Your search keyword '"V., Giancotti"' showing total 121 results

1. Roles of HMGA proteins in cancer: Expression, pathways, and redundancies

Author

V, Giancotti, primary, P, Cataldi, additional, and C, Rizzi, additional

Published

2016

2. Identification of the unknown transformation products derived from clarithromycin and carbamazepine using liquid chromatography/high-resolution mass spectrometry

Author

P, Calza, C, Medana, E, Padovano, V, Giancotti, and C, Baiocchi

Subjects

Carbamazepine, Photolysis, Clarithromycin, Hydroxylation, Carbon, Mass Spectrometry, Water Pollutants, Chemical, Chromatography, Liquid

Abstract

A comprehensive study of the environmental fate of pollutants is more and more required, above all on new contaminants, i.e. pharmaceuticals. As high-resolution mass spectrometry (HRMS(n)) may be a suitable analytical approach for characterization of unknown compounds, its performance was evaluated in this study.The analyses were carried out using liquid chromatography (LC) (electrospray ionization (ESI) in positive mode) coupled with a LTQ-Orbitrap analyzer. High-resolution mass spectrometry was employed to assess the evolution of the drug transformation processes over time; accurate masses of protonated molecular ions and sequential product ions were reported with an error below 5 millimass units, which guarantee the correct assignment of their molecular formula in all cases, while their MS(2) and MS(3) spectra showed several structurally diagnostic ions that allowed characterization of the different transformation products (TPs) and to distinguish the isobaric species.The simulation of phototransformation occurring in the aquatic environment and identification of biotic and abiotic transformation products of the two pharmaceuticals were carried out in heterogeneous photocatalysis using titanium dioxide, aimed to recreate conditions similar to those found in the environmental samples. Twenty-eight main species were identified after carbamazepine transformation and twenty-nine for clarithromycin.This study demonstrates that HRMS, combined with LC, is a technique able to play a key role in the evaluation of the environmental fate of pollutants and allows elucidation of the transformation pathways followed by the two drugs.

Published

2012

3. Characterization of phenazone transformation products on light-activated TiO2 surface by high-resolution mass spectrometry

Author

P, Calza, C, Medana, E, Raso, V, Giancotti, and C, Minero

Subjects

Titanium, Photolysis, Light, Rivers, Toxicity Tests, Water, Hydroxylation, Antipyrine, Mass Spectrometry, Water Pollutants, Chemical

Abstract

The paper examines the transformation of phenazone (2,3-dimethyl-1-phenyl-3-pyrazolin-5-one), a widely used analgesic and antipyretic drug, under simulated solar irradiation in pure water, using titanium dioxide, and in river water. High-resolution mass spectrometry was employed to monitor the evolution of photoinduced processes. Initially, laboratory experiments were performed to simulate drug-transformation pathways in aqueous solution, using TiO(2) as photocatalyst. Thirteen main phenazone transformation products were detected, and full analysis of their MS and MS(n) spectra identified the diverse isobaric species. All these transformation products were themselves easily degraded, and no compounds were recognized to remain until 1h of irradiation. From these findings, a tentative degradation pathway is proposed to account for the photoinduced transformation of phenazone in natural waters. These simulation experiments were verified in the field, seeking phenazone in River Po water samples.

Published

2011

4. HMGI proteins interfere with the homeodomains binding to DNA

Author

ARLOTTA P., RUSTIGHI, ALESSANDRA, MANTOVANI, FIAMMA, V. GIANCOTTI, G. TELL AND G. DAMANTE, MANFIOLETTI, GUIDALBERTO, Arlotta, P., Rustighi, Alessandra, Mantovani, Fiamma, Manfioletti, Guidalberto, V., Giancotti, and G. TELL AND G., Damante

Published

1997

5. The Expression of the High-mobility Group Hmgi (y) Proteins Correlates With the Malignant Phenotype of Human Thyroid Neoplasias

Author

G. CHIAPPETTA, A. BANDIERA, M. T. BERLINGIERI, R. VISCONTI, G. MANFIOLETTI, S. BATTISTA, F. J. MARTINEZTELLO, V. GIANCOTTI, SANTORO, MASSIMO, FUSCO, ALFREDO, G., Chiappetta, A., Bandiera, M. T., Berlingieri, R., Visconti, G., Manfioletti, S., Battista, F. J., Martineztello, Santoro, Massimo, V., Giancotti, and Fusco, Alfredo

Abstract

High Mobility Group I(HMGI) proteins are nuclear proteins involved in the regulation of chromatin structure and function, Elevated expression of the HMGI proteins (HMGI, HMGY and HMGI-C) has been correlated with the presence of a highly malignant phenotype in epithelial and fibroblastic rat thyroid cells, and in several experimental carcinomas, Here, we demonstrate that HMGI and HMGY proteins are expressed in human thyroid carcinomas and thyroid carcinoma cell lines, but not in adenomas, goiters, normal thyroid tissues and cells, These results indicate a correlation between HMGI and HMGY expression and the malignant phenotype of thyroid neoplasias, suggesting that these proteins may be used as markers in thyroid cancer.

Published

1995

6. Reduction of risk factors for cardiovascular diseases in morbid-obese patients following biliary-intestinal bypass: 3 years' follow-up

Author

Giovanni Spera, Mario Marini, E Fabbrini, Silvia Migliaccio, N Falsetto, S. Falcone, F Brandetti, G Prossomariti, M Badiali, M Pili, S Ginanni-Corradini, C. Lubrano, V Giancotti, Alessandra Cornoldi, and A Eramo

Subjects

Adult, Blood Glucose, Male, medicine.medical_specialty, Endocrinology, Diabetes and Metabolism, medicine.medical_treatment, Medicine (miscellaneous), Blood Pressure, Gastroenterology, Body Mass Index, Jejunoileal Bypass, Weight loss, Internal medicine, Weight Loss, medicine, Humans, Insulin, risk factors, Postoperative Period, Risk factor, bypass, cardiovascular, disease, Triglycerides, Nutrition and Dietetics, medicine.diagnostic_test, Anthropometry, Vascular disease, business.industry, Middle Aged, medicine.disease, Obesity, Obesity, Morbid, Blood pressure, Endocrinology, Cholesterol, Cardiovascular Diseases, Female, medicine.symptom, Lipid profile, business, Body mass index, Follow-Up Studies

Abstract

BACKGROUND: Obese patients are often affected by hypertension, dyslipidaemia, impaired glucose metabolism, and suffer from cardiovascular disease (CVD), related to the characteristic metabolic alterations. AIM OF THE STUDY: To evaluate reduction of risk factors for CVDs in morbid-obese patients (body mass index (BMI)>40kg/m2) after weight loss upon bariatric surgery intervention of biliary-intestinal bypass. SUBJECTS: 45 (17 men, 28 women) morbid-obese patients (age: 19–49 y, BMI>40 kg/m2). All patients were selected on the basis of medical history, physical and biochemical evaluation and of psychiatric tests, which were performed on all individuals admitted to our Day Hospital to verify the safety of surgical intervention. MEASUREMENTS: Body weight, body composition (by dual X-ray absorptiometry, DXA), blood pressure, lipid profile, fibrinogen and glucose metabolism were monitored at baseline and 1, 3, 6, 9, 12, 24 and 36 months after surgery. RESULTS: A significant and persistent weight loss was present in all patients at the end of the 3 y follow-up period (P

Published

2004

7. High Mobility Group (HMGA1a) protein expression as a diagnostic indicator of human colorectal neoplastic diseases

Author

G. Chiappetta, G. Manfioletti, F. Pentimalli, M. Molnaco, R. Pasquinelli, T. Watanabe, M. Fedele, G. Viglietto, M. Santoro, and V. Giancotti A. Fusco

Published

2002

8. Expression of HMGI-C and HMGI(Y) in ordinary lipoma and atypical lipomatous tumors: immunohistochemical reactivity correlates with karyotypic alterations

Author

G, Tallini, P, Dal Cin, K J, Rhoden, G, Chiapetta, G, Manfioletti, V, Giancotti, A, Fusco, H, Van den Berghe, and R, Sciot

Subjects

Adult, Chromosome Aberrations, Karyotyping, HMGA2 Protein, High Mobility Group Proteins, Humans, Soft Tissue Neoplasms, HMGA1a Protein, Lipoma, Liposarcoma, Immunohistochemistry, Neoplasm Proteins, Research Article

Abstract

The high mobility group proteins (HMGs) are a class of low molecular weight, nonhistone, nuclear proteins that bind DNA and function as transcription cofactors. This class includes the HMGI family members HMGI-C and HMGI(Y). Both are not significantly expressed in differentiated adult tissues, including fat, but their expression is induced in proliferating and transformed cells. Their involvement in the development of lipomatous tumors has been recently demonstrated for HMGI-C, which is encoded by a gene located at 12q15, the chromosomal segment often rearranged in ordinary lipomas. The same chromosomal segment is consistently amplified in the ring and giant marker chromosomes of atypical lipomatous tumors (ALTs), a term used to designate tumors previously labeled as well differentiated liposarcomas or atypical lipomas. The involvement of HMGI(Y) is strongly suspected as the gene coding for HMGI(Y) is located at 6p21, a chromosomal segment rearranged in a subset of ordinary lipomas. HMGI-C or HMGI(Y) protein expression was analyzed immunohistochemically in a group of 39 well differentiated adipose neoplasms (19 lipomas and 20 ALTs) of known karyotype using polyclonal antibodies raised against a recombinant protein (HMGI-C) and against a synthetic peptide (HMGI(Y)). The results of this study demonstrate that HMGI proteins are commonly expressed in well differentiated adipose neoplasms. Seventeen of twenty ALTS (85.0%), all of which had ring or giant marker chromosomes with amplification of 12q13-15, strongly expressed HMGI-C. HMGI-C expression was detected in 7 of 11 ordinary lipomas (63.6%) with alterations at 12q14-15 and in one case with an abnormal karyotype that included double minute chromosomes. HMGI-C immunoreactivity correlates with 12q13-15 chromosomal alterations (P = 0.001). HMGI(Y) reactivity was demonstrated in only two ordinary lipomas: one with 6p21 rearrangement and one with normal karyotype. No significant HMGI(Y) expression was found in the ALT group. The finding of aberrant expression of HMGI proteins in well differentiated adipose neoplasms in association with 12q13-15 and 6p21 chromosomal changes supports the proposed pathogenetic role of this group of proteins in the development of adipose tissue tumors.

