Your search keyword '"Fabio Tanfani"' showing total 116 results

1. Thermal stability, ligand binding and allergenicity data of Mus m 1.0102 allergen and its cysteine mutants

Author

Elena Ferrari, Romina Corsini, Samuele E. Burastero, Fabio Tanfani, and Alberto Spisni

Subjects

Computer applications to medicine. Medical informatics, R858-859.7, Science (General), Q1-390

Abstract

The presented data were obtained with the lipocalin allergen Mus m 1.0102 and its cysteine mutants MM-C138A, MM-C157A and MM-C138,157A, whose structural features and unfold reversibility investigations are presented in the research article entitled “The allergen Mus m 1.0102: cysteine residues and molecular allergology” [1].The data were obtained by means of a Dynamic Light Scattering-based thermal stability assay, a Fluorescence-based ligand-binding assay and a basophil degranulation test, and describe proteins’ fold stability, ligand binding ability and allergenic potential, respectively. Analysis of the collected data produced the temperatures corresponding to the onset of the protein unfolding, the dissociation constants for N-Phenyl-1-naphthylamine ligand and the profiles of β-hexosaminidase release from RBL SX-38 cells, sensitized with the serum of selected allergic patients and incubated with increasing antigens concentrations.These data allow for comparison of the lipocalin allergen Mus m 1.0102 with its conserved cysteines mutants and, with regard to their potential application in allergy diagnostics and immunotherapy, they contribute to the process of recombinant allergen characterization and standardization. Keywords: Lipocalin allergen, Mus m 1 allergen, Thermal stability, Aggregation

Published

2020

2. A Spectroscopic Study on Secondary Structure and Thermal Unfolding of the Plant Toxin Gelonin Confirms Some Typical Structural Characteristics and Unravels the Sequence of Thermal Unfolding Events

Author

Andrea Scirè, Fabio Tanfani, and Alessio Ausili

Subjects

Gelonin, Ribosome-inactivating protein, Infrared spectroscopy, Thermal unfolding, Two-dimensional correlation spectroscopy, Immunotoxins, Medicine

Abstract

Gelonin from the Indian plant Gelonium multiflorum belongs to the type I ribosome-inactivating proteins (RIPs). Like other members of RIPs, this toxin glycoprotein inhibits protein synthesis of eukaryotic cells; hence, it is largely used in the construction of immunotoxins composed of cell-targeted antibodies. Lysosomal degradation is one of the main issues in targeted tumor therapies, especially for type I RIP-based toxins, as they lack the translocation domains. The result is an attenuated cytosolic delivery and a decrease of the antitumor efficacy of these plant-derived toxins; therefore, strategies to permit their release from endosomal vesicles or modifications of the toxins to make them resistant to degradation are necessary to improve their efficacy. Using infrared spectroscopy, we thoroughly analyzed both the secondary structure and the thermal unfolding of gelonin. Moreover, by the combination of two-dimensional correlation spectroscopy and phase diagram method, it was possible to deduce the sequence of events during the unfolding, confirming the typical characteristic of the RIP members to denature in two steps, as a sequential loss of tertiary and secondary structure was detected at 58 °C and at 65 °C, respectively. Additionally, some discrepancies in the unfolding process between gelonin and saporin-S6, another type I RIP protein, were detected.

Published

2019

3. Analysis of the link between the redox state and enzymatic activity of the HtrA (DegP) protein from Escherichia coli.

Author

Tomasz Koper, Agnieszka Polit, Anna Sobiecka-Szkatula, Katarzyna Wegrzyn, Andrea Scire, Donata Figaj, Leszek Kadzinski, Urszula Zarzecka, Dorota Zurawa-Janicka, Bogdan Banecki, Adam Lesner, Fabio Tanfani, Barbara Lipinska, and Joanna Skorko-Glonek

Subjects

Medicine, Science

Abstract

Bacterial HtrAs are proteases engaged in extracytoplasmic activities during stressful conditions and pathogenesis. A model prokaryotic HtrA (HtrA/DegP from Escherichia coli) requires activation to cleave its substrates efficiently. In the inactive state of the enzyme, one of the regulatory loops, termed LA, forms inhibitory contacts in the area of the active center. Reduction of the disulfide bond located in the middle of LA stimulates HtrA activity in vivo suggesting that this S-S bond may play a regulatory role, although the mechanism of this stimulation is not known. Here, we show that HtrA lacking an S-S bridge cleaved a model peptide substrate more efficiently and exhibited a higher affinity for a protein substrate. An LA loop lacking the disulfide was more exposed to the solvent; hence, at least some of the interactions involving this loop must have been disturbed. The protein without S-S bonds demonstrated lower thermal stability and was more easily converted to a dodecameric active oligomeric form. Thus, the lack of the disulfide within LA affected the stability and the overall structure of the HtrA molecule. In this study, we have also demonstrated that in vitro human thioredoxin 1 is able to reduce HtrA; thus, reduction of HtrA can be performed enzymatically.

Published

2015

4. The allergen Mus m 1.0102: Cysteine residues and molecular allergology

Author

Alberto Spisni, Fabio Tanfani, Samuele E. Burastero, Romina Corsini, and Elena Ferrari

Subjects

Models, Molecular, 0301 basic medicine, Protein Folding, Protein Conformation, Immunology, Immunologic Tests, Protein aggregation, Ligands, Protein Structure, Secondary, Cell Line, Serine, Mice, 03 medical and health sciences, 0302 clinical medicine, Protein structure, Spectroscopy, Fourier Transform Infrared, Animals, Humans, Cysteine, Structural motif, Molecular Biology, Major urinary proteins, Protein Stability, Chemistry, Oxidative folding, Proteins, Allergens, Recombinant Proteins, Spectrometry, Fluorescence, 030104 developmental biology, Amino Acid Substitution, Biochemistry, Mutagenesis, Site-Directed, Protein folding, 030215 immunology

Abstract

Mus m 1.0102 is a member of the mouse Major Urinary Protein family, belonging to the Lipocalins superfamily. Major Urinary Proteins (MUPs) are characterized by highly conserved structural motifs. These include a disulphide bond, involved in protein oxidative folding and protein structure stabilization, and a free cysteine residue, substituted by serine only in the pheromonal protein Darcin (MUP20). The free cysteine is recognized as responsible for the onset of inter- or intramolecular thiol/disulphide exchange, an event that favours protein aggregation. Here we show that the substitution of selected cysteine residues modulates Mus m 1.0102 protein folding, fold stability and unfolding reversibility, while maintaining its allergenic potency. Recombinant allergens used for immunotherapy or employed in allergy diagnostic kits require, as essential features, conformational stability, sample homogeneity and proper immunogenicity. In this perspective, recombinant Mus m 1.0102 might appear reasonably adequate as lead molecule because of its allergenic potential and thermal stability. However, its modest resistance to aggregation renders the protein unsuitable for pharmacological preparations. Point mutation is considered a winning strategy. We report that, among the tested mutants, C138A mutant acquires a structure more resistant to thermal stress and less prone to aggregation, two events that act positively on the protein shelf life. Those features make that MUP variant an attractive lead molecule for the development of a diagnostic kit and/or a vaccine.

Published

2020

5. Thermal stability, ligand binding and allergenicity data of Mus m 1.0102 allergen and its cysteine mutants

Author

Romina Corsini, Alberto Spisni, Samuele E. Burastero, Elena Ferrari, and Fabio Tanfani

Subjects

Mutant, Lipocalin allergen, Lipocalin, medicine.disease_cause, lcsh:Computer applications to medicine. Medical informatics, law.invention, 03 medical and health sciences, Aggregation, 0302 clinical medicine, Allergen, Antigen, law, Biochemistry, Genetics and Molecular Biology, medicine, Mus m 1 allergen, lcsh:Science (General), 030304 developmental biology, 0303 health sciences, Multidisciplinary, Chemistry, Thermal stability, Ligand (biochemistry), Dissociation constant, Biochemistry, Recombinant DNA, lcsh:R858-859.7, 030217 neurology & neurosurgery, Cysteine, lcsh:Q1-390

Abstract

The presented data were obtained with the lipocalin allergen Mus m 1.0102 and its cysteine mutants MM-C138A, MM-C157A and MM-C138,157A, whose structural features and unfold reversibility investigations are presented in the research article entitled “The allergen Mus m 1.0102: cysteine residues and molecular allergology” [1].The data were obtained by means of a Dynamic Light Scattering-based thermal stability assay, a Fluorescence-based ligand-binding assay and a basophil degranulation test, and describe proteins’ fold stability, ligand binding ability and allergenic potential, respectively. Analysis of the collected data produced the temperatures corresponding to the onset of the protein unfolding, the dissociation constants for N-Phenyl-1-naphthylamine ligand and the profiles of β-hexosaminidase release from RBL SX-38 cells, sensitized with the serum of selected allergic patients and incubated with increasing antigens concentrations.These data allow for comparison of the lipocalin allergen Mus m 1.0102 with its conserved cysteines mutants and, with regard to their potential application in allergy diagnostics and immunotherapy, they contribute to the process of recombinant allergen characterization and standardization. Keywords: Lipocalin allergen, Mus m 1 allergen, Thermal stability, Aggregation

