.

Published
2015
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20. C-terminal domain small phosphatase 1 and MAP kinase reciprocally control REST stability and neuronal differentiation.

Author

Nesti E, Corson GM, McCleskey M, Oyer JA, and Mandel G

Subjects
Animals, Chickens, Chromatin metabolism, Epidermal Growth Factor metabolism, Green Fluorescent Proteins metabolism, HEK293 Cells, Humans, MAP Kinase Signaling System, Mice, Mutation genetics, NIMA-Interacting Peptidylprolyl Isomerase, PC12 Cells, Peptides metabolism, Peptidylprolyl Isomerase metabolism, Phosphorylation, Phosphoserine metabolism, Protein Binding, Protein Stability, Proteolysis, Rats, beta-Transducin Repeat-Containing Proteins metabolism, ras Proteins metabolism, Cell Differentiation, Extracellular Signal-Regulated MAP Kinases metabolism, Neurons cytology, Neurons metabolism, Nuclear Proteins metabolism, Phosphoprotein Phosphatases metabolism, Repressor Proteins metabolism
Abstract

The repressor element 1 (RE1) silencing transcription factor (REST) in stem cells represses hundreds of genes essential to neuronal function. During neurogenesis, REST is degraded in neural progenitors to promote subsequent elaboration of a mature neuronal phenotype. Prior studies indicate that part of the degradation mechanism involves phosphorylation of two sites in the C terminus of REST that require activity of beta-transducin repeat containing E3 ubiquitin protein ligase, βTrCP. We identify a proline-directed phosphorylation motif, at serines 861/864 upstream of these sites, which is a substrate for the peptidylprolyl cis/trans isomerase, Pin1, as well as the ERK1/2 kinases. Mutation at S861/864 stabilizes REST, as does inhibition of Pin1 activity. Interestingly, we find that C-terminal domain small phosphatase 1 (CTDSP1), which is recruited by REST to neuronal genes, is present in REST immunocomplexes, dephosphorylates S861/864, and stabilizes REST. Expression of a REST peptide containing S861/864 in neural progenitors inhibits terminal neuronal differentiation. Together with previous work indicating that both REST and CTDSP1 are expressed to high levels in stem cells and down-regulated during neurogenesis, our results suggest that CTDSP1 activity stabilizes REST in stem cells and that ERK-dependent phosphorylation combined with Pin1 activity promotes REST degradation in neural progenitors.

Published
2014
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21. Stable GM3 lactone mimetic raises antibodies specific for the antigens expressed on melanoma cells.

Author

Arcangeli A, Toma L, Contiero L, Crociani O, Legnani L, Lunghi C, Nesti E, Moneti G, Richichi B, and Nativi C

Subjects
Animals, Antibodies chemistry, Antibody Specificity, Antigen-Antibody Reactions, Carbohydrate Conformation, Computer Simulation, G(M3) Ganglioside chemistry, G(M3) Ganglioside genetics, G(M3) Ganglioside immunology, Hemocyanins chemistry, Hemocyanins immunology, Humans, Immunotherapy, Melanoma genetics, Melanoma therapy, Mice, Molecular Mimicry genetics, Antibodies immunology, G(M3) Ganglioside analogs & derivatives, Melanoma immunology, Molecular Mimicry immunology
Abstract