Published

1997

9. HMGA2 expression and response to anthracycline-based preoperative chemotherapy in patients with operable breast cancer

Author

M. Mansutti, V. Giancotti, C. Di Loreto, Federica Edith Pisa, Maura Pandolfi, Paola Ermacora, Pamela Driol, B. Alessi, P. Masolini, and Fabio Puglisi

Subjects

Oncology, Cancer Research, medicine.medical_specialty, biology, Anthracycline, business.industry, medicine.disease, Preclinical data, Breast cancer, HMGA2, Internal medicine, medicine, biology.protein, Preoperative chemotherapy, Doxorubicin, In patient, Breast cancer cells, business, medicine.drug

Abstract

22035 Background: Preclinical data suggest that increased expression of high mobility group A2 (HMGA2) protein could enhance chemosensitivity towards doxorubicin in breast cancer cells. The present...

Published

2008

10. HMGA1 protein over-expression is a frequent feature of epithelial ovarian carcinomas.

Author

G. Viglietto, V. Masciullo, G. Scambia, G. Baldassarre, A. Fusco, F. Pentimalli, M.T. Berlingieri, A. Boccia, G. Chiappetta, J. Palazzo, G. Manfioletti, and V. Giancotti

Subjects

OVARIAN cancer, IMMUNOHISTOCHEMISTRY

Abstract

High mobility group A 1 (HMGA1) proteins are chromatinic factors, which are absent or expressed at very low levels in normal adult tissues, while they are over-expressed in several human malignant tumors. In this study, HMGA1 protein expression was investigated by immunohistochemistry in a series of 44 epithelial ovarian specimens, which included four normal ovarian tissues, 29 primary invasive carcinomas, one metastatic ovarian tumor and 10 low malignant potential (LMP) tumors. HMGA1 staining was not detected in normal ovarian surface epithelium, which is the area from which ovarian adenocarcinoma frequently arises. HMGA1 proteins were expressed at low levels in some LMP tumors, whereas they were present in abundance in most of the primary ovarian adenocarcinomas. RT-PCR and western blot analysis correlated with immunohistochemical data. We demonstrated that the suppression of HMGA1 protein synthesis by an adenovirus carrying the HMGA1 gene in antisense orientation (Ad-Yas-GFP) inhibited the growth of two human ovarian carcinoma cell lines (OVCAR-5 and OVCAR-8). These results confirm HMGA1 over-expression as a general feature of human malignant neoplasias, including ovarian cancer and suggest that suppression of HMGA1 protein synthesis by an antisense adenoviral vector may represent a new and promising gene therapy for the treatment of ovarian cancer. [ABSTRACT FROM AUTHOR]

Published

2003

11. A method for silver staining HMG chromosomal proteins in polycarylamide electrophoretic gels

Author

G.H. Goodwin and V. Giancotti

Subjects

Silver, Staining and Labeling, Chemistry, High Mobility Group Proteins, Biophysics, Thymus Gland, Biochemistry, Molecular biology, Staining, Silver stain, Electrophoresis, Coomassie blue, Animals, Cattle, Electrophoresis, Polyacrylamide Gel

Abstract

A method is presented for sensitive staining of the HMG14 and 17 proteins in polycrylamide gels pre-stained with Coomassie Blue R250. The procedure involves binding negatively and positively charged polycyclic aromatic compounds to the proteins followed by staining with silver using the method of Wray et al. (1981)[4].

Published

1986

12. Conformational studies of poly(l-tyrosine) in solvent mixtures of dimethylsulphoxide with water and trimethylphosphate

Author

V. Giancotti, C. Crane-Robinson, E.M. Bradbury, and R.M. Stephens

Subjects

Solvent system, chemistry.chemical_classification, Polymers and Plastics, Chemistry, Organic Chemistry, Infrared spectroscopy, Polymer, Nuclear magnetic resonance spectroscopy, Random coil, Solvent, Crystallography, Materials Chemistry, Organic chemistry, Tyrosine, Optical rotation

Abstract

The conformational behaviour of poly( l -tyrosine) has been studied in dimethylsulphoxide/water and dimethylsulphoxide/trimethylphosphate solvent systems. The evidence provided by nuclear magnetic resonance and infrared spectroscopy shows that the conformation of the polymer in dimethylsulphoxide is most probably the random coil. Addition of 20% D 2 O or 50% trimethylphosphate to the dimethylsulphoxide/poly( l -tyrosine) solution results in a conformational transition of the polymer which can be followed by both infra-red and nuclear magnetic resonance spectroscopy and changes in optical rotation. The evidence supports the conclusion that this transition is to a largely, though not fully, right-handed α-helical conformation.

Published

1972

13. Solid state transitions in zinc(II) di-n-alkylphosphinate polymers

Author

P.A. Temussi, A. Ripamonti, and V. Giancotti

Subjects

chemistry.chemical_classification, Materials science, Polymers and Plastics, Organic Chemistry, Solid-state, chemistry.chemical_element, Zinc, Polymer, Crystal, Crystallography, Differential scanning calorimetry, chemistry, Materials Chemistry, Side chain

Abstract

A study has been made of the reversible solid state transitions in a series of eleven zinc(II) di-n-alkylphosphinate polymers, [Zn(R2PO2)2]n, with R from C4 to C18, by means of differential scanning calorimetry and x-ray analysis. Wide line n.m.r. measurements have been also made for some compounds. The existence of two crystal forms, denoted α and β, has been established for the compounds examined. The results indicate that the α→β polymorphic transition is associated with disordering of the hydrocatbon side chains.

Published

1971

14. [Effect of a component of human lymphocyte dialysate on the motor activity of polymorphonuclear leukocytes]

Author

S, Spisani, V, Giancotti, E, Russo, R, Carletti, and S, Traniello

Subjects

Chromatography, Leukemia, Chemotactic Factors, Cell Movement, Neutrophils, Humans, Lymphocytes, Dialysis

Abstract

Lymphocyte dialysates obtained from healthy volunteers and leukemic subject were chromatographed on Bio-Gel P-4. Partially purified fractions were assayed for neutrophil locomotion: a positive chemokinetic effect and no chemotactic activity was observed in both samples.

Published

1980

15. Letter: Heat of interaction of DNA with polylysine and trilysine

Author

V, Giancotti, A, Cesaro, and V, Crescenzi

Subjects

Solutions, Hot Temperature, Thermodynamics, Polylysine, DNA, Peptides

Published

1975

16. Helix sense of poly- -benzyl-L-aspartate

Author

V, Giancotti, F, Quadrifoglio, and V, Crescenzi

Subjects

Molecular Weight, Aspartic Acid, Polymers, Protein Conformation, Spectrum Analysis, Benzyl Compounds

Published

1972

17. Calorimetry of DNA-dye interactions in aqueous solution I. Proflavine and ethidium bromide

Author

F, Quadrifoglio, V, Crescenzi, and V, Giancotti

Abstract

The results of an investigation on the interaction of proflavine and of ethidium bromide with DNA (calf thymus) in dilute aqueous solution are reported. The binding of the two dyes by DNA has been studied by means of microcalorimetric and of equilibrium dialysis measurements. Data on the thermodynamics of dimerization of both proflavine and ethidium bromide in aqueous solution obtained on the basis of spectroscopic and/or calorimetric experiments are also reported. The enthalpy data show that dye-dimerization and dye "strong" interaction with DNA are energetically favourable and quite similar while only in the latter case the phenomenon is also entropy driven. This is taken as further evidence in support of the concept that "strong" interaction-of both proflavine and ethidium bromide with DNA means dye molecules intercalation into the native, double helical structure of the biopolymer.

Published

1973

18. Observations sur quelques aspects de la culture de Cris du Néolithique ancien de la Roumanie

Author

V. Giancotti-Tassone

Subjects

Ocean Engineering

Abstract

Résumé. — Dans cet article nous avons essayé de présenter les éléments essentiels de la culture de Cris de Roumanie, qui constitue le Néolithique le plus ancien du Bas-Danube. Les thèses principales soutenues dans l'article sont au nombre de quatre. 1) Le synchronisme de Starcevo (en Yougoslavie), Koros (en Hongrie) de la Céramique Linéaire (en Tchécoslovaquie), ainsi que de Karanovo I et Kremicovci en Bulgarie avec Cris. 2) Le refus d'une division des cultures de Starcevo et de Cris en quatre phases. 3) Le développement indépendant de toutes les cultures du Néolithique ancien de Roumanie, sans relations notables avec le Proche-Orient et la Méditerranée Occidentale. 4) Le postulat d'une continuité Cris-Vinca-Turdas et Petresti., Giancotti-Tassone Vicente. Observations sur quelques aspects de la culture de Cris du Néolithique ancien de la Roumanie. In: Bulletin de la Société préhistorique française. Études et travaux, tome 67, n°1, 1970. pp. 323-334.