Published

2020

6. Synthesis, Structural Insights and Activity of Different Classes of Biomolecules

Author

Mario Orena, Samuele Rinaldi, Elisabetta Giorgini, Francesca Biavasco, Giorgia Gioacchini, Francesco Spinozzi, Eleonora Giovanetti, Maria Grazia Ortore, Fabio Tanfani, Roberta Galeazzi, Andrea Scirè, Carla Vignaroli, Paolo Mariani, and Giovanna Mobbili

Subjects

chemistry.chemical_classification, Molecular dynamics, chemistry, Biomolecule, Drug delivery, Nanotechnology, Topology (chemistry), Characterization (materials science), Amino acid

Abstract

In this chapter, researches focusing on the synthesis, structural characterization and activity of different classes of biomolecules are reported. The covered topics range from the synthesis of new amino acids and foldamers to the structural and functional analysis of proteins, the preparation and characterization of nanosystems for drug delivery applications, the molecular bases of antibiotic resistance spread in Gram-positive bacteria and the study of topology and microstructure of tissues and cells. To this goal, different experimental and computational techniques are exploited, such as biomolecular assays, molecular dynamics, X-ray scattering and IR spectroscopy.

Published

2020

7. A Spectroscopic Study on Secondary Structure and Thermal Unfolding of the Plant Toxin Gelonin Confirms Some Typical Structural Characteristics and Unravels the Sequence of Thermal Unfolding Events

Author

Alessio Ausili, Fabio Tanfani, and Andrea Scirè

Subjects

endocrine system, Hot Temperature, endocrine system diseases, Endosome, Health, Toxicology and Mutagenesis, lcsh:Medicine, Toxicology, Spectrum Analysis, Raman, digestive system, Article, Protein Structure, Secondary, 03 medical and health sciences, 0302 clinical medicine, Immunotoxin, Spectroscopy, Fourier Transform Infrared, Protein biosynthesis, Gelonin, Protein secondary structure, Infrared spectroscopy, 030304 developmental biology, Protein Unfolding, Toxins, Biological, chemistry.chemical_classification, 0303 health sciences, Thermal unfolding, Ribosome-inactivating protein, Circular Dichroism, Immunotoxins, Suregada, lcsh:R, nutritional and metabolic diseases, food and beverages, Two-dimensional correlation spectroscopy, chemistry, 030220 oncology & carcinogenesis, Seeds, Biophysics, Ribosome Inactivating Proteins, Type 1, Glycoprotein, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

Gelonin from the Indian plant Gelonium multiflorum belongs to the type I ribosome-inactivating proteins (RIPs). Like other members of RIPs, this toxin glycoprotein inhibits protein synthesis of eukaryotic cells, hence, it is largely used in the construction of immunotoxins composed of cell-targeted antibodies. Lysosomal degradation is one of the main issues in targeted tumor therapies, especially for type I RIP-based toxins, as they lack the translocation domains. The result is an attenuated cytosolic delivery and a decrease of the antitumor efficacy of these plant-derived toxins, therefore, strategies to permit their release from endosomal vesicles or modifications of the toxins to make them resistant to degradation are necessary to improve their efficacy. Using infrared spectroscopy, we thoroughly analyzed both the secondary structure and the thermal unfolding of gelonin. Moreover, by the combination of two-dimensional correlation spectroscopy and phase diagram method, it was possible to deduce the sequence of events during the unfolding, confirming the typical characteristic of the RIP members to denature in two steps, as a sequential loss of tertiary and secondary structure was detected at 58 &deg, C and at 65 &deg, C, respectively. Additionally, some discrepancies in the unfolding process between gelonin and saporin-S6, another type I RIP protein, were detected.

Published

2019

8. Interaction of γ-conglutin from Lupinus albus with model phospholipid membranes: Investigations on structure, thermal stability and oligomerization status

Author

Maurizio Baldassarre, Marcello Duranti, Jessica Capraro, Andrea Scirè, Fabio Tanfani, and Alessio Scarafoni

Subjects

0301 basic medicine, Spectrophotometry, Infrared, Infrared, Lipid Bilayers, Biophysics, Phospholipid, Biochemistry, Analytical Chemistry, 03 medical and health sciences, Lupinus, chemistry.chemical_compound, Nephelometry and Turbidimetry, Transition Temperature, Thermal stability, Molecular Biology, Biological sciences, Plant Proteins, 030102 biochemistry & molecular biology, biology, Chemistry, food and beverages, Deuterium Exchange Measurement, Phosphatidylglycerols, Hydrogen-Ion Concentration, biology.organism_classification, Dihydroxyphenylalanine, 030104 developmental biology, Membrane, Chemical engineering, Seeds, Ft ir spectroscopy, hormones, hormone substitutes, and hormone antagonists

Abstract

Interaction with model phospholipid membranes of lupin seed gamma-conglutin, a glycaemia-lowering protein from Lupinus albus seeds, has been studied by means of Fourier-Transform infrared spectrosc ...

Published

2018

9. Bovine α1-acid glycoprotein, a thermostable version of its human counterpart: Insights from Fourier transform infrared spectroscopy and in silico modelling

Author

Roberta Galeazzi, Andrea Scirè, Fabio Tanfani, Beatrice Maggiore, and Maurizio Baldassarre

Subjects

chemistry.chemical_classification, Chemistry, Infrared spectroscopy, Biological activity, General Medicine, Glutamic acid, Biochemistry, Molten globule, chemistry.chemical_compound, TCEP, Denaturation (biochemistry), Glycoprotein, Thermostability

Abstract

a1-Acid glycoprotein (AGP) is a plasma protein and a member of the acute phase response. AGP is known to bind and carry several biologically active compounds, as well as to down-modulate the immune system activities. In this work, the structure of bovine AGP has been investigated by Fourier-Transform infrared spectroscopy. A model structure has been obtained on the basis of human AGP and refined by molecular dynamics. In spite of the similar structure, bovine AGP shows an unexpectedly higher (w20 � C) thermostability than its human counterpart. Inspection of the model structure has pointed out the presence of 12 ionic bridges and 2 sulphurearomatic interactions, whereas only 6 ionic bridges were detected in human AGP. The high number (9) of glutamic acid residues involved in the ionic interactions might explain the significantly decreased thermostability measured at pH 5.5 (Tm w 71 � C) with respect to pH 7.4 (Tm w 81 � C), whereas thermostability of human AGP was only slightly affected by lowering the pH. As in human AGP and several other lipocalins, a temperature-induced molten globule state has been observed in the denaturation pathway of bovine AGP. 2014 Published by Elsevier Masson SAS.

Published

2014

10. Fibrillation properties of human α1-acid glycoprotein

Author

Fabio Tanfani, Roberta Galeazzi, Maurizio Baldassarre, and Andrea Scirè

Subjects

Amyloid, Kinetics, General Medicine, Protein aggregation, Biochemistry, Congo red, chemistry.chemical_compound, Monomer, Protein structure, chemistry, Biophysics, TCEP, Thioflavin

Abstract

Human α(1)-acid glycoprotein (AGP) is a positive acute phase plasma protein containing two disulfide bridges. Structural studies have shown that under specific conditions AGP undergoes aggregation. In this study, we analysed the nature of AGP's aggregates formed under reducing and non-reducing conditions at pH 5.5 and at relatively low temperatures. Thioflavin T and Congo red spectroscopic analyses indicated the presence of cross-β structures in both unreduced and reduced AGP aggregates. In these samples amyloid-like fibrils were detected by transmission electron microscopy. The fibrils are branched and bent and present in very large amount in reduced AGP. Kinetics of AGP fibrillation proceeds without a lag phase and the rate constants of cross-β formation are linearly dependent on AGP concentration and result higher under reducing conditions. The data suggest a possible downhill mechanism of polymerization with a first-order monomer concentration dependence. Bioinformatics tools highlighted an extended region that sheathes one side of the molecule containing aggregation-prone regions. Reducing conditions make the extended region less constricted, allowing greater exposure of aggregation-prone regions, thus explaining the higher propensity of AGP to aggregate and fibrillate.