Immunotherapy of tumors and of melanoma in particular has a long history, and recently this therapeutic approach found a reliable scientific rationale. This biological therapy aims to teach the patient's immune system to recognize the antigens expressed on tumor cells and destroy them, leaving normal cells intact. The success of this therapy highly depends on the selection of target antigens that are essential for tumors growth and progression. The overexpression of GM(3) ganglioside 1 and especially the expression of its metabolite GM(3) lactone 2 characterize murine and human melanomas, playing an important role in tumor progression and making such self-antigens potential targets for the immunotherapy of these neoplasms. Although more immunogenic than its precursor, GM(3) lactone 2 is unsuitable to be used in immunotherapy as a melanoma-associated antigen (MAA) because it is unstable under physiological conditions. We designed and synthesized the hydrolytically stable mimetic 3, which is remarkably simpler than the native lactone 2; after conjugation of 3 to the protein carrier keyhole-limpet hemocyanin (KLH), the obtained glycoprotein 5 was used as the immunogen in vivo to successfully elicit specific antimelanoma antibodies. In fact, no appreciable binding to GM(1) was observed. Capitalizing on the stability and on the reduced structural complexity of mimetic 3, the immunostimulant 5 we report represents a new promising synthetic glycoconjugate for the immunotherapy of melanoma.

Published
2010
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22. New insights into the regulation of ion channels by integrins.

Author

Becchetti A, Pillozzi S, Morini R, Nesti E, and Arcangeli A

Subjects
Animals, Cell Movement physiology, Central Nervous System anatomy & histology, Central Nervous System physiology, Hematologic Neoplasms metabolism, Hematopoietic Stem Cells physiology, Humans, Ion Channels chemistry, Ion Channels classification, Ion Channels genetics, Microglia metabolism, Neuronal Plasticity physiology, Neurotransmitter Agents metabolism, Signal Transduction physiology, Synapses metabolism, Integrins metabolism, Ion Channel Gating physiology, Ion Channels metabolism
Abstract

By controlling cell adhesion to the extracellular matrix, integrin receptors regulate processes as diverse as cell migration, proliferation, differentiation, apoptosis, and synaptic stability. Because the underlying mechanisms are generally accompanied by changes in transmembrane ion flow, a complex interplay occurs between integrins, ion channels, and other membrane transporters. This reciprocal interaction regulates bidirectional signal transduction across the cell surface and may take place at all levels of control, from transcription to direct conformational coupling. In particular, it is becoming increasingly clear that integrin receptors form macromolecular complexes with ion channels. Besides contributing to the membrane localization of the channel protein, the integrin/channel complex can regulate a variety of downstream signaling pathways, centered on regulatory proteins like tyrosine kinases and small GTPases. In turn, the channel protein usually controls integrin activation and expression. We review some recent advances in the field, with special emphasis on hematology and neuroscience. Some oncological implications are also discussed., (Copyright 2010 Elsevier Inc. All rights reserved.)

Published
2010
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23. Endocytosis as a mechanism for tyrosine kinase-dependent suppression of a voltage-gated potassium channel.

Author

Nesti E, Everill B, and Morielli AD

Subjects
Amino Acid Substitution, Animals, Antibodies, Monoclonal, Carbachol pharmacology, Cell Line, Dynamins genetics, Dynamins metabolism, Endocytosis, Humans, In Vitro Techniques, Kv1.2 Potassium Channel, Mutagenesis, Site-Directed, Potassium Channels, Voltage-Gated genetics, Potassium Channels, Voltage-Gated metabolism, Rats, Recombinant Proteins antagonists & inhibitors, Recombinant Proteins genetics, Recombinant Proteins metabolism, Transfection, Vanadates pharmacology, Potassium Channels, Voltage-Gated antagonists & inhibitors, Protein-Tyrosine Kinases metabolism
Abstract

The voltage-gated potassium channel Kv1.2 undergoes tyrosine phosphorylation-dependent suppression of its ionic current. However, little is known about the physical mechanism behind that process. We have found that the Kv1.2 alpha-subunit protein undergoes endocytosis in response to the same stimuli that evoke suppression of Kv1.2 ionic current. The process is tyrosine phosphorylation-dependent because the same tyrosine to phenylalanine mutation in the N-terminus of Kv1.2 that confers resistance to channel suppression (Y132F) also confers resistance to channel endocytosis. Overexpression of a dominant negative form of dynamin blocked stimulus-induced Kv1.2 endocytosis and also blocked suppression of Kv1.2 ionic current. These data indicate that endocytosis of Kv1.2 from the cell surface is a key mechanism for channel suppression by tyrosine kinases.