Published

1970

19. Mechanism of enhanced RNA synthesis in acute-phase rat liver and its relationship to chromatin structure

Author

Gaetano Cairo, V Giancotti, Luisa Schiaffonati, Aldo Bernelli-Zazzera, and Lidia Bardella

Subjects

Electrophoresis, Male, Transcription, Genetic, Chromosomal Proteins, Non-Histone, Turpentine, Polynucleotides, Inbred Strains, Biochemistry, Genetic, Animals, Cell Nucleus, metabolism, Chromatin, metabolism, Chromosomal Proteins, Non-Histone, metabolism, DNA-Directed RNA Polymerases, metabolism, Drug-Induced Liver Injury, metabolism, Electrophoresis, Polyacrylamide Gel, Liver, metabolism, Male, Micrococcal Nuclease, Polynucleotides, metabolism, RNA, biosynthesis, Rats, Rats, Inbred Strains, Transcription, Genetic, Turpentine, Animals, Micrococcal Nuclease, Molecular Biology, Polymerase, Cell Nucleus, Polyacrylamide Gel, biology, Rats, Inbred Strains, Drug-Induced Liver Injury, Cell Biology, DNA-Directed RNA Polymerases, Molecular biology, Chromatin, Rats, Chromosomal Proteins, Liver, Rat liver, biology.protein, RNA, Electrophoresis, Polyacrylamide Gel, Chemical and Drug Induced Liver Injury, biosynthesis, Digestion, metabolism, Transcription, Research Article, Acute inflammatory reaction

Abstract

Nuclei isolated from the liver of rats undergoing an acute inflammatory reaction induced by turpentine treatment show increased RNA synthesis. This increase is essentially determined by a faster polyribonucleotide-elongation rate while the number of transcribing polymerase molecules is unchanged. The sensitivity of chromatin to micrococcal-nuclease digestion and the composition of chromosomal proteins are not affected by the acute-phase process. Therefore the increased RNA synthesis by liver nuclei from acutely inflamed rats does not seem to correlate with major changes in chromatin structure.

20. X-Ray study of zinc(II) di-n-alkylphosphinate copolymers

Author

A. Ripamonti, V. Giancotti, L. Randaccio, and F. Giordano

Subjects

chemistry.chemical_classification, Inorganic chemistry, X-ray, chemistry.chemical_element, Polymer, Zinc, Phosphinate, Inorganic Chemistry, Metal, Crystallography, chemistry, visual_art, visual_art.visual_art_medium, Copolymer, Physical and Theoretical Chemistry

Abstract

The mixed-ligand species Zn[(R12PO2)2 – 2x(R22PO2)2x](R1= Bun; R2= n-C6H13 or n-C10H21) are linear coordination copolymers with a random distribution of two different bridging phosphinate groups along the molecular chains. Single crystals of the copolymer {Zn[Bun2PO2(n-C6H13)2PO2]}n are disordered. A three-dimensional X-ray analysis has been attempted. The crystals contain chains characterised by a backbone structure with alternate single and triple bridging phosphinate groups between tetrahedral metal atoms. The structural features common to those of the β-form of zinc(II) di-n-butylphosphinate polymer are discussed.

Published

1968

21. Structure and properties of beryllium phosphinate polymers

Author

V. Giancotti, A. Ripamonti, and F. Gemiti

Subjects

chemistry.chemical_classification, Chemistry, Inorganic chemistry, Polymer, Crystal structure, Phosphinate, Inorganic Chemistry, Solvent, Metal, Crystallography, Hydrocarbon, visual_art, Copolymer, visual_art.visual_art_medium, Physical and Theoretical Chemistry, Alkyl

Abstract

The characterisation of beryllium phosphinates of stoicheiometry Be(Bun2PO2)2, Be(Ph2PO2)2, and of some mixed-ligand species Be[(Bun2PO2)2 – 2x(Ph2PO2)2x] is reported. The compounds richer in alkyl groups give stable solutions in hydrocarbon and halogenated solvents. Solution properties indicate that these compounds are linear polymers which undergo a reversible degradation influenced by the nature of the solvent, concentration, and temperature. The mixed-ligand species can be crystallised and are formulated as random copolymers. Isomorphous replacement of the two kinds of phosphinate groups within the crystal lattice of the related homopolymers is observed. The X-ray diffraction fibre photographs indicate that the homopolymer [Be(Bun2PO2)2]n and the copolymers {Be[(Ben2PO2)2 – 2x(Ph2PO2)2x]}n(x= 0·20 or 0·33) have a backbone structure with alternate single and triple bridging phosphinate groups between tetrahedral metal atoms. The same chain-type structure is proposed for the homopolymer [Be(Ph2PO2)2]n and the copolymers richer in diphenylphosphinate groups.

Published

1968

22. Isomorphism and polymorphism in zinc(II) and cobalt(II) phosphinate polymers

Author

A. Ripamonti and V. Giancotti

Subjects

Stereochemistry, chemistry.chemical_element, Zinc, Crystal structure, Phosphinate, Inorganic Chemistry, Crystallography, Differential scanning calorimetry, chemistry, Polymorphism (materials science), Isomorphous substitution, Physical and Theoretical Chemistry, Solubility, Cobalt

Abstract

A study has been made of the iso- and poly-morphism phenomena in a series of mixed-ligand species, {M[(Bun2PO2)2 – 2x(Ph2PO2)2x]}n(M = ZnII or CoII), by means of differential scanning calorimetry and X-ray analysis. These compounds are linear copolymers and the di-n-butylphosphinate and diphenylphosphinate groups are randomly distributed along the molecular chains. The homopolymer, [Zn(BunPhPO2)2]n, has been studied as a model system with a disordered positioning of the n-butylphenylphosphinate groups along the molecular chains. This compound exhibits polymorphism and its γ-form is isomorphous with that of [Zn(Ph2PO2)2]n.The zinc(II) mixed-ligand species are crystalline and isomorphous with the blue cobalt(II) compounds. Their solubility in non-co-ordinating solvents decreases with increasing the content of Ph2PO2– groups. Isomorphous substitution of some Ph2PO2– groups with Bun2PO2– groups in the crystal lattice of the [Zn(Ph2PO2)2]n homopolymer or of some Bun2PO2– groups with Ph2PO2– groups in the crystal lattice of the [Zn(Bun2PO2)2]n homopolymer takes place. On the basis of the structures of the crystalline form of [Zn(Bun2PO2)2]n, stable at room temperature, and of the γ-form of [Zn(BunPhPO2)2]n, the solid-state transitions and the isomorphism and polymorphism phenomena of the various co-ordination polymers are discussed.

Published

1969

23. HMGA1 protein over-expression is a frequent feature of epithelial ovarian carcinomas

Author

Giuseppe Viglietto, Francesca Pentimalli, Gustavo Baldassarre, Giovanni Scambia, Juan P. Palazzo, Guidalberto Manfioletti, Vincenzo Giancotti, Angelo Boccia, Alfredo Fusco, Maria Teresa Berlingieri, Gennaro Chiappetta, Valeria Masciullo, V., Masciullo, G., Baldassarre, F., Pentimalli, M. T., Berlingieri, A., Boccia, G., Chiappetta, J., Palazzo, G., Manfioletti, V., Giancotti, G., Viglietto, G., Scambia, and Fusco, Alfredo

Subjects

Cancer Research, endocrine system diseases, Adenocarcinoma, Biology, DNA, Antisense, Adenoviridae, Immunoenzyme Techniques, Ovarian tumor, Western blot, Ovarian carcinoma, Tumor Cells, Cultured, medicine, Carcinoma, Humans, HMGA1a Protein, Adaptor Proteins, Signal Transducing, DNA Primers, GRB2 Adaptor Protein, Ovarian Neoplasms, medicine.diagnostic_test, Reverse Transcriptase Polymerase Chain Reaction, Proteins, General Medicine, medicine.disease, HMGA1, female genital diseases and pregnancy complications, Epithelium, Gene Expression Regulation, Neoplastic, medicine.anatomical_structure, biology.protein, Cancer research, Immunohistochemistry, Female, Ovarian cancer

Abstract

High mobility group A 1 (HMGA1) proteins are chromatinic factors, which are absent or expressed at very low levels in normal adult tissues, while they are over-expressed in several human malignant tumors. In this study, HMGA1 protein expression was investigated by immunohistochemistry in a series of 44 epithelial ovarian specimens, which included four normal ovarian tissues, 29 primary invasive carcinomas, one metastatic ovarian tumor and 10 low malignant potential (LMP) tumors. HMGA1 staining was not detected in normal ovarian surface epithelium, which is the area from which ovarian adenocarcinoma frequently arises. HMGA1 proteins were expressed at low levels in some LMP tumors, whereas they were present in abundance in most of the primary ovarian adenocarcinomas. RT-PCR and western blot analysis correlated with immunohistochemical data. We demonstrated that the suppression of HMGA1 protein synthesis by an adenovirus carrying the HMGA1 gene in antisense orientation (Ad-Yas-GFP) inhibited the growth of two human ovarian carcinoma cell lines (OVCAR-5 and OVCAR-8). These results confirm HMGA1 over-expression as a general feature of human malignant neoplasias, including ovarian cancer and suggest that suppression of HMGA1 protein synthesis by an antisense adenoviral vector may represent a new and promising gene therapy for the treatment of ovarian cancer.

Published

2003

24. Thyroid cell transformation requires the expression of the HMGA1 proteins

Author

Alfredo Fusco, Giovanna Maria Pierantoni, Maria Teresa Berlingieri, Vincenzo Giancotti, Massimo Santoro, M. T., Berlingieri, Pierantoni, GIOVANNA MARIA, V., Giancotti, Santoro, Massimo, and Fusco, Alfredo

Subjects

Cancer Research, DNA, Complementary, HMGI, Recombinant Fusion Proteins, Cell, Thyroid Gland, Mice, Nude, Oncogene Protein p21(ras), Transfection, medicine.disease_cause, DNA, Antisense, thyroid, Mice, Species Specificity, Genetics, medicine, Animals, Neoplastic transformation, HMGA1a Protein, Molecular Biology, Cells, Cultured, Tumor Stem Cell Assay, Cell Line, Transformed, biology, Oncogene, HMGA2 Protein, Thyroid, Cell Transformation, Viral, HMGA1, Rats, Inbred F344, Rats, Transcription Factor AP-1, Genes, ras, Phenotype, medicine.anatomical_structure, Cell culture, biology.protein, Cancer research, Carcinogenesis, Kirsten murine sarcoma virus, neoplasm

Abstract

Elevated expression of HMGA1 and HMGA2 proteins is correlated with a highly malignant phenotype in several human tumors. We previously demonstrated that the block of HMGA2 protein synthesis prevented rat thyroid cell transformation by murine retroviruses. Suppression of HMGA2 synthesis was associated with lack of induction of HMGA1 proteins suggesting that both HMGA1 and HMGA2 play a role in the process of neoplastic transformation. To determine the role of the HMGA1 gene in thyroid cell transformation, we blocked HMGA1 protein synthesis by an antisense methodology. Here we report that transfection of an HMGA1 cDNA antisense construct into a normal rat thyroid cell line (FRTL-5 Cl2), followed by infection with Kirsten murine sarcoma virus (KiMSV), generated a transformed cell line that expresses high levels of the v-ras-Ki oncogene and that does not require thyroid-stimulating hormones for growth. However, this cell line does not show the malignant phenotype, i.e., it neither grows in soft agar nor induces tumors after injection in athymic mice. Moreover, the lack of the neoplastic phenotype in the virus-infected thyroid cells carrying the HMGA1 antisense construct correlates with the absence of induction of AP-1 transcriptional activity.

