Your search keyword '"Fini C"' showing total 9 results

1. The ecto-5'-nucleotidase subunits in dimers are not linked by disulfide bridges but by non-covalent bonds.

Author

Martínez-Martínez A, Muñoz-Delgado E, Campoy FJ, Flores-Flores C, Rodríguez-López JN, Fini C, and Vidal CJ

Subjects

Animals, Cattle, Centrifugation, Density Gradient, Chromatography, High Pressure Liquid, Dimerization, Dithiothreitol, Electrophoresis, Polyacrylamide Gel, Guanidine, Male, Protein Structure, Quaternary, Urea, 5'-Nucleotidase chemistry, Sulfhydryl Compounds chemistry

Abstract

It has long been considered that ecto-5'-nucleotidase (eNT) dimers consist of subunits linked by disulfide bonds. Hydrophilic (6.7S) and amphiphilic (4.0S) dimers were separated by sedimentation analysis of eNT purified from bull seminal plasma. Hydrophilic (4. 2S) and amphiphilic (2.6S) eNT monomers were obtained after reduction of disulfide bonds in dimers. The amphiphilic eNT dimers or monomers were converted into their hydrophilic variants with phosphatidylinositol-specific phospholipase C. SDS-PAGE plus Western blot showed 68 kDa subunits, regardless of the addition of beta-mercaptoethanol to the SDS mixture. Active eNT monomers were obtained by addition of 1 M guanidinium chloride (Gdn) to dimers, and unfolded subunits by addition of 4 M Gdn. The results unambiguously demonstrate that the subunits in eNT dimers are not linked by disulfide bridges, but by non-covalent bonds, and that dissociation precedes inactivation and unfolding.

Published

2000

2. Porcine odorant-binding protein: structural stability and ligand affinities measured by fourier-transform infrared spectroscopy and fluorescence spectroscopy.

Author

Paolini S, Tanfani F, Fini C, Bertoli E, and Paolo Pelosi

Subjects

Animals, Anthracenes, Binding, Competitive, Ligands, Molecular Structure, Protein Structure, Secondary, Spectrometry, Fluorescence, Spectroscopy, Fourier Transform Infrared, Swine, Temperature, Nasal Mucosa chemistry, Receptors, Odorant chemistry

Abstract

Infrared spectra show that the binding of the odorants 2-isobuthyl-3-methoxypyrazine (PYR) and 3,7-dimethyl-1-octanol (DMO) stabilises the tertiary structure of porcine OBP-I against thermal denaturation. The fluorescence emission spectrum of the single tryptophan shows a lambdamax at 337 nm, indicating that the residue is not directly exposed to the solvent. Tryptophan does not appear to be involved in the odorant binding process and it is not accessible to the fluorescence quenchers NaI, CsCl and acrylamide. The binding of the fluorescent dye 1-aminoanthracene (1-AMA), a strong ligand, does not modify the tryptophan fluorescence spectrum. In contrast, the lambdamax of 1-AMA bound to OBP-I is shifted from 537 to 481 nm, with a lambdamax intensity increase by a factor of 80. Bound 1-AMA is displaced by odorant molecules in competitive binding assays and can be employed in simple and rapid binding assay, avoiding the use of radioactive ligands. The Scatchard plot shows that 1-AMA binds to OBP-I with a dissociation constant of 1.3 microM and an equimolar stoichiometry.

Published

1999

3. Biochemical properties of 5'-nucleotidase from mouse skeletal muscle.

Author

Martínez-Martínez A, Flores-Flores C, Campoy FJ, Muñoz-Delgado E, Fini C, and Vidal CJ

Subjects

5'-Nucleotidase antagonists & inhibitors, 5'-Nucleotidase metabolism, Animals, Cations, Divalent pharmacology, Centrifugation, Density Gradient, Chromatography, Affinity, Mice, Molecular Weight, Nucleotidases metabolism, Substrate Specificity, Zinc analysis, 5'-Nucleotidase isolation & purification, Muscle, Skeletal enzymology

Abstract

Ecto-5'-nucleotidase (eNT) from mouse muscle has been purified after extraction with detergent followed by chromatography on concanavalin A- and AMP-Sepharose. Three fractions were recovered: UF was NT non-retained in immobilised AMP; F-I was bound enzyme eluted with beta-glycerophosphate, and F-II was bound NT released with AMP. eNT was 80000-fold purified in F-II, this fraction showing proteins of 74, 68 and 51 kDa after immunoblotting. NT in UF migrated at 6.7S after centrifugation in sucrose gradients with Triton X-100, the peak being split into two of 6.7S and 4.4S in gradients with Brij 96. Ecto-NT in F-I or F-II migrated at 5.8S in Triton X-100-, or 4.4S in Brij 96-containing gradients. The hydrodynamic behaviour, concentration in Triton X-114, binding to phenyl-agarose, and sensitivity to phosphatidylinositol-specific phospholipase C revealed that enzyme forms in F-I or F-II were amphiphilic dimers with linked phosphatidylinositol residues, whilst most of NT forms in UF were hydrophilic dimers. A zinc/protein molar ratio of 2.2 was determined for eNT in F-II. NT activity was decreased in assays made in imidazole buffer, and was partly restored with 10 microM Zn2+ or 100 microM Mn2+. In assays with Tris buffer, NT showed a Km for AMP of 12 microM, and was competitively inhibited by ATP or ADP.