Published
2004
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24. [Thrombophilic syndrome associated to phenotypic resistance to activated protein C in postmenopausal women].

Author

Caserta L, Caserta R, Torella M, Perricone F, Nesti E, Sessa M, Tagliaferri A, De Francesco F, De Lucia D, and Panariello S

Subjects
Activated Protein C Resistance genetics, Adult, Female, Humans, Middle Aged, Phenotype, Syndrome, Activated Protein C Resistance chemically induced, Estrogen Replacement Therapy adverse effects, Postmenopause, Progestins adverse effects, Thrombophilia chemically induced
Abstract

Aim: Hormone replacement therapy (HRT) may reduce the risk of cardiovascular events in healthy postmenopausal women. However recent studies suggest a 2-4 fold increased risk of idiopathic venous thromboembolism (VTE) among users of HRT. Our aim was to evaluate the overall effect of HRT on hemostatic variables probably related to increased VTE risk reported in epidemiological studies., Methods: Therefore, 100 healthy postmenopausal women aged 45-60 years divided into 50 HRT non-users and 50 HRT users were examined. The authors assayed on the automated coagulometer ACL7000 (Instrumentation Laboratory, Milan) the procoagulant proteins: factor VIII (VIII:C) and factor VII (VII:C); the natural anticoagulant proteins: antithrombin (ATIII), protein C (PC), protein S (PS) and the resistance to anticoagulant action of activated protein C (APC-Resistance). The free tissue factor pathway inhibitor (TFPI) was measured with an ELISA method (Diagnostica Stagò; France, Roche). The in vivo coagulation and fibrinolysis activation was evaluated by the assays of prothrombin fragment 1+2 (F1+2) and plasmin- antiplasmin complexes (PAP) using ELISA techniques., Results: Increased levels of FVIII:C and FVII:C were observed in HRT users and HRT non-users women compared to controls (FVIII:C= 126+/-58%, 120+/-59% vs 85+/-15% p=0.0001; FVII: C 113+/-23%, 103+/-19% vs 90+/-16% p=0.0001). The activation peptides were significantly different compared to those found in control subjects; higher values were observed in HRT users compared to HRT non-users (F1+2=1.11+/-0.44 nM, 077+/-0.31 nM vs 0.45+/-0.35 p=0.00001; P-AP= 606+/-406 ng/ml, 514+/-205 ng/ml vs 235+/-59 p=0.0001). The ATIII and the PC were similar among the 3 different groups of subjects, but reduced levels of PS were observed in HRT users (PS 93+/-23%, 105+/-22% vs 109+/-12 p=0.0001). The mean normalized APC sensitivity ratio (APC-SR) was lower in the two populations of women as compared with that of controls (nAPC-SR 1.02+/-0.7, 1.02+/-0.8 vs 1.1+/-25 p=0.02). The values of free TFPI were reduced in HRT users compared to HRT non-users (9.1+/-1.9 ng/ml, 10.1+/-2.3 ng/ml vs 4.6+/-1.5 ng/ml p<0.0001)., Conclusion: HRT appears to be associated to a shift in the procoagulant-anticoagulant balance towards a procoagulant state. The changes in hemostatic system could explain the increased risk of VTE in healthy postmenopausal women during HRT, nevertheless this risk could be higher in women known to have a congenital or acquired thrombophilic state.