Published

2013

11. Characterization of Thymoquinone Binding to Human α1-Acid Glycoprotein

Author

Emidio Camaioni, Elisabetta Damiani, Hamal Khalifé, Fabio Tanfani, Giulio Lupidi, Andrea Scirè, and Luca Avenali

Subjects

biology, Molecular model, Chemistry, Stereochemistry, Hydrogen bond, thymoquinone, Molecular modeling, Pharmaceutical Science, Orosomucoid, drug interactions, Plasma protein binding, alpha 1-acid glycoprotein, Fluorescence spectroscopy, Hydrophobic effect, FTIR, chemistry.chemical_compound, biology.protein, Binding site, Thymoquinone

Abstract

Thymoquinone (TQ) is the main bioactive component isolated from Nigella sativa essential oil and seeds and has been used for the treatment of inflammations, liver disorders, arthritis, and is of great importance as a promising therapeutic drug for different diseases including cancer. This paper reports the first experimental evidence on binding of TQ to human α(1)-acid glycoprotein (AGP), an important drug-binding glycoprotein in human plasma, which affects pharmacokinetic properties of various therapeutic agents. The interaction of TQ with AGP has been characterized by Fourier transform infrared (FTIR) and fluorescence spectroscopy, as well as by molecular docking experiments. FTIR spectroscopy showed that the binding of TQ to AGP slightly increases its thermal stability and shifts the existence of a molten globule-like state observed in a previous study to higher temperature. The binding constants K(a); the number of binding sites n; and the corresponding thermodynamic parameters ΔG, ΔH, and ΔS at different temperatures were calculated through fluorescence spectroscopy. Fluorescence quenching experiments indicated that TQ binding involves hydrophobic interactions and to a lower extent hydrogen bonds, in agreement with molecular docking experiments. The data on binding ability of TQ to AGP represent basic information for the TQ pharmacokinetics such as drug metabolism and distribution in the body.

Published

2012

12. Turning pyridoxal-5′-phosphate-dependent enzymes into thermostable binding proteins: d-Serine dehydratase from baker’s yeast as a case study

Author

Maurizio Baldassarre, Fabio Tanfani, and Andrea Scirè

Subjects

Hot Temperature, Saccharomyces cerevisiae Proteins, Stereochemistry, medicine.medical_treatment, Molecular Sequence Data, Saccharomyces cerevisiae, Protein Engineering, Biochemistry, Catalysis, Protein Structure, Secondary, Cofactor, Serine, Serine dehydratase, Protein structure, Enzyme Stability, Spectroscopy, Fourier Transform Infrared, Escherichia coli, medicine, Amino Acid Sequence, Protein secondary structure, Hydro-Lyases, chemistry.chemical_classification, Protease, biology, Stereoisomerism, General Medicine, biology.organism_classification, Recombinant Proteins, Kinetics, Zinc, Enzyme, chemistry, Pyridoxal Phosphate, biology.protein, Holoenzymes

Abstract

d -serine dehydratase from Saccharomyces cerevisae is a recently discovered dimeric enzyme catalyzing the β-elimination of d -serine to pyruvate and ammonia. The reaction is highly enantioselective and depends on cofactor pyridoxal-5′-phosphate (PLP) and Zn2+. In our work, the aldimine linkage tethering PLP to recombinant, tagged d -serine dehydratase (Dsd) has been reduced by treatment with NaBH4 so as to yield an inactive form of the holoenzyme (DsdR), which was further treated with a protease in order to remove the amino-terminal purification tag. Fourier Transform infrared (FT-IR) spectroscopic analysis revealed that both the reduced form (DsdR) and the reduced/detagged form (DsdRD) maintain the overall secondary structure of Dsd, but featured a significant increased thermal stability. The observed Tm values for DsdR and for DsdRD shifted to 71.5 °C and 73.3 °C, respectively, resulting in nearly 11 °C and 13 °C higher than the one measured for Dsd. Furthermore, the analysis of the FT-IR spectra acquired in the presence of d -serine and l -serine indicates that, though catalytically inert, DsdRD retains the ability to enantioselectively bind its natural substrate. Sequence analysis of d -serine dehydratase and other PLP-dependent enzymes also highlighted critical residues involved in PLP binding. In virtue of its intrinsic properties, DsdRD represents an ideal candidate for the design of novel platforms based on stable, non-consuming binding proteins aimed at measuring d -serine levels in biological fluids.

Published

2012

13. Detection of temperature-induced molten globule states in small, β-sheet-rich proteins by infrared spectroscopy

Author

Fabio Tanfani, Maurizio Baldassarre, and Andrea Scirè

Subjects

Folding (chemistry), Circular dichroism, Crystallography, Chemistry, Beta sheet, Infrared spectroscopy, Radiology, Nuclear Medicine and imaging, Protein folding, Spectroscopy, Protein secondary structure, Molten globule

Abstract

The study of the mechanisms underlying formation of molten globule states in proteins is gaining growing interest due to recent discoveries concerning the involvement of this folding intermediate in several biological processes and to the possibility it offers to clarify the general process of protein folding. Different spectroscopic techniques, such as fluorescence, circular dichroism, nuclear magnetic resonance and infrared, have proved to be invaluable tools in the detection and charac- terization of molten globule states. In this review, the use of Fourier Transform infrared (FT-IR) spectroscopy to shed light on the formation of molten globules is discussed. Due to its ability to simultaneously probe the secondary structure and com- pactness/flexibility of protein samples prepared in deuterated media, FT-IR spectroscopy is particularly well suited to detect temperature-induced molten globule states in small, β-sheet-rich proteins. Several approaches for analysis and interpretation

Published

2012

14. Importance of pH and disulfide bridges on the structural and binding properties of human α1-acid glycoprotein

Author

Fabio Tanfani, Maurizio Baldassarre, Giulio Lupidi, and Andrea Scirè

Subjects

chemistry.chemical_classification, Chemistry, Ligand, Biological membrane, Context (language use), General Medicine, Protein aggregation, Biochemistry, chemistry.chemical_compound, Affinity chromatography, TCEP, Glycoprotein, Thermostability

Abstract

Human α 1 -acid glycoprotein (AGP) is an acute phase plasma glycoprotein containing two disulfide bridges. As a member of the lipocalin superfamily, it binds and transports several basic and neutral ligands, but a number of other activities have also been described. Thanks to its binding properties, AGP is also a good candidate for the development of biosensors and affinity chromatography media, and in this context detailed structural information is needed. The structural properties of AGP at different p 2 Hs and under reducing conditions were analysed by FT-IR spectroscopy. The obtained data indicate that AGP, when denatured, does not aggregate at neutral or basic p 2 Hs whilst it does at acidic p 2 Hs. Under reducing conditions the protein is remarkably less thermostable than its oxidized counterpart and presents an enhanced tendency to aggregate, even at neutral p 2 H. A heat-induced molten globule-like state (MG) was detected at 55 °C at p 2 H 7.4 and 5.5. At p 2 H 4.5 the MG occurred at 45 °C with an onset of formation at 40 °C. The MG was not observed under reducing conditions. A lower affinity of chlorpromazine and progesterone for the MG formed at p 2 H 4.5 and 40 °C was observed, suggesting that ligand(s) may be released near the negative surfaces of biological membranes. Furthermore, the reduced AGP displays an enhanced affinity for progesterone, indicating the importance of disulfide bonds for the binding capacity of AGP.

Published

2011

15. Insights into the structural properties of d-serine dehydratase from Saccharomyces cerevisiae: An FT-IR spectroscopic and in silico approach

Author

Andrea Scirè, Maurizio Baldassarre, Imma Fiume, and Fabio Tanfani

Subjects

Models, Molecular, Stereochemistry, Coenzymes, Saccharomyces cerevisiae, Biochemistry, Protein Structure, Secondary, Cofactor, Serine, Serine dehydratase, Protein structure, Catalytic Domain, Enzyme Stability, Spectroscopy, Fourier Transform Infrared, Homology modeling, Amino-acid racemase, Hydro-Lyases, chemistry.chemical_classification, Sequence Homology, Amino Acid, biology, Chemistry, Computational Biology, Reproducibility of Results, Active site, General Medicine, Hydrogen-Ion Concentration, Amino acid, Zinc, Pyridoxal Phosphate, biology.protein

Abstract

d -serine dehydratase (Dsd) from baker’s yeast is a recently discovered enzyme catalyzing the oxidation of d -serine to pyruvate and ammonia. The reaction depends on the cofactors pyridoxal-5′-phosphate (PLP) and Zn2+, featuring a very high selectivity towards the d -enantiomer of the amino acid serine. In humans, altered levels of d -serine in the cerebrospinal fluid (CSF) and blood correlate with the onset and evolution of a number of neurodegenerative diseases. Up to date very little is known on the structure of Dsd. Hence, we have investigated the structure of this enzyme by means of Fourier Transform infrared (FT-IR) spectroscopy and used the structural data derived thereof to validate a homology model of Dsd. In this model, Dsd adopts a fold that is characteristic of type III pyridoxal-dependent enzymes. This consists of an α/β (TIM) barrel and a β-sandwich domain at the N- and C-termini, respectively. Analysis of the Amide I and Amide III infrared bands revealed that the amounts of α (24%), β (29%) and unordered structures (47%) correlate well with those derived from the model (25%, 29% and 46% respectively), suggesting reliability of the latter. In addition, the model of Dsd was further refined by recreating the PLP- and zinc-restored active site based on a PLP- and zinc-dependent bacterial amino acid racemase recently crystallized, allowing us to identify the potential cofactor and metal binding residues of Dsd.