Published

2002

25. High mobility group HMGI(Y) protein expression in human colorectal hyperplastic and neoplastic diseases

Author

Maurizio Di Bonito, Nobutsugu Abe, Ada Giuliano, Maria Teresa Vento, Guidalberto Manfioletti, Takashi Watanabe, Massimo Santoro, Alfredo Fusco, Gennaro Chiappetta, Francesca Pentimalli, Monica Fedele, Giuseppe Viglietto, Vincenzo Giancotti, G., Chiappetta, G., Manfioletti, F., Pentimalli, N., Abe, M. D., Bonito, M. T., Vento, A., Giuliano, M., Fedele, G., Viglietto, Santoro, Massimo, T., Watanabe, V., Giancotti, Fusco, Alfredo, Chiappetta, G., Manfioletti, Guidalberto, Pentimalli, F., Abe, N., DI BONITO, M., Vento, M. T., Giuliano, A., Fedele, M., Viglietto, G., Santoro, M., Watanabe, T., Giancotti, V., and AND FUSCO, A.

Subjects

Adenoma, Cancer Research, Pathology, medicine.medical_specialty, analysis, Colon, Cell, Colonic Polyps, Biology, medicine.disease_cause, Malignant transformation, Gene expression, medicine, Carcinoma, Humans, Neoplastic transformation, HMGA1a Protein, Hyperplasia, High Mobility Group Proteins, chemistry/pathology, HMGA1a Protein, High Mobility Group Protein, medicine.disease, chemistry/pathology, Colorectal Neoplasm, Immunohistochemistry, digestive system diseases, Neoplasm Proteins, analysis, Humans, Hyperplasia, Immunohistochemistry, Neoplasm Protein, medicine.anatomical_structure, Oncology, analysis, Transcription Factor, chemistry, Colon, Cancer research, pathology, Colonic Polyp, Carcinogenesis, Colorectal Neoplasms, Transcription Factors

Abstract

HMGI(Y) proteins are overexpressed in experimental and human malignancies, including colon, prostate and thyroid carcinomas. To determine at which step of the carcinogenic process HMGI(Y) induction occurs, we analysed the expression of the HMGI(Y) proteins in hyperplastic, preneoplastic and neoplastic tissues of colorectal origin by immunohistochemistry. All the colorectal carcinomas were HMGI(Y)-positive, whereas no expression was detected in normal colon mucosa tissue. HMGI(Y) expression in adenomas was closely correlated with the degree of cellular atypia. Only 2 of the 18 non-neoplastic polyps tested were HMGI(Y)-positive. These data indicate that HMGI(Y) protein induction is associated with the early stages of neoplastic transformation of colon cells and only rarely with colon cell hyperproliferation.

Published

2001

26. ROLE OF THE HIGH MOBILITY GROUP A PROTEINS IN HUMAN LIPOMAS

Author

Sabrina Battista, Monica Fedele, Guidalberto Manfioletti, Alfredo Fusco, Vincenzo Giancotti, Carlo M. Croce, Fedele, M, Battista, S, Manfioletti, Guidalberto, Croce, Cm, Giancotti, V, Fusco, A., M., Fedele, S., Battista, G., Manfioletti, C. M., Croce, V., Giancotti, and Fusco, Alfredo

Subjects

Cancer Research, biology, Alternative splicing, High Mobility Group Proteins, HMGA, Mice, Transgenic, General Medicine, HMGA1, Molecular biology, HMGA1 Gene, Gene product, Mice, HMGA2, Non-histone protein, Adipose Tissue, Adipocytes, biology.protein, Animals, Humans, Lipoma, HMGA Proteins, Plant Proteins

Abstract

The HMGA family is comprised of four proteins: HMGA1a, HMGA1b, HMGA1c and HMGA2. The first three proteins are products of the same gene, HMGA1, generated through an alternative splicing mechanism. The HMGA proteins are involved in the regulation of chromatin structure and HMGA DNA-binding sites have been identified in functional regions of many gene promoters. Rearrangements of the HMGA2 gene have been frequently detected in human benign tumors of mesenchymal origin including lipomas. 12q13-15 chromosomal translocations involving the HMGA2 gene locus, account for these rearrangements. The HMGA proteins have three AT-hook domains and an acidic C-terminal tail. The HMGA2 modifications consist in the loss of the C-terminal tail and fusion with ectopic sequences. A pivotal role of the HMGA2 rearrangements in the process of lipomagenesis is suggested by experiments showing that transgenic mice carrying a truncated HMGA2 gene showed a giant phenotype together with abdominal/pelvic lipomatosis. As HMGA2 null mice showed a great reduction in fat tissue, a positive role of the HMGA2 gene in adipocytic cell proliferation is proposed. More recently, similar alterations of the HMGA1 gene have been described. As the block of the HMGA1 protein synthesis induces an increase in growth rate of the pre-adipocytic cell line 3T3-L1, we suggest a negative role of the HMGA1 proteins in adipocytic cell growth and, therefore, we propose that adipocytic cell growth derives from the balance of the HMGA1 and HMGA2 protein functions.

Published

2001

27. Sp1 and CTF/NF-1 transcription factors are involved in the basal expression of the Hmgi-c proximal promoter

Author

Alfredo Fusco, Guidalberto Manfioletti, Alessandra Rustighi, Fiamma Mantovani, Vincenzo Giancotti, Rustighi, Alessandra, Mantovani, Fiamma, Fusco, A, Giancotti, Vincenzo, Manfioletti, Guidalberto, A., Rustighi, F., Mantovani, Fusco, Alfredo, V., Giancotti, and G., Manfioletti

Subjects

Sp1 Transcription Factor, Response element, Molecular Sequence Data, Biophysics, Gene Expression, Genetic, Promoter Region, E-box, Biology, Gene Expression Re, Biochemistry, Cell Line, Promoter Regions, Mice, Genetic, Sp3 transcription factor, Trinucleotide Repeats, Humans, Animals, Polymorphism, Enhancer, Promoter Regions, Genetic, Molecular Biology, Transcription factor, DNA Primers, Sequence Deletion, Genetic, Sp1 Transcription Factor, Binding Sites, General transcription factor, Base Sequence, HMGA2 Protein, High Mobility Group Proteins, RNA-Binding Proteins, Promoter, Cell Biology, DNA, Molecular biology, DNA-Binding Proteins, NFI Transcription Factors, nuclear matrix protein, 5' Untranslated Regions, Gene Expression, Gene Expression Re, Humans, Polymorphism, Genetic, Promoter Regions, Sp3 Transcription Factor, Gene Expression Regulation, CCAAT-Enhancer-Binding Proteins, Drosophila, 5' Untranslated Regions, Transcription factor II A, Transcription Factors

Abstract

HMGI-C is a nuclear architectural factor which is expressed during embryogenesis but not in adult tissues while it becomes re-expressed following neoplastic transformation. In this paper we identify the promoter region of the mouse Hmgi-c gene and by stepwise deletion of the 5' sequences we map the promoter activity of the most abundant transcript to a very short fragment containing a long polypyrimidine/polypurine (ppyr/ppur) tract. We demonstrate that this tract is a multiple binding site for the transcription factors Sp1 and Sp3 and that in Drosophila SL2 cells, Spl activates the Hmgi-c promoter. In addition, another transcription factor, CTF/NF-1, binds the proximal promoter immediately downstream of this region and its mutation decreases transcription in NIH-3T3 cells. This study identifies factors responsible for the basal activity of Hmgi-c gene and provides a foundation for further analysis of the mechanism of its regulation.

Published

1999

28. Human colorectal carcinomas express high levels of High Mobility Group HMGI(Y) proteins

Author

Monica Fedele, Bandiera, A., Chiappetta, G., Battista, S., Viglietto, G., Manfioletti, G., Casamassimi, A., Santoro, M., Giancotti, V., Fusco, A., Fedele, M, Bandiera, Antonella, Chiappetta, G, Battista, S, Viglietto, G, Manfioletti, Guidalberto, Casamassimi, A, Santoro, M, Giancotti, V, Fusco, A., M., Fedele, A., Bandiera, G., Chiappetta, S., Battista, G., Viglietto, G., Manfioletti, A., Casamassimi, Santoro, Massimo, V., Giancotti, and Fusco, Alfredo

Subjects

Male, Colon, Molecular Sequence Data, metabolism, Thyroid Neoplasm, Thyroid Gland, Gene Expression, Amino Acid Sequence, Animals, Antibodies, Cell Line, Colon, analysis/biosynthesis, Humans, Immunohistochemistry, Male, Molecular Sequence Data, Peptide Fragment, Antibodies, Epithelium, Cell Line, metabolism/pathology, Tumor Cell, Reference Values, Tumor Cells, Cultured, Animals, Humans, Amino Acid Sequence, HMGA1a Protein, Thyroid Neoplasms, metabolism, Female, Fibroblast, metabolism/pathology/surgery, Colorectal Neoplasm, metabolism/pathology, Epithelium, Cultured, cytology/metabolism/pathology, Colonic Neoplasm, High Mobility Group Proteins, Fibroblasts, Immunohistochemistry, Peptide Fragments, Rats, chemical synthesis/immunology, Rats, Reference Values, Thyroid Gland, metabolism, Gene Expression, HMGA1a Protein, High Mobility Group Protein, Colonic Neoplasms, Female, Colorectal Neoplasms

Abstract

A correlation has previously been demonstrated between the presence of the three HMGI proteins (HMGI, HMGY, and HMGI-C) and the expression of a highly malignant phenotype in epithelial and fibroblastic rat thyroid cells; this being subsequently extended to experimental thyroid, lung, prostate, mammary, and skin carcinomas. Recently, we have demonstrated that expression of HMGI and HMGY proteins, coded for by the HMGI(Y) gene, is associated with the malignant phenotype of human thyroid neoplasias. Here, we show that HMGI(Y) gene expression is present both at the RNA and protein level in human colorectal carcinoma cell lines and tissues examined in this study. Conversely, no HMGI(Y) proteins were detected in normal intestinal mucosa. Therefore, these results suggest an involvement of HMGI and HMGY proteins overexpression in colorectal tumorigenesis.