Published
2004

25. Tyrosine phosphorylation of Kv1.2 modulates its interaction with the actin-binding protein cortactin.

Author

Hattan D, Nesti E, Cachero TG, and Morielli AD

Subjects
Actins metabolism, Animals, Brain Chemistry, Cell Fractionation, Cell Line, Cortactin, Cytoskeleton metabolism, Humans, Immunohistochemistry, Kv1.2 Potassium Channel, Mutagenesis, Site-Directed, Oocytes physiology, Patch-Clamp Techniques, Phosphorylation, Potassium Channels genetics, Protein Binding, Protein Structure, Tertiary, Rats, Receptor, Muscarinic M1, Receptors, Muscarinic metabolism, Recombinant Fusion Proteins metabolism, Xenopus laevis, Microfilament Proteins metabolism, Potassium Channels metabolism, Potassium Channels, Voltage-Gated, Tyrosine metabolism
Abstract

Tyrosine phosphorylation evokes functional changes in a variety of ion channels. Modulation of the actin cytoskeleton also affects the function of some channels. Little is known about how these avenues of ion channel regulation may interact. We report that the potassium channel Kv1.2 associates with the actin-binding protein cortactin and that the binding is modulated by tyrosine phosphorylation. Immunocytochemical and biochemical analyses show that Kv1.2 and cortactin co-localize to the cortical actin cytoskeleton at the leading edges of the cell. Binding assays using purified recombinant proteins reveal a 19-amino acid span within the carboxyl terminus of Kv1.2 that is necessary for direct cortactin binding. Phosphorylation of specific tyrosines within the C terminus of Kv1.2 attenuates that binding. In HEK293 cells, activation of the M1 muscarinic acetylcholine receptor evokes tyrosine phosphorylation-dependent suppression of Kv1.2 ionic current. We show that M1 receptor activation also reduces the interaction of cortactin with Kv1.2 and that mutant Kv1.2 channels deficient for cortactin binding exhibit strongly attenuated ionic current. These results demonstrate a dynamic, phosphorylation-dependent interaction between Kv1.2 and the actin cytoskeleton-binding protein cortactin and suggest a role for that interaction in the regulation of Kv1.2 ionic current.

Published
2002
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26. [Small ovarian cysts in postmenopause: assessment of their malignant potential with vaginal ultrasonography and tumor marker Ca125 titration].

Author

Caserta R, Nesti E, Caserta L, Guerriero V, Di Francesco D, and Panariello S

Subjects
Aged, Female, Humans, Middle Aged, Ultrasonography, CA-125 Antigen blood, Ovarian Cysts blood, Ovarian Cysts diagnostic imaging, Postmenopause, Precancerous Conditions blood, Precancerous Conditions diagnostic imaging
Abstract

Background: The aim of this study was to determine the risk of malignancy in cystic ovarian tumors < 10 cm in diameter in asymptomatic postmenopausal women., Methods: All cystic ovarian tumors, detected by abdominal and transvaginal sonography screening, in asymptomatic postmenopausal women were evaluated with respect to size and morphology. Follow-up data were available both on patients undergoing surgery and on those who elected to be followed without operative intervention. Titration of the tumoral marker Ca125 was carried out, too., Results: Unilocular cystic tumors were detected in 32 of 352 postmenopausal patients (9%), of 45-65 years of age arrived at the "Centre for diagnosis and therapy of menopausal diseases" of the III Divisione di Ginecologia e Ostetricia della Seconda Università degli Studi di Napoli from the 1st January to the 31st December 1999. All tumors were < 10 cm in diameter and 98% were < 5 cm in diameter; just one tumor was hardly > 5 cm in diameter (5.8), 14 of these cystic ovarian tumors (49%) resolved spontaneously within 60 days while 18 (51%) persisted. Seven patients with persistent cystic ovarian tumors underwent operative tumor removal. Five of these patients had serous cystadenoma and 2 other women had cystoadenofibroma. Not even one case of ovarian carcinoma was found in this group. The remaining 11 patients with unilocular cystic ovarian tumors underwent sonography control every 3 months for one year and no one of these patients developed ovarian carcinoma. In all these patients the dosage of the tumoral marker Ca125 remained under the suspicious threshold of malignant ovaric tumor (Ca125 = 35 U/ml)., Conclusions: Unilocular cystic ovarian tumors < 5 cm in diameter in asymptomatic postmenopausal women were associated with minimal risk for ovarian cancer. In contrast, complex ovarian cysts wall abnormalities or solid areas are associated with a significant risk for malignancy. These date are important in determining therapeutic optimal strategies in these patients.