Published

2011

16. Temperature-induced conformational changes within the regulatory loops L1–L2–LA of the HtrA heat-shock protease from Escherichia coli

Author

Dorota Zurawa-Janicka, Agnieszka Polit, Andrea Scirè, Zaneta Szkarlat, Jerzy Ciarkowski, Barbara Lipinska, Anna Sobiecka-Szkatula, Fabio Tanfani, Joanna Skorko-Glonek, and Artur Giełdoń

Subjects

Protein Denaturation, Circular dichroism, Protein Conformation, medicine.medical_treatment, Biophysics, Biochemistry, Analytical Chemistry, Serine, acrylamide quenching, Protein structure, Heat shock protein, Spectroscopy, Fourier Transform Infrared, Escherichia coli, medicine, protein structure, Heat shock, Molecular Biology, HtrA protein, Heat-Shock Proteins, Serine protease, Protease, biology, Chemistry, Circular Dichroism, Serine Endopeptidases, Active site, fluorescence spectroscopy, Crystallography, Trp mutant, structural change, biology.protein, Periplasmic Proteins, Heat-Shock Response

Abstract

The present investigation was undertaken to characterize mechanism of thermal activation of serine protease HtrA (DegP) from Escherichia coli. We monitored the temperature-induced structural changes within the regulatory loops L1, L2 and LA using a set of single-Trp HtrA mutants. The accessibility of each Trp residue to aqueous medium at temperature range 25-45 degrees C was assessed by steady-state fluorescence quenching using acrylamide and these results in combination with mean fluorescence lifetimes (tau) and wavelength emission maxima (lambda(em)max) were correlated with the induction of the HtrA proteolytic activity. Generally the temperature shift caused better exposure of Trps to the quencher; although, each of the loops was affected differently. The LA loop seemed to be the most prone to temperature-induced conformational changes and a significant opening of its structure was observed even at the lowest temperatures tested (25-30 degrees C). To the contrary, the L1 loop, containing the active site serine, remained relatively unchanged up to 40 degrees C. The L2 loop was the most exposed element and showed the most pronounced changes at temperatures exceeding 35 degrees C. Summing up, the HtrA structure appears to open gradually, parallel to the gradual increase of its proteolytic activity.

Published

2009

17. Structure and Stability of a Rat Odorant-Binding Protein: Another Brick in the Wall

Author

Sabato D'Auria, Fabio Tanfani, Anna Marabotti, Maria Staiano, Loic Briand, Andrea Scirè, Antonio Varriale, Enrico Bertoli, Università Politecnica delle Marche [Ancona] (UNIVPM), FLAveur, VIsion et Comportement du consommateur (FLAVIC), Etablissement National d'Enseignement Supérieur Agronomique de Dijon (ENESAD)-Institut National de la Recherche Agronomique (INRA)-Université de Bourgogne (UB), Laboratory for Molecular Sensing, and IBP-CNR

Subjects

Models, Molecular, Protein Folding, 030303 biophysics, Infrared spectroscopy, ODORANT-BINDING PROTEIN, FOURIER TRANSFORM INFRARED SPECTROSCOPIE, LIPOCALIN, RAT, Receptors, Odorant, Biochemistry, Protein Structure, Secondary, 03 medical and health sciences, chemistry.chemical_compound, Molecular dynamics, Amide, Spectroscopy, Fourier Transform Infrared, Animals, Intermediate state, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, Computer Simulation, Denaturation (biochemistry), Least-Squares Analysis, Fourier transform infrared spectroscopy, 030304 developmental biology, Phase diagram, 0303 health sciences, Protein Stability, Chemistry, Temperature, General Chemistry, Recombinant Proteins, Rats, Crystallography, protéine, spectrométrie, Two-dimensional nuclear magnetic resonance spectroscopy, olfaction

Abstract

Andrea Scire, Anna Marabotti, Maria Staiano: These authors contributed equally to the work.; International audience; The effect of temperature on the structure of the rat odorant-binding protein was investigated by spectroscopic and in silico methodologies. In particular, in this work, we examined the structural features of the rat OBP-1F by Fourier-transform infrared spectroscopy and molecular dynamics investigations. The obtained spectroscopic results were analyzed using the following three different methods based on the unexchanged amide hydrogens of the protein sample: (1) the analysis of difference spectra; (2) the generalized 2D-IR correlation spectroscopy; (3) the phase diagram method. The three methods indicated that at high temperatures the rOBP-1F structure undergoes a relaxation process involving the protein tertiary organization before undergoing the denaturation and aggregation processes, suggesting the presence of an intermediate state such as a molten globule-like state. Importantly, the proposed analyses represent a general approach that could be applied to the study of protein stability.

Published

2009

18. A comparative infrared spectroscopic study of glycoside hydrolases from extremophilic archaea revealed different molecular mechanisms of adaptation to high temperatures

Author

Rossana D'Avino, Andrea Scirè, Fabio Tanfani, Enrico Bertoli, Giuseppe Perugino, Barbara Di Lauro, Alessio Ausili, Beatrice Cobucci-Ponzano, Marco Moracci, Mosè Rossi, Ausili, A, COBUCCI PONZANO, B, DI LAURO, B, Davino, R, Perugino, G, Bertoli, E, Scire, A, Rossi, Mose', Tanfani, F, Moracci, M., Ausili, Alessio, Cobucci Ponzano, Beatrice, DI LAURO, Barbara, D'Avino, Rossana, Perugino, Giuseppe, Bertoli, Enrico, Scirè, Andrea, Tanfani, Fabio, and Moracci, Marco

Subjects

Models, Molecular, Protein Denaturation, animal structures, Glycoside Hydrolases, Spectrophotometry, Infrared, ved/biology.organism_classification_rank.species, Glycoside Hydrolase, Adaptation, Biological, Biology, Biochemistry, Protein Structure, Secondary, Protein structure, Structural Biology, Glycoside hydrolase, protein structure, infrared spectroscopy, Molecular Biology, Protein secondary structure, beta-glycosidase, integumentary system, Desulfurococcaceae, ved/biology, Thermophile, Sulfolobus solfataricus, Temperature, Computational Biology, Sulfolobus solfataricu, biology.organism_classification, Hyperthermophile, Protein Structure, Tertiary, Pyrococcus furiosus, embryonic structures, Protein stabilization, Pyrococcus furiosu

Abstract

The identification of the determinants of protein thermal stabilization is often pursued by comparing enzymes from hyperthermophiles with their mesophilic counterparts while direct structural comparisons among proteins and enzymes from hyperthermophiles are rather uncommon. Here, oligomeric beta-glycosidases from the hyperthermophilic archaea Sulfolobus solfataricus (Ss beta-gly), Thermosphaera aggregans (Ta beta-gly), and Pyrococcus furiosus (Pf beta-gly), have been compared. Studies of FTIR spectroscopy and kinetics of thermal inactivation showed that the three enzymes had similar secondary structure composition, but Ss beta-gly and Ta beta-gly (temperatures of melting 98.1 and 98.4 degrees C, respectively) were less stable than Pf beta-gly, which maintained its secondary structure even at 99.5 degrees C. The thermal denaturation of Pf beta-gly, followed in the presence of SDS, suggested that this enzyme is stabilized by hydrophobic interactions. A detailed inspection of the 3D-structures of these enzymes supported the experimental results: Ss beta-gly and Ta beta-gly are stabilized by a combination of ion-pairs networks and intrasubunit S-S bridges while the increased stability of Pf beta-gly resides in a more compact protein core. The different strategies of protein stabilization give experimental support to recent theories on thermophilic adaptation and suggest that different stabilization strategies could have been adopted among archaea.