Published

1996

29. Analysis of the Hmgi Nuclear Proteins In Mouse Neoplastic-cells Induced By Different Procedures

Author

L. Perissin, Alfredo Fusco, Vincenzo Giancotti, Sonia Zorzet, Alan Balmain, Giuseppe Portella, Graham H. Goodwin, Emanuele Buratti, V., Giancotti, E., Buratti, L., Perissin, S., Zorzet, A., Balmain, Portella, Giuseppe, Fusco, Alfredo, and G. H., Goodwin

Subjects

Cell Nucleus, Gel electrophoresis, Lung Neoplasms, Ratón, High Mobility Group Proteins, Mice, Nude, Nuclear Proteins, Lewis lung carcinoma, Neoplasms, Experimental, Cell Biology, Hmg protein, Biology, Molecular biology, Phenotype, Mice, Biochemistry, Cell culture, Gene expression, Animals, Amino Acids, Nuclear protein, Chromatography, High Pressure Liquid

Abstract

Four malignant tumors induced in mouse by different experimental procedures were compared as regards their high-mobility-group (HMG) proteins. All tumors showed the complete set of three HMG proteins which we call HMGI-C, I-D, and I-E. The presence of the three HMGI proteins is a characteristic of the transformed phenotype regardless of whether the tumor was chemically, virally, or spontaneously derived. However, the level of expression of the HMGI proteins is not constant in the four tumors. Using reverse-phase HPLC, the individual HMGI proteins were isolated from the spontaneously derived tumor (Lewis lung carcinoma) and shown by amino acid analysis to be similar to those previously obtained from a tumor grown in nude mice by inoculation of in vitro-transformed cells.

Published

1989

30. High level expression of the HMGI (Y) gene during embryonic development

Author

Chiappetta, G., Avantaggiato, V., Visconti, R., Monica Fedele, Battista, S., Trapasso, F., Merciai, B. M., Fidanza, V., Giancotti, V., Santoro, M., Simeone, A., Fusco, A., G., Chiappetta, V., Avantaggiato, R., Visconti, M., Fedele, S., Battista, F., Trapasso, B. M., Merciai, V., Fidanza, V., Giancotti, Santoro, Massimo, A., Simeone, and Fusco, Alfredo

Subjects

Adult, Inbred C57BL, RNA, physiology, Gene Expression Regulation, Messenger, High Mobility Group Proteins, Gene Expression Regulation, Developmental, Adult, Animals, Embryonic and Fetal Development, Gestational Age, Developmental, Gestational Age, HMGA1a Protein, High Mobility Group Protein, genetics/metabolism, Humans, In Situ Hybridization, Mice, Mice, Mice, Inbred C57BL, Embryonic and Fetal Development, Mice, Animals, Humans, HMGA1a Protein, RNA, Messenger, metabolism, In Situ Hybridization

Abstract

The HMGI protein family includes three proteins, named HMG-I, HMG-Y and HMGI-C. The first two proteins are coded for by the same gene, HMGI (Y), through an alternative splicing mechanism. Their expression is elevated in neoplastic tissues and cells and this overexpression has a causal role in the process of cellular neoplastic transformation. We demonstrate that the HMGI (Y) gene is expressed at very low levels in normal adult tissues, whereas in embryonic tissues it is expressed at high levels comparable to those detected in neoplastic tissues. Specifically, a very high expression of the HMGI (Y) gene was detected in all embryonic tissues at 8.5 dpc. Then in the following days, even though the gene is expressed essentially in all tissues, an abundant gene expression was restricted to some tissues. These results indicate an important role of the HMGI (Y) gene in development.

31. Expression of HMGI(Y) proteins in squamous intraepithelial and invasive lesions of the uterine cervix

Author

Bandiera, A., Bonifacio, D., Manfioletti, G., Mantovani, F., Rustighi, A., FABRIZIO ZANCONATI, Fusco, A., Di Bonito, L., Giancotti, V., Bandiera, Antonella, Bonifacio, Daniela, Manfioletti, Guidalberto, Mantovani, Fiamma, Rustighi, Alessandra, Zanconati, Fabrizio, Fusco, A, DI BONITO, Luigi, Giancotti, Vincenzo, A., Bandiera, D., Bonifacio, G., Manfioletti, F., Mantovani, A., Rustighi, F., Zanconati, Fusco, Alfredo, L. D., Bonito, and V., Giancotti

Subjects

Paraffin Embedding, HMGI(Y) protein, Blotting, Western, High Mobility Group Proteins, Antibodies, Monoclonal, Gene Expression, Uterine Cervical Neoplasms, Blotting, Northern, Uterine Cervical Dysplasia, markers to detect cancer, Immunoenzyme Techniques, intraepithelial and invasive lesions of the uterine cervix, Ki-67 Antigen, Antigens, Neoplasm, Biomarkers, Tumor, Carcinoma, Squamous Cell, Tumor Cells, Cultured, Humans, Female, Neoplasm Invasiveness, HMGA1a Protein, HMGI(Y) proteins, HMGA

Abstract

The expression of nuclear proteins high mobility group (HMG) I and HMGY was investigated in intraepithelial and invasive lesions of the uterine cervix. Human carcinoma cell lines C-41, ME-180, and CaSki were used for testing protein expression in neoplastic cells from the cervix. Morphological grading of the dysplasias (CIN 1, CIN 2, and CIN 3) and invasive carcinomas from formalin-fixed paraffin-embedded samples parallels the degree of nuclear immunostaining obtained using a polyclonal antibody raised against the amino-terminal region of HMGI(Y) proteins. The immunostaining obtained with HMGI(Y) antibody was compared with that observed using the antibody Ki-67, and the results were similar. We suggest the use of HMGI(Y) antibody in clinical oncology as a useful marker of intraepithelial lesions and invasive carcinomas.

32. Expression of HMGI-C and HMGI(Y) in ordinary lipoma and atypical lipomatous tumors: Immunohistochemical reactivity correlates with karyotypic alterations

Author

Giovanni Tallini, Dalcin, P., Rhoden, Kj, Chiapetta, G., Manfioletti, G., Giancotti, V., Fusco, A., Vandenberghe, H., Sciot, R., G. Tallini, P. DalCin, K. J. Rhoden, G. Chiapetta, G. Manfioletti, V. Giancotti, A. Fusco, H. VandenBerghe, and R. Sciot

Abstract

The high mobility group proteins (HMGs) are a class of low molecular weight, nonhistone, nuclear proteins that bind DNA and function as transcription cofactors. This class includes the HMGI family members HMGI-C and HMGI(Y). Both are not significantly expressed in differentiated adult tissues, including fat, but their expression is induced in proliferating and transformed cells. Their involvement in the development of lipomatous tumors has been recently demonstrated for HMGI-C, which is encoded by a gene located at 12q15, the chromosomal segment often rearranged ill ordinary lipomas. The same chromosomal segment is consistently amplified in the ring and giant marker chromosomes of atypical lipomatous tumors (ALTs), a term used to designate tumors previously labeled as well differentiated liposarcomas or atypical lipomas. The involvement of HMGI(Y) is strongly suspected as the gene coding for HMGI(Y) is located at 6p21, a chromosomal segment rearranged in a subset of ordinary lipomas. HMGI-C or HMGI(Y) protein expression was analyzed immunohistochemically in a group of 39 well differentiated adipose neoplasms (19 lipomas and 20 ALTs) of known karyotype using polyclonal antibodies raised against a recombinant protein (HMGI-C) and against a synthetic peptide (HMGI(Y)) Tbe results of this study demonstrate that HMGI proteins are commonly expressed in well differentiated adipose neoplasms. Seventeen of twenty ALTS (85.0%), all of which had ring or giant marker chromosomes with amplification of 12q13-15, strongly expressed HMGI-C. HMGI-C expression was detected in 7 of 11 ordinary lipomas (63.6%) with alterations at 12q14-15 and in one case with an abnormal karyotype that included double minute chromosomes. HMGI-C immunoreactivity correlates with 12q13-15 chromosomal alterations (P = 0.001). HMGI(Y) reactivity was demonstrated in only two ordinary lipomas: one with 6p21 rearrangement and one with normal karyotype. No significant HMGI(Y) expression was found in the ALT group. The finding of aberrant expression of HMGI proteins in well differentiated adipose neoplasms ill association with 12q13-15 and 6p21 chromosomal changes supports the proposed pathogenetic role of this group of proteins in the development of adipose tissue tumors.

33. Epigenetic Contribution of High-Mobility Group A Proteins to Stem Cell Properties.

Author

Giancotti V, Bergamin N, Cataldi P, and Rizzi C

Abstract

High-mobility group A (HMGA) proteins have been examined to understand their participation as structural epigenetic chromatin factors that confer stem-like properties to embryonic stem cells (ESCs), induced pluripotent stem cells (iPSCs), and cancer stem cells (CSCs). The function of HMGA was evaluated in conjunction with that of other epigenetic factors such as histones and microRNAs (miRs), taking into consideration the posttranscriptional modifications (PTMs) of histones (acetylation and methylation) and DNA methylation. HMGA proteins were coordinated or associated with histone and DNA modification and the expression of the factors related to pluripotency. CSCs showed remarkable differences compared with ESCs and iPSCs.