Published
2001

27. [Relation between asymmetrical hypertrophy of the interventricular septum and plasma levels of catecholamines in normotensive chronic uremic patients undergoing hemodialysis treatment].

Author

Bernardi D, Bernini L, Cini G, Nesti E, Brandinelli Geri A, Ferreri A, Urti DA, and Bonechi I

Subjects
Adult, Aged, Cardiomegaly blood, Chronic Disease, Echocardiography, Female, Humans, Male, Middle Aged, Renal Dialysis, Uremia blood, Uremia therapy, Cardiomegaly complications, Epinephrine blood, Heart Septum pathology, Norepinephrine blood, Uremia complications
Abstract

Sympathetic-adrenergic activity has been evaluated in 23 chronic uremic, normotensive patients on regular hemodialysis, 7 of which (30.4%) with M-mode and bidimensional echocardiographic finding of asymmetric septal hypertrophy. The sympathetic function has been assessed by measuring arterial plasma norepinephrine and epinephrine levels before and after postural activation, just before and after dialysis. After dialysis, standing caused a significant increase of plasma norepinephrine levels in patients with asymmetric septal hypertrophy in comparison with patients without asymmetric septal hypertrophy and with the control non uremic group. Moreover, a significant decrease in blood pressure and a sharp heart rate increase were noted in the patients without asymmetric septal hypertrophy, whereas mean blood pressure and heart rate were unchanged in the patients with asymmetric septal hypertrophy. These results suggest that increased plasma norepinephrine concentration may have a role in the development of interventricular septal hypertrophy.

Published
1984

28. Carotid artery atherosclerotic disease assessed by flow velocity wave form analysis in hemodialyzed normotensive and hypertensive patients.

Author

Bernardi D, Ferreri A, Moretti P, Nesti E, Urti DA, and Bonechi I

Subjects
Adult, Arteriosclerosis complications, Blood Chemical Analysis, Blood Pressure, Carotid Arteries physiology, Female, Humans, Hypertension, Renal complications, Kidney Failure, Chronic complications, Kidney Failure, Chronic therapy, Male, Ultrasonography, Uremia complications, Uremia physiopathology, Uremia therapy, Arteriosclerosis physiopathology, Carotid Arteries physiopathology, Hypertension, Renal physiopathology, Kidney Failure, Chronic physiopathology, Renal Dialysis
Abstract

Cerebrovascular accidents, often secondary to severe atherosclerotic disease, are very common in uremic patients on long-term hemodialysis. The aim of the present study is to assess asymptomatic carotid artery atherosclerotic disease (CAAD) in hemodialyzed normotensive and hypertensive patients in comparison with age-matched controls, by the use of Doppler ultrasound flow velocity wave form analysis (FVWFA), recorded from the common carotid artery. This study was performed on 47 subjects divided into four groups: 10 young and 10 middle-aged normals were considered in groups I and II, respectively, 5 young uremic normotensive, 6 young uremic hypertensive and 16 middle-aged uremic normotensive patients in groups III, IV and V, respectively. All the examined patients were nonsmokers, without diabetes or cardiopathy. The five wave form dimensions most capable of separating different degrees of atherosclerotic disease were determined on every common carotid tracing and used in a single best fit discriminant equation; the resultant discriminant score (DS) classified each carotid tracing and consequently every group's range. DS of groups I and III were not different, but significantly higher compared to the other three groups; besides DS was statistically not different in groups II, IV and V. In conclusion, FVWFA did not detect a different degree of CAAD between normotensive dialyzed patients and age-matched normals, whereas the blood pressure pharmacological control did not affect the velocity findings of advanced CAAD in young uremic hypertensive patients.

Published
1986
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