Published

2007

19. The thermal unfolding of the ribosome-inactivating protein saporin-S6 characterized by infrared spectroscopy

Author

Andrea Scirè, Marina Gacto Sánchez, Alessio Ausili, and Fabio Tanfani

Subjects

Models, Molecular, Protein Denaturation, Hot Temperature, Saporin, Biophysics, Biochemistry, Protein Structure, Secondary, Analytical Chemistry, Saponaria, Spectroscopy, Fourier Transform Infrared, Saponaria officinalis, Denaturation (biochemistry), Molecular Biology, Protein secondary structure, Infrared spectroscopy, Thermostability, Protein Unfolding, Thermal unfolding, biology, Chemistry, Protein Stability, Ribosome-inactivating protein, Hydrogen-Ion Concentration, biology.organism_classification, Saporins, Protein Structure, Tertiary, Solutions, Seeds, biology.protein, Ribosome Inactivating Proteins, Type 1, Protein A, Saporin-S6, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

Saporin-S6 is a plant toxin belonging to the type 1 ribosome-inactivating protein (RIP) family. Since it was extracted and isolated from Saponaria officinalis for the first time almost thirty years ago, the protein has been widely studied mainly for its potential applications in anti-tumour and anti-viral infection therapy. Like other RIPs, saporin-S6 is particularly effective in the form of immunotoxin conjugated with monoclonal antibodies and its chemico-physical characteristics made the protein a perfect candidate for the synthesis, development and use of saporin-S6-based chimeric toxins. The high stability of the protein against different denaturing agents has been broadly demonstrated, however, its complete thermal unfolding characterization has not already been performed. In this work we analyse in detail structure, thermostability and unfolding features by means of infrared spectroscopy coupled with two-dimensional correlation spectroscopy. Our data showed that saporin-S6 in solution at neutral pH exhibits a secondary structure analogue to that of the crystal and confirmed its good stability at moderately high temperatures, with a temperature of melting of 58 �C. Our results also demonstrated that the thermal unfolding process is non-cooperative and occurs in two steps, and revealed the sequence of the events that take place during the denaturation, showing a higher stability of the N-terminal domain of the protein. © 2015 Elsevier B.V.

Published

2015

20. Analysis of the link between the redox state and enzymatic activity of the HtrA (DegP) protein from Escherichia coli

Author

Anna Sobiecka-Szkatula, Barbara Lipinska, Agnieszka Polit, Bogdan Banecki, Urszula Zarzecka, Donata Figaj, Leszek Kadziński, Joanna Skorko-Glonek, Dorota Zurawa-Janicka, Tomasz Koper, Andrea Scirè, Fabio Tanfani, Adam Lesner, and Katarzyna Wegrzyn

Subjects

Proteases, Proteolysis, Recombinant Fusion Proteins, Science, Molecular Sequence Data, medicine.disease_cause, complex mixtures, Substrate Specificity, Protein structure, Heat shock protein, medicine, Escherichia coli, Histidine, Amino Acid Sequence, Disulfides, Peptide sequence, Heat-Shock Proteins, chemistry.chemical_classification, Multidisciplinary, medicine.diagnostic_test, Chemistry, Circular Dichroism, Mutagenesis, Serine Endopeptidases, Temperature, Surface Plasmon Resonance, bacterial infections and mycoses, Kinetics, Enzyme, Biochemistry, bacteria, Medicine, Periplasmic Proteins, Oligopeptides, Oxidation-Reduction, Sequence Alignment, Research Article

Abstract

Bacterial HtrAs are proteases engaged in extracytoplasmic activities during stressful conditions and pathogenesis. A model prokaryotic HtrA (HtrA/DegP from Escherichia coli) requires activation to cleave its substrates efficiently. In the inactive state of the enzyme, one of the regulatory loops, termed LA, forms inhibitory contacts in the area of the active center. Reduction of the disulfide bond located in the middle of LA stimulates HtrA activity in vivo suggesting that this S-S bond may play a regulatory role, although the mechanism of this stimulation is not known. Here, we show that HtrA lacking an S-S bridge cleaved a model peptide substrate more efficiently and exhibited a higher affinity for a protein substrate. An LA loop lacking the disulfide was more exposed to the solvent; hence, at least some of the interactions involving this loop must have been disturbed. The protein without S-S bonds demonstrated lower thermal stability and was more easily converted to a dodecameric active oligomeric form. Thus, the lack of the disulfide within LA affected the stability and the overall structure of the HtrA molecule. In this study, we have also demonstrated that in vitro human thioredoxin 1 is able to reduce HtrA; thus, reduction of HtrA can be performed enzymatically.

Published

2015

21. Temperature-, SDS-, and pH-Induced Conformational Changes in Protein Disulfide Oxidoreductase from the Archaeon Pyrococcus furiosus: A Dynamic Simulation and Fourier Transform Infrared Spectroscopic Study

Author

Simonetta Bartolucci, Emilia Pedone, Mosè Rossi, Alessio Ausili, Fabio Tanfani, Michele Saviano, Enrico Bertoli, and Andrea Scirè

Subjects

Models, Molecular, Protein Denaturation, Protein Folding, Hot Temperature, Protein Conformation, Archaeal Proteins, Molecular Sequence Data, Molecular Conformation, Molecular Dynamics, Biochemistry, Protein Structure, Secondary, Molecular dynamics, Protein structure, Oxidoreductase, Spectrophotometry, Spectroscopy, Fourier Transform Infrared, medicine, Computer Simulation, NADH, NADPH Oxidoreductases, Amino Acid Sequence, Disulfides, Binding site, oxidoreductase, Thermostability, Adenosine Triphosphatases, chemistry.chemical_classification, Binding Sites, biology, medicine.diagnostic_test, Temperature, Proteins, Sodium Dodecyl Sulfate, General Chemistry, Hydrogen-Ion Concentration, biology.organism_classification, Pyrococcus furiosus, FT-IR, Crystallography, chemistry, Protein folding

Abstract

The effect of SDS, pD, and temperature on the structure and stability of the protein disulfide oxidoreductase from Pyrococcus furiosus (PfPDO) was investigated by molecular dynamic (MD) simulations and FT-IR spectroscopy. pD affects the thermostability of alpha-helices and beta-sheets differently, and 0.5% or higher SDS concentration influences the structure significantly. The experiments allowed us to detect a secondary structural reorganization at a definite temperature and pD which may correlate with a high ATPase activity of the protein. The MD simulations supported the infrared data and revealed the different behavior of the N and C terminal segments, as well as of the two active sites.

Published

2005

22. Binding of glutamine to glutamine-binding protein from Escherichia coli induces changes in protein structure and increases protein stability

Author

Antonio Varriale, Fabio Tanfani, Viviana Scognamiglio, Sabato D'Auria, Alessio Ausili, Mosè Rossi, Andrea Scirè, Maria Staiano, and Anna Marabotti

Subjects

chemistry.chemical_classification, biology, Escherichia coli Proteins, Glutamine, Peptide, Periplasmic space, Glutamine binding, Biochemistry, Protein Structure, Secondary, Protein tertiary structure, Protein structure, chemistry, Structural Biology, Escherichia coli, biology.protein, Thermodynamics, Protein G, Carrier Proteins, Molecular Biology, Protein secondary structure, Protein Binding

Abstract

Glutamine-binding protein (Gl- nBP) from Escherichia coli is a monomeric protein localized in the periplasmic space of the bacterium. It is responsible for the first step in the active transport of L-glutamine across the cytoplasmic membrane. The protein consists of two similar globu- lar domains linked by two peptide hinges, and X-ray crystallographic data indicate that the two domains undergo large movements upon ligand binding. Fou- rier transform infrared spectroscopy (FTIR) was used to analyze the structure and thermal stability of the protein in detail. The data indicate that glutamine binding induces small changes in the secondary structure of the protein and that it ren- ders the structure more thermostable and less flex- ible. Detailed analyses of IR spectra show a lower thermal sensitivity of -helices than -sheets in the protein both in the absence and in the presence of glutamine. Generalized two-dimensional (2D) analy- ses of IR spectra reveal the same sequence of unfold- ing events in the protein in the absence and in the presence of glutamine, indicating that the amino acid does not affect the unfolding pathway of the protein. The data give new insight into the struc- tural characteristics of GlnBP that are useful for both basic knowledge and biotechnological applica- tions. Proteins 2005;58:80 - 87. © 2004 Wiley-Liss, Inc.