Published

2018

34. Translating Proteomic Into Functional Data: An High Mobility Group A1 (HMGA1) Proteomic Signature Has Prognostic Value in Breast Cancer.

Author

Maurizio E, Wiśniewski JR, Ciani Y, Amato A, Arnoldo L, Penzo C, Pegoraro S, Giancotti V, Zambelli A, Piazza S, Manfioletti G, and Sgarra R

Subjects

ATPases Associated with Diverse Cellular Activities, Blotting, Western, Breast Neoplasms diagnosis, Breast Neoplasms genetics, Carrier Proteins genetics, Carrier Proteins metabolism, Cell Cycle Proteins, Cell Line, Tumor, Disease-Free Survival, Gene Expression Regulation, Neoplastic, HMGA1a Protein genetics, Humans, Immunohistochemistry, Kaplan-Meier Estimate, Kinesins genetics, Kinesins metabolism, Mass Spectrometry, Membrane Proteins genetics, Membrane Proteins metabolism, Multivariate Analysis, Prognosis, Proteome genetics, RNA Interference, Reverse Transcriptase Polymerase Chain Reaction, Translational Research, Biomedical methods, Breast Neoplasms metabolism, HMGA1a Protein metabolism, Proteome metabolism, Proteomics methods

Abstract

Cancer is a very heterogeneous disease, and biological variability adds a further level of complexity, thus limiting the ability to identify new genes involved in cancer development. Oncogenes whose expression levels control cell aggressiveness are very useful for developing cellular models that permit differential expression screenings in isogenic contexts. HMGA1 protein has this unique property because it is a master regulator in breast cancer cells that control the transition from a nontumorigenic epithelial-like phenotype toward a highly aggressive mesenchymal-like one. The proteins extracted from HMGA1-silenced and control MDA-MB-231 cells were analyzed using label-free shotgun mass spectrometry. The differentially expressed proteins were cross-referenced with DNA microarray data obtained using the same cellular model and the overlapping genes were filtered for factors linked to poor prognosis in breast cancer gene expression meta-data sets, resulting in an HMGA1 protein signature composed of 21 members (HRS, HMGA1 reduced signature). This signature had a prognostic value (overall survival, relapse-free survival, and distant metastasis-free survival) in breast cancer. qRT-PCR, Western blot, and immunohistochemistry analyses validated the link of three members of this signature (KIFC1, LRRC59, and TRIP13) with HMGA1 expression levels both in vitro and in vivo and wound healing assays demonstrated that these three proteins are involved in modulating tumor cell motility. Combining proteomic and genomic data with the aid of bioinformatic tools, our results highlight the potential involvement in neoplastic transformation of a restricted list of factors with an as-yet-unexplored role in cancer. These factors are druggable targets that could be exploited for the development of new, targeted therapeutic approaches in triple-negative breast cancer., (© 2016 by The American Society for Biochemistry and Molecular Biology, Inc.)

Published

2016

35. Analysis of regioisomers of polyunsaturated triacylglycerols in marine matrices by HPLC/HRMS.

Author

Baiocchi C, Medana C, Dal Bello F, Giancotti V, Aigotti R, and Gastaldi D

Subjects

Animals, Chromatography, High Pressure Liquid, Lipase metabolism, Tandem Mass Spectrometry, Temperature, Tuna, Fatty Acids, Omega-3 analysis, Fish Oils chemistry, Triglycerides analysis

Abstract

Natural sources of triacylglycerols containing ω-3 fatty acids are of particular interest due to their protective role against several human diseases. However, as it has been well ascertained, the position of the ω-3 fatty acid on the triacylglycerol backbone influences how digestion occurs. In particular, occurrence at the sn-2 position allows optimal intestinal absorption conditions. The analytical protocol for regioisomer characterisation of fatty acids in a triacylglycerol usually requires the use of stereospecific lipases before instrumental identification. In this paper, we propose a more direct instrumental determination of triacylglycerol composition along with sn-2 positional identification of the fatty acids constituents by Liquid Chromatography-High Resolution Mass Spectrometry. Different intensities of product signals obtained in MS(2) and MS(3) experiments were used to define an interpretative scheme able to rationalise the stereochemistry of the TAGs. Marine matrices like tuna and algae oils have been studied in detail, their triacylglycerols identified and sn-2 positional arrangement of fatty acid constituents assessed., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published

2015

36. Fate of selected pharmaceuticals in river waters.

Author

Calza P, Medana C, Padovano E, Giancotti V, and Minero C

Subjects

Anti-Bacterial Agents radiation effects, Anticonvulsants radiation effects, Carbamazepine radiation effects, Chromatography, High Pressure Liquid, Clarithromycin radiation effects, Environmental Monitoring, Italy, Lincomycin radiation effects, Mass Spectrometry, Photolysis, Water Pollutants, Chemical radiation effects, Water Pollution, Chemical analysis, Anti-Bacterial Agents analysis, Anticonvulsants analysis, Carbamazepine analysis, Clarithromycin analysis, Lincomycin analysis, Rivers chemistry, Water Pollutants, Chemical analysis

Abstract

The aqueous environmental fate of two antibiotics, lincomycin and clarithromycin, and an antiepileptic drug, carbamazepine, was investigated by monitoring drugs decomposition and identifying intermediates in Po river water (North Italy). Initially, control experiments in the dark and under illumination were performed on river water spiked with drugs to simulate all possible transformation processes occurring in the aquatic system. Under illumination, these pharmaceuticals were degraded and transformed into numerous organic intermediate compounds. Several species were formed and characterised by analysing MS and MS(n) spectra and by comparison with parent molecule fragmentation pathways. River water was sampled at three sampling points in an urban area. The selected pharmaceuticals were detected in all samples. Eight transformation products identified in the laboratory simulation were found in natural river water from carbamazepine degradation, three from clarithromycin and two from lincomycin. Their transformation occurring in aquatic system mainly involved mono- and poly-hydroxylation followed by oxidation of the hydroxyl groups.

Published

2013

37. Effect of prolonged refrigeration on the lipid profile, lipase activity, and oxidative status of human milk.

Author

Bertino E, Giribaldi M, Baro C, Giancotti V, Pazzi M, Peila C, Tonetto P, Arslanoglu S, Moro GE, Cavallarin L, and Gastaldi D

Subjects

Antioxidants analysis, Antioxidants metabolism, Dietary Fats metabolism, Enzyme Stability, Fatty Acids analysis, Fatty Acids metabolism, Fatty Acids, Nonesterified analysis, Fatty Acids, Nonesterified metabolism, Female, Humans, Hydrogen-Ion Concentration, Italy, Lipid Peroxides analysis, Lipid Peroxides metabolism, Lipoprotein Lipase metabolism, Malondialdehyde analysis, Malondialdehyde metabolism, Milk, Human enzymology, Milk, Human metabolism, Postpartum Period, Refrigeration, Time Factors, Dietary Fats analysis, Food Storage, Lipase metabolism, Lipid Peroxidation, Lipolysis, Milk, Human chemistry

Abstract

Objective: The study was aimed at evaluating the effect of prolonged refrigeration of fresh human milk (HM) on its fatty acid profile, free fatty acid content, lipase activities, and oxidative status., Methods: HM from mothers of preterm newborns was collected, pooled, and placed in the neonatal intensive care unit (NICU) refrigerator. Pooled milk was aliquoted and analyzed within 3 hours of collection, and after 24, 48, 72, and 96 hours of storage. The milk samples were analyzed for pH, total and free fatty acid profile, lipase activity at room temperature and at 4°C, lipase activity at room temperature in presence of sodium cholate (bile salt-dependent lipase), total antioxidant capacity, thiobarbituric acid reactive species, malondialdehyde, and conjugated diene concentration. The experiment was replicated in 3 independent trials., Results: Prolonged refrigeration did not affect the fatty acid composition of breast milk, and preserved both its overall oxidative status and the activity of HM lipolytic enzymes. In particular, bile salt-dependent lipase activity, long-chain polyunsaturated fatty acids, and medium-chain saturated fatty acid concentrations were unaffected for up to 96 hours of refrigerated storage., Conclusions: Prolonged refrigeration of fresh HM for 96 hours maintained its overall lipid composition. The limited lipolysis during storage should be ascribed to the activity of lipoprotein lipase, responsible for the decrease in pH. Our study demonstrates that infants who receive expressed milk stored for up to 96 hours receive essentially the same supply of fatty acids and active lipases as do infants fed directly at the breast.

Published

2013

38. The expression of the high-mobility group A2 protein in colorectal cancer and surrounding fibroblasts is linked to tumor invasiveness.

Author

Rizzi C, Cataldi P, Iop A, Isola M, Sgarra R, Manfioletti G, and Giancotti V

Subjects

Adult, Aged, Aged, 80 and over, Biomarkers metabolism, Cell Communication genetics, Colorectal Neoplasms genetics, Female, HMGA2 Protein biosynthesis, Humans, Male, Middle Aged, Neoplasm Invasiveness pathology, Young Adult, Colorectal Neoplasms metabolism, Colorectal Neoplasms pathology, Fibroblasts metabolism, Fibroblasts pathology, HMGA2 Protein genetics

Abstract

Tumor staging of colorectal cancer is typically based on conventional TNM and Dukes classifications. However, additional information could be useful, and there is a significant interest in identifying molecular markers that are related to genetic or epigenetic processes. Using immunohistochemistry, we analyzed the expression of the high-mobility group A2 (previously high-mobility group 1-C [HMGI-C]) protein in 103 colorectal cancer cases to determine its use as a biomarker in colorectal cancer to integrate morphological staging. We found a progressive increase of the high-mobility group A2 protein expression in colorectal cancer tumor samples from cases in which all of the tumor cells were negative up to cases in which all of the tumor cells stained positive. Increased high-mobility group A2 expression is strongly associated with an increase in tumor invasiveness, which was measured through both budding and vascular invasion (P < .0001). Kaplan-Meier estimates showed a decrease in overall survival when vascular invasion is present (P = .023). Moreover, a fraction of the analyzed samples showed high-mobility group A2-positive stromal fibroblasts. Although high-mobility group A2-positive tumors were associated with cell invasiveness, high-mobility group A2-positive stromal fibroblasts were correlated with less invasive tumors. High-mobility group A2 protein expression could be used as a prognostic marker to provide prospective information on patient outcome, complementing the data obtained using conventional pathologic staging systems., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013

39. Qualitative characterization of Desmodium adscendens constituents by high-performance liquid chromatography-diode array ultraviolet-electrospray ionization multistage mass spectrometry.