Published

1998

4. Structural and functional relationships in 5'-nucleotidase from bull seminal plasma. A Fourier transform infrared study.

Author

Fini C, Bertoli E, Albertini G, Floridi A, and Tanfani F

Subjects

Animals, Cattle, Dithiothreitol metabolism, Fourier Analysis, Male, Nitrilotriacetic Acid metabolism, Protein Conformation, Spectrophotometry, Infrared, 5'-Nucleotidase metabolism, Semen enzymology

Abstract

Fourier transform infrared spectroscopy (FTIR) was used to investigate the secondary structure of 5'-nucleotidase from bull seminal plasma (BSP). Spectra of protein in both D2O and H2O were analyzed by deconvolution and second derivative methods in order to observe the overlapping components of the amide I band. The protein, which is made up of two apparently identical subunits and which contains two zinc atoms, was studied in its native form, in the presence of dithiotreitol (DTT) and after removal of the two zinc atoms by means of nitrilotriacetic acid (NTA). Deconvolved and second derivative spectra of amide I band showed that the native protein contains mostly beta-sheet structure with a minor content of alpha-helix. The quantitative analysis of the amide I components was performed by a curve-fitting procedure which revealed 54% beta-sheet, 18% alpha-helix, 22% beta-turns and 6% unordered structure. The second derivative and deconvolved spectra of amide I band showed that no remarkable changes in the secondary structure of 5'-nucleotidase were induced by either DTT or NTA. These results were confirmed by the curve-fitting analysis where little or no changes occurred in the relative content of amide I components when the protein was treated with DTT or with NTA. Major changes, however, were observed in the thermal denaturation behavior of the protein. The native protein showed denaturation at temperatures between 70 and 75 degrees C, while the maximum of denaturation was observed between 65 and 70 degrees C and between 55 and 60 degrees C in the presence of NTA and DTT, respectively. The results obtained indicate that the two separate subunits of the protein have essentially the same secondary structure as that of the native enzyme.

Published

1992

5. Purification of 5'-nucleotidase from human seminal plasma.

Author

Fini C, Coli M, and Floridi A

Subjects

5'-Nucleotidase metabolism, Animals, Blotting, Western, Cattle, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Humans, Male, Nucleotidases metabolism, Phosphatidylinositol Diacylglycerol-Lyase, Phosphoric Diester Hydrolases metabolism, 5'-Nucleotidase isolation & purification, Semen enzymology

Abstract

5'-Nucleotidase from human seminal plasma was purified to electrophoretic homogeneity and some of its kinetic and molecular properties compared with those of 5'-nucleotidase from bull seminal plasma. The purification of the enzyme was achieved by using the same affinity chromatography media (Con A-Sepharose and AMP-Agarose or ADP-Agarose) previously used for the purification of bull seminal plasma 5'-nucleotidase (Fini, C., Ipata, P.L., Palmerini, C.A. and Floridi, A. (1983) Biochim. Biophys. Acta 748, 405-412). However, in the present purification procedure no detergent was used as it had been necessary for the purification of the bovine enzyme. The experimental data reveal some main differences between these two enzymes; first, the human enzyme seems to be constituted of a single polypeptide chain of about 71 kDa, while the 5'-nucleotidase of bull seminal plasma, in non denaturing detergent solutions, is a homodimer of about 160 kDa. Another most remarkable difference is that the human enzyme does not seem to contain a phosphatidylinositol anchoring system like the one present in the bovine enzyme and in 5'-nucleotidase of different sources (Low, M.G. (1987) Biochem. J. 244, 1-13). Finally, the AMPase activity of 5'-nucleotidase from human seminal plasma is not affected by dithiothreitol which, on the contrary, is a powerful inhibitor of the bovine enzyme causing the dissociation of its subunits which are held together by disulphide bridges (Fini, C., Minelli, A., Camici, M. and Floridi, A. (1985) Biochem. Biophys. Acta 827, 403-409).

Published

1991

6. 5'-nucleotidase from bull seminal plasma, chicken gizzard and snake venom is a zinc metalloprotein.