Published

2004

23. Thermal Stability and Aggregation of Sulfolobus solfataricus β-Glycosidase Are Dependent upon the N-∈-Methylation of Specific Lysyl Residues

Author

Enrico Bertoli, S. Formisano, Roberto Nucci, Piero Pucci, Fabrizio Gentile, Annapaola Andolfo, Fabio Tanfani, Andrea Scirè, Carlo Vaccaro, Raffaella Briante, and Ferdinando Febbraio

Subjects

chemistry.chemical_classification, biology, ved/biology, Sulfolobus solfataricus, ved/biology.organism_classification_rank.species, Cell Biology, Methylation, medicine.disease_cause, biology.organism_classification, Biochemistry, law.invention, Enzyme, chemistry, law, medicine, Recombinant DNA, Glycoside hydrolase, Molecular Biology, Escherichia coli, Protein secondary structure, Bacteria

Abstract

Methylation in vivo is a post-translational modification observed in several organisms belonging to eucarya, bacteria, and archaea. Although important implications of this modification have been demonstrated in several eucaryotes, its biological role in hyperthermophilic archaea is far from being understood. The aim of this work is to clarify some effects of methylation on the properties of β-glycosidase from Sulfolobus solfataricus, by a structural comparison between the native, methylated protein and its unmethylated counterpart, recombinantly expressed in Escherichia coli. Analysis by Fourier transform infrared spectroscopy indicated similar secondary structure contents for the two forms of the protein. However, the study of temperature perturbation by Fourier transform infrared spectroscopy and turbidimetry evidenced denaturation and aggregation events more pronounced in recombinant than in native β-glycosidase. Red Nile fluorescence analysis revealed significant differences of surface hydrophobicity between the two forms of the protein. Unlike the native enzyme, which dissociated into SDS-resistant dimers upon exposure to the detergent, the recombinant enzyme partially dissociated into monomers. By electrospray mapping, the methylation sites of the native protein were identified. A computational analysis of β-glycosidase three-dimensional structure and comparisons with other proteins from S. solfataricus revealed analogies in the localization of methylation sites in terms of secondary structural elements and overall topology. These observations suggest a role for the methylation of lysyl residues, located in selected domains, in the thermal stabilization of β-glycosidase from S. solfataricus.

Published

2004

24. Effects induced by mono- and divalent cations on protein regions responsible for thermal adaptation in �-glycosidase from Sulfolobus solfataricus

Author

Fabrizio Gentile, Enrico Bertoli, Pietro Amodeo, Andrea Scirè, Roberto Nucci, Ferdinando Febbraio, Fabio Tanfani, Ettore Bismuto, and Raffaella Briante

Subjects

Models, Molecular, Hofmeister series, Cations, Divalent, Beta-glycosidase, Static Electricity, ved/biology.organism_classification_rank.species, Biophysics, Ionic bonding, Crystallography, X-Ray, Biophysical Phenomena, Protein Structure, Secondary, Sulfolobus, Divalent, Enzyme Stability, Spectroscopy, Fourier Transform Infrared, Cation effects, Protein Structure, Quaternary, Protein secondary structure, Thermostability, chemistry.chemical_classification, ved/biology, Chemistry, Circular Dichroism, Sulfolobus solfataricus, General Medicine, Cations, Monovalent, Enzyme structure, Crystallography, Thermodynamics, Protein quaternary structure, Glucosidases

Abstract

The perturbation induced by mono- and divalent cations on the thermophilicity and thermostability of Solfolobus solfataricus beta-glycosidase, a hyperthermophilic tetrameric enzyme, has been investigated by spectroscopic and computational simulation methods to ascertain the Hofmeister effects on two strategic protein regions identified previously. Specifically, (1). an extra segment (83-124), present only in the sequence of hyperthermophilic glycosidases and recognized as an important thermostability determinant for the enzyme structure; and (2). a restricted area of the subunit interface responsible for the quaternary structure maintenance. Mono- and divalent cations inhibit to a different extent the beta-glycosidase activity, whose kinetic constants show an apparent competitive inhibition of the catalytic process that reflects the Hofmeister order. The thermostability is also affected by the nature and charge of the cations, reaching maximal effects for the case of Mg(2+). Fourier transform infrared spectroscopy has revealed very small changes in the protein secondary structure in the presence of the investigated cations at 20 degrees C, while large effects on the protein melting temperatures are observed. Computational analysis of the enzyme structure has identified negative patches on the accessible surface of the two identified regions. Following the Hofmeister series, cations weaken the existing electrostatic network that links the extra segment to the remaining protein matrix. In particular, the perturbing action of cations could involve the ionic pair interactions E107-R245 and E109-R185, thus leading to a local destructuring of the extra segment as a possible starting event for thermal destabilization. A detailed investigation of the electrostatic network at the A-C intermolecular interface of Sbetagly after energy minimization suggests that cations could cause a strong attenuation of the ion pair interactions E474-K72 and D473-R402, with consequent partial dissociation of the tetrameric structure.

Published

2004

25. Mutagenesis of the Dimer Interface Region of Corynebacterium callunae Starch Phosphorylase Perturbs the Phosphate-Dependent Conformational Relay that Enhances Oligomeric Stability of the Enzyme

Author

Richard Griessler, Barbara Psik, Bernd Nidetzky, Francesco-Maria Pierfederici, Andrea Scirè, and Fabio Tanfani

Subjects

Protein Denaturation, Conformational change, Spectrophotometry, Infrared, Protein Conformation, Stereochemistry, Dimer, Molecular Sequence Data, Mutant, Corynebacterium, Biochemistry, Phosphates, chemistry.chemical_compound, Protein structure, Spectroscopy, Fourier Transform Infrared, Denaturation (biochemistry), Amino Acid Sequence, Protein Structure, Quaternary, Molecular Biology, Alanine, Starch phosphorylase, Temperature, Wild type, Starch Phosphorylase, Hydrogen Peroxide, General Medicine, Kinetics, Crystallography, chemistry, Mutation, Mutagenesis, Site-Directed, Protein quaternary structure, Dimerization, Plasmids

Abstract

We have used alanine-scanning site-directed mutagenesis of the dimer contact region of starch phosphorylase from Corynebacterium callunae to explore the relationship between a protein conformational change induced by phosphate binding and the up to 500-fold kinetic stabilization of the functional quarternary structure of this enzyme when phosphate is present. Purified mutants (at positions Ser-224, Arg-226, Arg-234, and Arg-242) were characterized by Fourier transform-infrared (FT-IR) spectroscopy and enzyme activity measurements at room temperature and under conditions of thermal denaturation. Difference FT-IR spectra of wild type and mutants in (2)H(2)O solvent revealed small changes in residual amide II band intensities at approximately 1,550 cm(-1), indicating that (1)H/(2)H exchange in the wild type is clearly perturbed by the mutations. Decreased (1)H/(2)H exchange in comparison to wild type suggests formation of a more compact protein structure in S224A, R234A, and R242A mutants and correlates with rates of irreversible thermal denaturation at 45 degrees C that are up to 10-fold smaller for the three mutants than the wild type. By contrast, the mutant R226A inactivates 2.5-fold faster at 45 degrees C and shows a higher (1)H/(2)H exchange than the wild type. Phosphate (20 mM) causes a greater change in FT-IR spectra of the wild type than in those of S224A and 234A mutants and leads to a 5-fold higher stabilization of the wild type than the two mutants. Therefore, structural effects of phosphate binding leading to kinetic stability of wild-type starch phosphorylase are partially complemented in the S224A and R234A mutants. Infrared spectroscopic measurements were used to compare thermal denaturations of the mutants and the wild type in the absence and presence of stabilizing oxyanion. The broad denaturation transition of unliganded wild type in the range 40-50 degrees C is reduced in the S224A and R234A mutants, and this reflects mainly a shift of the onset of denaturation to a 4-5 degrees C higher value.

Published

2003

26. Structural and thermal stability analysis of Escherichia coli and Alicyclobacillus acidocaldarius thioredoxin revealed a molten globule-like state in thermal denaturation pathway of the proteins: an infrared spectroscopic study

Author

Andrea Scirè, Tiziana Cacciamani, Fabio Tanfani, Francesco Maria Pierfederici, Mosè Rossi, Emilia Pedone, Simonetta Bartolucci, Pedone, E, Bartolucci, Simonetta, Rossi, Mose', Pierfederici, F, Scire, A, Cacciamani, T, Tanfani, F., F., Pierfederici, A., Scire, Cacciamani, and F., Tanfani

Subjects

molten globule-like states, Protein Denaturation, animal structures, Spectrophotometry, Infrared, Protein Conformation, Infrared, Mutant, Infrared spectroscopy, Alicyclobacillus acidocaldariu, Protein aggregation, medicine.disease_cause, Biochemistry, Thioredoxins, Fourier-transform IR spectroscopy, Enzyme Stability, Escherichia coli, medicine, Thermal stability, Molecular Biology, Chemistry, thioredoxin, Cell Biology, Molten globule, Crystallography, Thioredoxin, Research Article

Abstract

The structure of thioredoxin from Alicyclobacillus acidocaldarius (previously named Bacillus acidocaldarius) (BacTrx) and from Escherichia coli (E. coli Trx) was studied by Fourier-transform IR spectroscopy. Two mutants of BacTrx [Lys18→Gly (K18G) and Arg82→Glu (R82E)] were also analysed. The data revealed similar secondary structures in all proteins, but BacTrx and its mutants showed a more compact structure than E. coli Trx. In BacTrx and its mutants, the compactness was p2H-dependent. All proteins revealed the existence of a molten globule-like state. At p2H 5.8, the temperature at which this state was detected was higher in BacTrx and decreased in the different proteins in the following order: BacTrx>R82E>K18G>E. coli Trx. At neutral or basic p2H, the molten globule-like state was detected at the same temperature in both BacTrx and R82E, whereas it was found at the same temperature in all p2Hs tested for E. coli Trx. The thermal stability of the proteins was in the following order at all p2Hs tested: BacTrx>R82E>K18G>E. coli Trx, and was lower for each protein at p2H 8.4 than at neutral or acidic p2Hs. The formation of protein aggregates, brought about by thermal denaturation, were observed for BacTrx and K18G at all p2Hs tested, whereas they were present in R82E and E. coli Trx samples only at p2H 5.8. The results indicated that a single mutation might affect the structural properties of a protein, including its propensity to aggregate at high temperatures. The data also indicated a possible application of Fourier-transform IR spectroscopy for assessing molten globule-like states in small proteins.