Author

Baiocchi C, Medana C, Giancotti V, Aigotti R, Dal Bello F, Massolino C, Gastaldi D, and Grandi M

Subjects

Alkaloids analysis, Alkaloids chemistry, Oleanolic Acid analogs & derivatives, Oleanolic Acid analysis, Oleanolic Acid chemistry, Saponins analysis, Saponins chemistry, Spectrophotometry, Ultraviolet methods, Chromatography, High Pressure Liquid methods, Fabaceae chemistry, Plant Extracts chemistry, Spectrometry, Mass, Electrospray Ionization methods

Abstract

The many effects of the African medicinal herb Desmodium adscendens were studied in the 1980s and 1990s. In spite of this, a comprehensive analytical protocol for the quality control of its constituents (soyasaponins, alkaloids and flavonoids) has not yet been formulated and reported. This study deals with the optimization of extraction conditions from the plant and qualitative identification of the constituents by HPLC-diode array UV and multistage mass spectrometry. Plant constituents were extracted from leaves by liquid-liquid and solid matrix dispersion extraction. Separation was achieved via RP-C18 liquid chromatographywith UV and MS(n) detection and mass spectrometry analysis was conducted by electrospray ionization ion trap or orbitrap mass spectrometry. High resolution mass spectrometry (HRMS) was used for structural identification of active molecules relating to soyasaponins and alkaloids. The flavonoid fragmentations were preliminarily studied by HRMS in order to accurately characterize the more common neutral losses. However, the high number of isomeric species induced us to make recourse to a more extended chromatographic separation in order to enable useful tandem mass spectrometry and ultraviolet spectral interpretation to propose a reasonable chemical classification of these polyphenols. 35 compounds of this class were identified herein with respect to the five reported in literature in this way we made up a comprehensive protocol for the qualitative analysis of the high complexity content of this plant. This result paves the way for both reliable quality control of potential phytochemical medicaments and possible future systematic clinical studies.

Published

2013

40. Study of the photocatalytic transformation of synephrine: a biogenic amine relevant in anti-doping analysis.

Author

Medana C, Calza P, Giancotti V, Dal Bello F, Aragno M, and Baiocchi C

Subjects

Animals, Biogenic Amines blood, Biogenic Amines urine, Biotransformation radiation effects, Dietary Supplements analysis, Dietary Supplements radiation effects, Doping in Sports, Female, Humans, Male, Photolysis, Rats, Rats, Wistar, Synephrine blood, Synephrine urine, Biogenic Amines chemistry, Chromatography, High Pressure Liquid methods, Mass Spectrometry methods, Synephrine chemistry

Abstract

The occurrence of some cases of positive results in anti-doping analysis of octopamine requires clarification as to whether its methylated derivative synephrine could be a metabolic precursor of octopamine itself. Synephrine is a natural phenylethylamine derivative present in some food supplements containing Citrus aurantium, permitted in sport regulations. A simulative laboratory study had been done using a photocatalytic process, to identify all possible main and secondary transformation products, in a clean matrix; these were then sought in biological samples obtained from three human volunteers and four rats treated with synephrine; the parent compound and its new potential metabolic products were investigated in human urine and rat plasma samples. The transformation of synephrine and octopamine and the formation of intermediate products were evaluated, adopting titanium dioxide as photocatalyst. Several products were formed and characterized using the HPLC-HRMS(n) technique. The main intermediates identified in these experimental conditions were compared with the major synephrine metabolites found in in vivo studies on rats and humans. Some more oxidized species, already formed in the photocatalytic process, were also found in urine and plasma samples of treated animals. These new findings could be of interest in further metabolism studies. The main photocatalytic pathway involving synephrine appears to be N-demethylation to give octopamine. On the contrary, we demonstrate the inconsistency of this reaction in both rat and human in vivo determinations, resulting in forensic importance.

Published

2013

41. Identification of the unknown transformation products derived from clarithromycin and carbamazepine using liquid chromatography/high-resolution mass spectrometry.

Author

Calza P, Medana C, Padovano E, Giancotti V, and Baiocchi C

Subjects

Carbamazepine analogs & derivatives, Carbamazepine metabolism, Carbon, Clarithromycin analogs & derivatives, Clarithromycin metabolism, Hydroxylation, Photolysis, Water Pollutants, Chemical metabolism, Carbamazepine chemistry, Chromatography, Liquid methods, Clarithromycin chemistry, Mass Spectrometry methods, Water Pollutants, Chemical chemistry

Abstract

Rationale: A comprehensive study of the environmental fate of pollutants is more and more required, above all on new contaminants, i.e. pharmaceuticals. As high-resolution mass spectrometry (HRMS(n)) may be a suitable analytical approach for characterization of unknown compounds, its performance was evaluated in this study., Methods: The analyses were carried out using liquid chromatography (LC) (electrospray ionization (ESI) in positive mode) coupled with a LTQ-Orbitrap analyzer. High-resolution mass spectrometry was employed to assess the evolution of the drug transformation processes over time; accurate masses of protonated molecular ions and sequential product ions were reported with an error below 5 millimass units, which guarantee the correct assignment of their molecular formula in all cases, while their MS(2) and MS(3) spectra showed several structurally diagnostic ions that allowed characterization of the different transformation products (TPs) and to distinguish the isobaric species., Results: The simulation of phototransformation occurring in the aquatic environment and identification of biotic and abiotic transformation products of the two pharmaceuticals were carried out in heterogeneous photocatalysis using titanium dioxide, aimed to recreate conditions similar to those found in the environmental samples. Twenty-eight main species were identified after carbamazepine transformation and twenty-nine for clarithromycin., Conclusions: This study demonstrates that HRMS, combined with LC, is a technique able to play a key role in the evaluation of the environmental fate of pollutants and allows elucidation of the transformation pathways followed by the two drugs., (Copyright © 2012 John Wiley & Sons, Ltd.)

Published

2012

42. Characterization of phenazone transformation products on light-activated TiO2 surface by high-resolution mass spectrometry.

Author

Calza P, Medana C, Raso E, Giancotti V, and Minero C

Subjects

Antipyrine toxicity, Hydroxylation, Light, Photolysis, Rivers chemistry, Toxicity Tests, Water chemistry, Water Pollutants, Chemical chemistry, Water Pollutants, Chemical toxicity, Antipyrine chemistry, Antipyrine radiation effects, Mass Spectrometry methods, Titanium chemistry

Abstract

The paper examines the transformation of phenazone (2,3-dimethyl-1-phenyl-3-pyrazolin-5-one), a widely used analgesic and antipyretic drug, under simulated solar irradiation in pure water, using titanium dioxide, and in river water. High-resolution mass spectrometry was employed to monitor the evolution of photoinduced processes. Initially, laboratory experiments were performed to simulate drug-transformation pathways in aqueous solution, using TiO(2) as photocatalyst. Thirteen main phenazone transformation products were detected, and full analysis of their MS and MS(n) spectra identified the diverse isobaric species. All these transformation products were themselves easily degraded, and no compounds were recognized to remain until 1h of irradiation. From these findings, a tentative degradation pathway is proposed to account for the photoinduced transformation of phenazone in natural waters. These simulation experiments were verified in the field, seeking phenazone in River Po water samples., (Copyright © 2011 John Wiley & Sons, Ltd.)

Published

2011

43. Horse metabolism and the photocatalytic process as a tool to identify metabolic products formed from dopant substances: the case of sildenafil.

Author

Medana C, Calza P, Giancotti V, Dal Bello F, Pasello E, Montana M, and Baiocchi C

Subjects

Animals, Chromatography, High Pressure Liquid methods, Doping in Sports, Horses blood, Horses urine, Phosphodiesterase 5 Inhibitors blood, Phosphodiesterase 5 Inhibitors urine, Photochemical Processes, Piperazines blood, Piperazines urine, Purines blood, Purines metabolism, Purines urine, Sildenafil Citrate, Sulfones blood, Sulfones urine, Horses metabolism, Phosphodiesterase 5 Inhibitors metabolism, Piperazines metabolism, Substance Abuse Detection methods, Sulfones metabolism

Abstract

Two horses were treated with sildenafil, and its metabolic products were sought in both urine and plasma samples. Prior to this, a simulative laboratory study had been done using a photocatalytic process, to identify all possible main and secondary transformation products, in a clean matrix; these were then sought in the biological samples. The transformation of sildenafil and the formation of intermediate products were evaluated adopting titanium dioxide as photocatalyst. Several products were formed and characterized using the HPLC/HRMS(n) technique. The main intermediates identified in these experimental conditions were the same as the major sildenafil metabolites found in in vivo studies on rats and horses. Concerning horse metabolism, sildenafil and the demethylated product (UK 103,320) were quantified in blood samples. Sildenafil propyloxide, de-ethyl, and demethyl sildenafil, were the main metabolites quantified in urine. Some more oxidized species, already formed in the photocatalytic process, were also found in urine and plasma samples of treated animals. Their formation involved hydroxylation on the aromatic ring, combined oxidation and dihydroxylation, N-demethylation on the pyrazole ring, and hydroxylation. These new findings could be of interest in further metabolism studies., (Copyright © 2011 John Wiley & Sons, Ltd.)