Author

Fini C, Palmerini CA, Damiani P, Stochaj U, Mannherz HG, and Floridi A

Subjects

Animals, Apoenzymes, Cattle, Chickens, Cobalt pharmacology, Copper pharmacology, Gizzard, Avian enzymology, Metalloproteins, Nitrilotriacetic Acid pharmacology, Nucleotidases metabolism, Semen enzymology, Snake Venoms analysis, Snakes, 5'-Nucleotidase metabolism, Zinc metabolism

Abstract

Using flame atomic absorption spectrometry the tight association of zinc to three different purified 5'-nucleotidases at a molar ratio of 2 could be proven. These 5'-nucleotidases purified from bull seminal plasma (BSP), chicken gizzard (CG) and snake venom (SV) are thus zinc metalloproteins. Removal of zinc results in the loss of their AMPase activity, which could be fully restored after readdition of zinc at a molar ratio of 2, for BSP and CG, and 1.5, for SV 5'-nucleotidase. Reactivation of their AMPase activity after the removal of zinc could also be obtained by addition of cobalt and copper ions, which were found to also bind with a molar ratio of 2 to the three 5'-nucleotidases tested.

Published

1990

7. Effects of dithiothreitol, dithioerythritol and chelating agents on 5'-nucleotidase from bull seminal plasma.

Author

Fini C, Minelli A, Camici M, and Floridi A

Subjects

5'-Nucleotidase, Animals, Calcium Chloride pharmacology, Cattle, Chromatography, High Pressure Liquid, Disulfides metabolism, Edetic Acid pharmacology, Egtazic Acid pharmacology, Macromolecular Substances, Magnesium pharmacology, Magnesium Chloride, Male, Molecular Weight, Chelating Agents pharmacology, Dithioerythritol pharmacology, Dithiothreitol analogs & derivatives, Dithiothreitol pharmacology, Nucleotidases metabolism, Semen enzymology

Abstract

5'-Nucleotidase from bull seminal plasma is inhibited by dithiothreitol and dithioerythritol. These reactives proved to dissociate the dimeric glycoprotein 5'-nucleotidase of Mr 160 000 into two subunits of apparent Mr 80 000, indicating that the subunits are held together by interchain disulfide bridges. HPLC determinations of cysteic acid and carboxymethylcysteine protein derivatives resulted in 50 +/- 3 half-cystine plus cysteine residues, while 1.9 +/- 0.4 free cysteine residues were estimated by HPLC analysis. The enzyme is inhibited by EDTA and EGTA, and the inhibition appears to be of the non-competitive type for both the chelating agents. Experiments for the enzyme activity recovery by MgCl2 and CaCl2 additions, after the EDTA and EGTA treatments in the presence of 8 M urea, are reported.

Published

1985

8. Isolation and kinetic properties of 5'-nucleotidase from guinea-pig skeletal muscle.

Author

Camici M, Fini C, and Ipata PL

Subjects

5'-Nucleotidase, Animals, Cations, Divalent, Guinea Pigs, Hydrogen-Ion Concentration, Kinetics, Lectins pharmacology, Molecular Weight, Nucleotidases antagonists & inhibitors, Nucleotidases metabolism, Nucleotides pharmacology, Substrate Specificity, Thermodynamics, Muscles enzymology, Nucleotidases isolation & purification

Abstract

5'-Nucleotidase (EC 3.1.3.5) has been solubilized and purified 1200-fold from guinea-pig skeletal muscle, to a specific activity of 40 U/mg protein. The purified enzyme yields a single protein band on polyacrylamide gel electrophoresis in the presence of sodium dodecyl sulfate. Guinea-pig skeletal muscle 5'-nucleotidase is extremely sensitive to inhibition by nucleoside di- and triphosphates. The inhibition is of the competitive type, and can be reversed only by strong excess of Mg2+. Nucleoside diphosphates are more powerful inhibitors than nucleoside triphosphates. The Ki values for ADP and ATP are 0.036 and 0.28 microM, respectively. The purified enzyme does not require exogenous cations for maximal activity and is inhibited by EDTA. This inhibition is reversed by divalent cations. This indicates that the enzyme contains a tightly bound metal cation.

Published

1985

9. 5'-nucleotidase from bull seminal plasma.

Author

Fini C, Ipata PL, Palmerini CA, and Floridi A

Subjects

5'-Nucleotidase, Animals, Cattle, Male, Molecular Weight, Nucleotidases isolation & purification, Octoxynol, Polyethylene Glycols pharmacology, Substrate Specificity, Nucleotidases metabolism, Semen enzymology

Abstract

5'-Nucleotidase (5'-ribonucleotide phosphohydrolase, EC 3.1.3.5) occurs in bull seminal plasma in multiple forms. The heterogeneity does not reflect the existence of true isoenzymes, but is due to the association of the enzyme with particulate material and to molecular aggregation phenomena. Addition of detergents to native bull seminal plasma prevents molecular aggregation, solubilizes the particulate form of the enzyme, and results in the appearance of a single molecular form of the enzyme. Enzyme purification can be achieved after three chromatographic steps which involve negative adsorption of 5'-nucleotidase activity on DEAE-Sephadex A-50 followed by two affinity chromatographies on concanavalin A-Sepharose 4B and ADP-agarose. The enzyme appears to be a dimeric glycoprotein. Some properties of the enzyme, including substrate specificity and the effects of hydrogen ion concentration and of various divalent cations, are reported.

Published

1983