Published

2003

27. Effect of acidic phospholipids on the structural properties of recombinant cytosolic human glyoxalase II

Author

Enrico Bertoli, Fabio Tanfani, Sabato D'Auria, Giovanni Principato, Maria Teresa Cambria, Andrea Scirè, and Franca Saccucci

Subjects

chemistry.chemical_classification, Liposome, virus diseases, Biochemistry, Protein tertiary structure, Hydrophobic effect, chemistry.chemical_compound, Enzyme, Non-competitive inhibition, chemistry, Structural Biology, Phosphatidylcholine, Molecular Biology, Protein secondary structure, Glyoxalase system

Abstract

A peculiar characteristic of highly concentrated cytosolic recombinant human glyoxalase II (GII) solutions is to undergo partial precipitation. Previous work indicated that anionic phospholipids (PLs) exert a noncompetitive inhibition on the enzymatic activity of the soluble enzyme. In this study, FTIR spectroscopy was used to analyze the structural properties and the thermal stability of the soluble protein in the absence and in the presence of liposomes made of different phospholipids (PLs). The structural analysis was performed on the precipitate as well. The interaction of acidic PLs with GII lowered the thermal stability of the enzyme and inhibited protein intermolecular interactions (aggregation) brought about by thermal denaturation. Infrared data indicated that ionic and hydrophobic interactions occur between GII and acidic PLs causing small changes in the secondary structure of the enzyme. No interactions of the protein with egg phosphatidylcholine liposomes were detected. The results are consistent with the destabilization of the protein tertiary structure, and indicate that GII possesses hydrophobic part(s) that interact with the acyl chains of PLs. Data on precipitated GII did not show remarkable modification of secondary structure, suggesting that hydrophobic stretches of the enzyme may also be involved in the protein-protein association (precipitation) at high GII concentration. The alterations in the GII structure and the noncompetitive inhibition exerted by acidic PLs are strictly related.

Published

2002

28. Two-dimensional gel electrophoresis and FTIR spectroscopy reveal both forms of yeast plasma membrane H+-ATPase in activated and basal-level enzyme preparations

Author

Arnošt Kotyk, Georgios Lapathitis, Enrico Bertoli, and Fabio Tanfani

Subjects

Saccharomyces cerevisiae, Biophysics, Biochemistry, Protein Structure, Secondary, Structural Biology, Secondary structure, Yeasts, Two-dimensional gel electrophoresis, Spectroscopy, Fourier Transform Infrared, Genetics, Electrophoresis, Gel, Two-Dimensional, Phosphorylation, Fourier transform infrared spectroscopy, Molecular Biology, Protein secondary structure, chemistry.chemical_classification, biology, Cell Membrane, Cell Biology, biology.organism_classification, Yeast, Enzyme Activation, Proton-Translocating ATPases, Electrophoresis, Membrane, Enzyme, chemistry, H+-ATPase, Plasma membrane

Abstract

Plasma membrane H+-ATPase of the yeast Saccharomyces cerevisiae was isolated and purified in its two forms, the activated A-ATPase from glucose-metabolizing cells, and the basal-level B-ATPase from cells with endogenous metabolism only. Using two-dimensional gel electrophoretic analysis, we showed that both enzyme preparations are actually mixtures of the non-active, i.e. non-phosphorylated, and the active, i.e. phosphorylated, forms of the enzyme. Previous deliberations suggesting that the B-ATPase displays some activity which is lower than that of A-ATPase were apparently wrong. It seems that, molecularly speaking, the B-form is actually not active at all, and what activity we measure in our preparation is due to an admixture of the true active form (A-form). Fourier transform infrared spectroscopic study of the secondary structure and particularly thermal denaturation data suggest the possibility that the two enzyme forms interact to form complexes less stable than the single forms. On the whole then, there apparently is a different ratio of the active and inactive forms and/or complexes between the two forms present in all enzyme preparations.

Published

2001

29. Oxyanion-Mediated Protein Stabilization: Differential Roles of Phosphate for Preventing Inactivation of Bacterial α-Glucan Phosphorylases

Author

Bernd Nidetzky, Marlene Pickl, Fabio Tanfani, Richard Grieβler, and Sabato D'Auria

Subjects

chemistry.chemical_classification, Starch phosphorylase, Oxyanion, Phosphate, Biochemistry, Catalysis, chemistry.chemical_compound, Glycogen phosphorylase, Enzyme, chemistry, Urea, Protein stabilization, Pyridoxal, Biotechnology

Abstract

Maltodextrin phosphorylase (MalP) from Escherichia coli and starch phosphorylase (StP) from Corynebacterium callunae are significantly stabilized in the presence of phosphate against inactivation by elevated temperature or urea. The stabilizing effect of phosphate was observed at ion concentrations below 50 mM. Therefore, it is probably due to preferential binding of phosphate to the folded conformations of the phosphorylases. For StP, phosphate binding inhibited the dissociation of the active-site cofactor pyridoxal 5′-phosphate. Phosphate-liganded StP was at least 500-fold more stable at 60d`C than the free enzyme at the same temperature. It showed an apparent transition midpoint of 5.2 M for irreversible denaturation by urea, and this midpoint was increased by a denaturant concentration of 4M relative to the corresponding transition midpoint of free StP in urea. The mechanisms of inactivation and denaturation of MalP at 45d`C and by urea involve formation of a cofactor-containing, insoluble protein agg...

Published

2001

30. The thermophilic esterase fromArchaeoglobus fulgidus: Structure and conformational dynamics at high temperature

Author

Joseph R. Lakowicz, Petr Herman, Sabato D'Auria, Fabio Tanfani, Giuseppe Manco, Enrico Bertoli, and Mosè Rossi

Subjects

chemistry.chemical_classification, Protein Denaturation, Hot Temperature, Quenching (fluorescence), biology, Chemistry, Esterases, Archaeoglobus fulgidus, Deuterium, Biochemistry, Esterase, Fluorescence, Article, Protein Structure, Secondary, Fluorescence spectroscopy, Enzyme assay, Crystallography, Spectrometry, Fluorescence, Enzyme, Structural Biology, Spectroscopy, Fourier Transform Infrared, biology.protein, Molecular Biology, Protein secondary structure

Abstract

The esterase from the hyperthermophilic archaeon Archaeoglobus fulgidus is a monomeric protein with a molecular weight of about 35.5 kDa. The enzyme is barely active at room temperature, displaying the maximal enzyme activity at about 80 degrees C. We have investigated the effect of the temperature on the protein structure by Fourier-transform infrared spectroscopy. The data show that between 20 degrees C and 60 degrees C a small but significant decrease of the beta-sheet bands occurred, indicating a partial loss of beta-sheets. This finding may be surprising for a thermophilic protein and suggests the presence of a temperature-sensitive beta-sheet. The increase in temperature from 60 degrees C to 98 degrees C induced a decrease of alpha-helix and beta-sheet bands which, however, are still easily detected at 98 degrees C indicating that at this temperature some secondary structure elements of the protein remain intact. The conformational dynamics of the esterase were investigated by frequency-domain fluorometry and anisotropy decays. The fluorescence studies showed that the intrinsic tryptophanyl fluorescence of the protein was well represented by the three-exponential model, and that the temperature affected the protein conformational dynamics. Remarkably, the tryptophanyl fluorescence emission reveals that the indolic residues remained shielded from the solvent up to 80 degrees C, as shown from the emission spectra and by acrylamide quenching experiments. The relationship between enzyme activity and protein structure is discussed.