Published

2011

44. N,N-diethyl-m-toluamide transformation in river water.

Author

Calza P, Medana C, Raso E, Giancotti V, and Minero C

Subjects

DEET analysis, Insect Repellents analysis, Italy, Mass Spectrometry, Water Pollutants, Chemical analysis, DEET chemistry, Insect Repellents chemistry, Rivers chemistry, Water Pollutants, Chemical chemistry

Abstract

The paper deals with the aqueous environmental fate of N,N-diethyl-m-toluamide (DEET), one of the most widespread and efficient mosquito repellents. The investigation involved monitoring of the DEET decomposition and the identification of intermediate compounds. Initially, control experiments in the dark and under illumination were performed on sterilized and river water spiked with DEET, with the aim to simulate all possible transformation processes occurring in aquatic system. Under illumination, DEET was degraded and transformed into numerous organic intermediate compounds, 37 of which could be identified. Several isomeric species were formed and characterized by analysing MS and MS(n) spectra, and by comparison with parent molecule fragmentation pathways. These laboratory simulation experiments were verified in the field to check the mechanism previously supposed. River water was sampled and analysed at eight sampling points. Among the transformation products (TPs) identified in river water spiked with DEET, twelve of them were also found in natural river water. The transformation occurring in aquatic systems involved dealkylation, mono- and poly-hydroxylation followed by oxidation of the hydroxyl groups and cleavage of the alkyl chains. Two TPs were principally formed in dark condition, while the others are mainly produced through indirect photolysis processes mediated by natural photosensitizers., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2011

45. Conformational role for the C-terminal tail of the intrinsically disordered high mobility group A (HMGA) chromatin factors.

Author

Maurizio E, Cravello L, Brady L, Spolaore B, Arnoldo L, Giancotti V, Manfioletti G, and Sgarra R

Subjects

Amino Acid Sequence, Cell Transformation, Neoplastic genetics, Cell Transformation, Neoplastic metabolism, Chromatin metabolism, HMGA Proteins genetics, HMGA Proteins metabolism, Humans, Methylation, Molecular Sequence Data, Phosphorylation, Protein Processing, Post-Translational, Protein Structure, Tertiary, Recombinant Proteins genetics, Recombinant Proteins metabolism, Spectrometry, Mass, Electrospray Ionization, Static Electricity, Chromatin chemistry, HMGA Proteins chemistry, Proteomics methods, Recombinant Proteins chemistry

Abstract

The architectural factors HMGA are highly connected hubs in the chromatin network and affect key cellular functions. HMGA have a causal involvement in cancer development; in fact, truncated or chimeric HMGA forms, resulting from chromosomal rearrangements, lack the constitutively phosphorylated acidic C-terminal tail and display increased oncogenic potential, suggesting a functional role for this domain. HMGA belong to the intrinsically disordered protein category, and this prevents the use of classical approaches to obtain structural data. Therefore, we combined limited proteolysis, ion mobility separation-mass spectrometry (IMS-MS), and electrospray ionization-mass spectrometry (ESI-MS) to obtain structural information regarding full length and C-terminal truncated HMGA forms. Limited proteolysis indicates that HMGA acidic tail shields the inner portions of the protein. IMS-MS and ESI-MS show that HMGA proteins can assume a compact form and that the degree of compactness is dependent upon the presence of the acidic tail and its constitutive phosphorylations. Moreover, we demonstrate that C-terminal truncated forms and wild type proteins are post-translationally modified in a different manner. Therefore, we propose that the acidic tail and its phosphorylation could affect HMGA post-translational modification status and likely their activity. Finally, the mass spectrometry-based approach adopted here proves to be a valuable new tool to obtain structural data regarding intrinsically disordered proteins.

Published

2011

46. Determination of carnosine, anserine, homocarnosine, pentosidine and thiobarbituric acid reactive substances contents in meat from different animal species.

Author

Peiretti PG, Medana C, Visentin S, Giancotti V, Zunino V, and Meineri G

Abstract

The aim of this research was to determine the content of the histidinic antioxidants, advanced glycation end products (pentosidine) and thiobarbituric acid reactive substance (TBARS) in the meat from different animal species. Carnosine, anserine, homocarnosine and pentosidine were quantified by HPLC/MS, while TBARS was determined by photometric measurements. The total CRCs (carnosine+anserine+homocarnosine) content was in the increasing order: beef

Published

2011

47. Microwave-assisted Maillard reactions for the preparation of advanced glycation end products (AGEs).

Author

Visentin S, Medana C, Barge A, Giancotti V, and Cravotto G

Subjects

Arginine analogs & derivatives, Arginine chemical synthesis, Arginine chemistry, Chromatography, High Pressure Liquid, Chromatography, Liquid, Glycation End Products, Advanced chemistry, Gold Compounds chemical synthesis, Gold Compounds chemistry, Imidazoles chemical synthesis, Imidazoles chemistry, Indicators and Reagents, Kinetics, Lysine analogs & derivatives, Lysine chemical synthesis, Lysine chemistry, Mass Spectrometry, Glycation End Products, Advanced chemical synthesis, Maillard Reaction radiation effects, Microwaves

Abstract

The application of microwaves as an efficient form of volumetric heating to promote organic reactions was recognized in the mid-1980 s. It has a much longer history in the food research and industry where microwave irradiation was studied in depth to optimize food browning and the development of desirable flavours from Maillard reactions. The microwave-promoted Maillard reaction is a challenging synthetic method to generate molecular diversity in a straightforward way. In this paper we present a new rapid and efficient one-pot procedure for the preparation of pentosidine and other AGEs under microwave irradiation.

Published

2010

48. HMGA molecular network: From transcriptional regulation to chromatin remodeling.

Author

Sgarra R, Zammitti S, Lo Sardo A, Maurizio E, Arnoldo L, Pegoraro S, Giancotti V, and Manfioletti G

Subjects

Animals, Humans, Models, Biological, Chromatin Assembly and Disassembly genetics, Gene Regulatory Networks, HMGA Proteins metabolism, Transcription, Genetic

Abstract

Nuclear functions rely on the activity of a plethora of factors which mostly work in highly coordinated molecular networks. The HMGA proteins are chromatin architectural factors which constitute critical hubs in these networks. HMGA are referred to as oncofetal proteins since they are highly expressed and play essential functions both during embryonic development and neoplastic transformation. A particular feature of HMGA is their intrinsically disordered status, which confers on them an unusual plasticity in contacting molecular partners. Indeed these proteins are able to bind to DNA at the level of AT-rich DNA stretches and to interact with several nuclear factors. In the post-genomic era, and with the advent of proteomic tools for the identification of protein-protein interactions, the number of HMGA molecular partners has increased rapidly. This has led to the extension of our knowledge of the functional involvement of HMGA from the transcriptional regulation field to RNA processing, DNA repair, and chromatin remodeling and dynamics. This review focuses mainly on the protein-protein interaction network of HMGA and its functional outcome. HMGA molecular partners have been functionally classified and all the information collected in a freely available database (http://www.bbcm.units.it/ approximately manfiol/INDEX.HTM)., (Copyright 2009 Elsevier B.V. All rights reserved.)

Published

2010

49. Macroscopic differences in HMGA oncoproteins post-translational modifications: C-terminal phosphorylation of HMGA2 affects its DNA binding properties.

Author

Sgarra R, Maurizio E, Zammitti S, Lo Sardo A, Giancotti V, and Manfioletti G

Subjects

Amino Acid Sequence, Cell Line, Tumor, Chromatography, Liquid, HMGA Proteins genetics, HMGA Proteins metabolism, HMGA2 Protein genetics, HMGN Proteins genetics, HMGN Proteins metabolism, Humans, Mass Spectrometry, Methylation, Molecular Sequence Data, Neoplasms metabolism, Phosphorylation, Protein Binding, Protein Interaction Mapping, Sequence Alignment, Serine metabolism, HMGA Proteins chemistry, HMGA2 Protein chemistry, HMGA2 Protein metabolism, HMGN Proteins chemistry, Protein Processing, Post-Translational

Abstract

HMGA is a family of nuclear proteins involved in a huge number of functions at the chromatin level. It consists of three members, HMGA1a, HMGA1b, and HMGA2, having high sequence homology and sharing the same structural organization (three highly conserved DNA-binding domains, an acidic C-terminal tail, and a protein-protein interaction domain). They are considered important nodes in the chromatin context, establishing a complex network of interactions with both promoter/enhancer sequences and nuclear factors. They are involved in a plethora of biological processes and their activities are finely tuned by several different post-translational modifications. We have performed an LC/MS screening on several different cell lines to investigate HMGA proteins expression and their post-translational modifications in order to detect distinctive modification patterns for each. Our analyses evidenced relevant macroscopic differences in the phosphorylation and methylation patterns of these proteins. These differences occur both within the HMGA family members and in the different cell types. Focusing on HMGA2, we have mapped its in vivo phosphorylation sites demonstrating that, similarly to the HMGA1 proteins, it is highly phosphorylated on the acidic C-terminal tail and that these modifications affect its DNA binding properties.

Published

2009

50. Interaction proteomics of the HMGA chromatin architectural factors.

Author

Sgarra R, Furlan C, Zammitti S, Lo Sardo A, Maurizio E, Di Bernardo J, Giancotti V, and Manfioletti G

Subjects

Animals, Cell Transformation, Neoplastic, Chromatography, Liquid, DNA Repair, Electrophoresis, Gel, Two-Dimensional, Gene Regulatory Networks, High Mobility Group Proteins genetics, Humans, Immunoblotting, Mice, RNA Processing, Post-Transcriptional, Recombinant Proteins genetics, Recombinant Proteins metabolism, Tandem Mass Spectrometry, Chromatin metabolism, High Mobility Group Proteins metabolism, Protein Interaction Domains and Motifs, Protein Interaction Mapping, Proteomics methods

Abstract

The high mobility group A (HMGA) chromatin architectural transcription factors are a group of proteins involved in development and neoplastic transformation. They take part in an articulated interaction network, both with DNA and other nuclear proteins, organizing multimolecular complexes at chromatin level. Here, we report the development of a novel in vitro strategy for the identification of HMGA molecular partners based on the combination of an RP-HPLC prefractionation procedure, 2-DE gels, blot-overlay and MS. To demonstrate that our approach could be a reliable screening method we confirmed a representative number of interactions in vitro by GST pull-down and far-Western and in vivo by co-affinity purification. This approach allowed us to enlarge the HMGA molecular network confirming their involvement also in non-transcriptional-related processes such as RNA processing and DNA repair.

Published

2008