Published

2000

31. Effects of fluorescent pseudo-ATP and ATP-metal analogs on secondary structure of Na+/K+-ATPase

Author

Wilhelm Schoner, Otakar Jelinek, Evzen Amler, Tomas Obsil, Rita Krumscheid, Holger Linnertz, Laura Mazzanti, Enrico Bertoli, Fabio Tanfani, and Petra Urbanova

Subjects

ATP analog, Stereochemistry, Backdoor phosphorylation, Biophysics, Biochemistry, Protein Structure, Secondary, Metal, chemistry.chemical_compound, Adenosine Triphosphate, Isothiocyanates, Spectroscopy, Fourier Transform Infrared, Organometallic Compounds, Na+/K+-ATPase, Fluorescein, Phosphorylation, Protein secondary structure, chemistry.chemical_classification, Tryptophan, Cell Biology, Fluorescence, Transmembrane protein, FT-IR, Enzyme, chemistry, Erythrosine, Ouabain-binding, visual_art, visual_art.visual_art_medium, Sodium-Potassium-Exchanging ATPase, Fluorescein-5-isothiocyanate

Abstract

The secondary structure of Na(+)/K(+)-ATPase after modification of the ATP-binding sites was analyzed. Consistently with recent reports, we found in trypsin-treated Na(+)/K(+)-ATPase additionally to alpha-helix also beta-sheet structures in the transmembrane segments. However, binding of fluorescein 5'-isothiocyanate (FITC), the pseudo-ATP analog, to the ATP-binding site did not affect the secondary structure of undigested Na(+)/K(+)-ATPase. Consequently, fluorescence intensity changes of FITC-labeled Na(+)/K(+)-ATPase commonly used to observe conformational transitions of the enzyme reflect physiological changes of the native structure. The metal complex analogues of ATP, Cr(H(2)O)(4)ATP and Co(NH(3))(4)ATP, on the other hand, affected the secondary structure of Na(+)/K(+)-ATPase. We propose that these changes in the secondary structure are responsible for inhibition of backdoor phosphorylation.

Published

2000

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

Author

Paolo Pelosi, Fabio Tanfani, Enrico Bertoli, Sara Paolini, and Carlo Fini

Subjects

Swine, Odorant binding, Biophysics, Analytical chemistry, Infrared spectroscopy, Ligands, Receptors, Odorant, Binding, Competitive, Biochemistry, Protein Structure, Secondary, Fluorescence spectroscopy, Structural Biology, Spectroscopy, Fourier Transform Infrared, Animals, Fourier transform infrared spectroscopy, Spectroscopy, Molecular Biology, Anthracenes, Molecular Structure, Chemistry, Ligand binding assay, Temperature, Fluorescence, Dissociation constant, Nasal Mucosa, Crystallography, Spectrometry, Fluorescence

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

33. Structural–Functional Relationships in Pig Heart AMP-Deaminase in the Presence of ATP, Orthophosphate, and Phosphatidate Bilayers

Author

Enrico Bertoli, E Kossowska, Dorota Kulawiak, Elizaveta Sarkissova, M M Zydowo, Jadwiga Purzycka Preis, Michal Wozniak, and Fabio Tanfani

Subjects

Hot Temperature, Protein Conformation, Swine, Endocrinology, Diabetes and Metabolism, Lipid Bilayers, Allosteric regulation, Phosphatidic Acids, Biochemistry, AMP Deaminase, Phosphates, Phosphatidate, Structure-Activity Relationship, chemistry.chemical_compound, Adenosine Triphosphate, Endocrinology, Non-competitive inhibition, Protein structure, Enzyme Stability, Spectroscopy, Fourier Transform Infrared, Genetics, Animals, Molecular Biology, Protein secondary structure, chemistry.chemical_classification, Myocardium, AMP deaminase, Phosphatidic acid, Enzyme, chemistry

Abstract

The secondary structure of pig heart AMP-deaminase (AMP-d) in the absence and in the presence of orthophosphate or dioleoyl phosphatidic acid (DOPA) or ATP was investigated by FT-IR spectroscopy. While the latter substance activates the enzyme, orthophosphate is a well-known negative allosteric effector and DOPA exerts a noncompetitive inhibition on AMP-deaminase. Small changes in the secondary structure of AMP-d were induced by the above mentioned substances. Only DOPA reduced the thermal stability of AMP-d and avoided protein intermolecular interactions suggesting structural–functional relationships in AMP-d in the presence of the above substances and a possible role of phosphatidic acid in the subtle regulation of AMP-d activity by temporary binding of the enzyme to cellular membranes.

Published

1998

34. Structure of yeast plasma membrane H+-ATPase: comparison of activated and basal-level enzyme forms

Author

Arnošt Kotyk, Georgios Lapathitis, Enrico Bertoli, and Fabio Tanfani

Subjects

Hot Temperature, Stereochemistry, ATPase, Adenylyl Imidodiphosphate, Saccharomyces cerevisiae, Biophysics, Infrared spectroscopy, Biochemistry, Protein Structure, Secondary, chemistry.chemical_compound, Secondary structure, Amide, Enzyme Stability, Spectroscopy, Fourier Transform Infrared, Enzyme Inhibitors, Diethylstilbestrol, Protein secondary structure, chemistry.chemical_classification, biology, Cell Biology, biology.organism_classification, Yeast, Enzyme Activation, Fourier transform-infrared (FT-IR) spectroscopy, Proton-Translocating ATPases, Yeast plasma membrane, Membrane, Enzyme, chemistry, biology.protein, H+-ATPase

Abstract

Plasma membrane H(+)-ATPase of the yeast Saccharomyces cerevisiae was isolated and purified in its two forms, the activated A-ATPase from glucose-metabolising cells, and the basal-level B-ATPase from cells with endogenous metabolism only. Structure of the two enzyme forms and the effects of beta, gamma-imidoadenosine 5'-triphosphate (AMP-PNP) and of diethylstilbestrol (DES) thereon were analysed by FT-IR spectroscopy. IR spectra revealed the presence of two populations of alpha-helices with different exposure to the solvent in both the A-ATPase and B-ATPase. AMP-PNP did not affect the secondary structure of A-ATPase while DES affected the ratio of the two alpha-helix populations. Thermal denaturation experiments suggested a more stable structure in the B-form than in the A-form. AMP-PNP stabilised the A-ATPase structure while DES destabilised both enzyme forms. IR spectra showed that 60% of the amide hydrogens were exchanged for deuterium in both forms at 20 degrees C. The remaining 40% were exchanged at higher temperatures. The maximum amount of H/D exchange was observed at 50-55 degrees C for both enzyme forms, while in the presence of DES it was observed at lower temperatures. The data do not contradict the possibility that the activation of H(+)-ATPase is due to the C-terminus of the enzyme dissociating from the ATP-binding site which is covered by it in the less active form.

Published

1998

35. Effects of temperature and SDS on the structure of β-glycosidase from the thermophilic archaeon Sulfolobus solfataricus

Author

Fabio Tanfani, Roberto Barone, Guido Barone, Roberto Nucci, Sabato D'Auria, Enrico Bertoli, Mosè Rossi, and Dimitrios Fessas

Subjects

Protein Denaturation, Circular dichroism, Spectrophotometry, Infrared, Detergents, ved/biology.organism_classification_rank.species, Infrared spectroscopy, Biochemistry, Protein Structure, Secondary, Sulfolobus, Differential scanning calorimetry, Protein structure, Bacterial Proteins, Molecular Biology, Protein secondary structure, Calorimetry, Differential Scanning, Chemistry, ved/biology, Circular Dichroism, Thermophile, Sulfolobus solfataricus, Temperature, Sodium Dodecyl Sulfate, Cell Biology, Protein tertiary structure, Crystallography, Glucosidases, Research Article

Abstract

The effects of temperature and SDS on the three-dimensional organization and secondary structure of β-glycosidase from the thermophilic archaeon Sulfolobus solfataricus were investigated by CD, IR spectroscopy and differential scanning calorimetry. CD spectra in the near UV region showed that the detergent caused a remarkable change in the protein tertiary structure, and far-UV CD analysis revealed only a slight effect on secondary structure. Infrared spectroscopy showed that low concentrations of the detergent (up to 0.02%) induced slight changes in the enzyme secondary structure, whereas high concentrations caused the α-helix content to increase at high temperatures and prevented protein aggregation.

Published

1997

36. HtrA Heat Shock Protease Interacts with Phospholipid Membranes and Undergoes Conformational Changes

Author

Fabio Tanfani, Joanna Skorko-Glonek, Barbara Lipinska, Enrico Bertoli, Konrad Krzewski, and Giovanna Zolese

Subjects

Cytoplasm, Protein Denaturation, Cardiolipins, Protein Conformation, Biology, complex mixtures, Biochemistry, Protein Structure, Secondary, chemistry.chemical_compound, Protein structure, Bacterial Proteins, Spectroscopy, Fourier Transform Infrared, Escherichia coli, Cardiolipin, Inner membrane, Molecular Biology, Heat-Shock Proteins, Phospholipids, Cellular localization, Phosphatidylglycerol, Phosphatidylethanolamines, Cell Membrane, Serine Endopeptidases, Peripheral membrane protein, Membranes, Artificial, Phosphatidylglycerols, Cell Biology, Periplasmic space, bacterial infections and mycoses, Protein tertiary structure, Spectrometry, Fluorescence, chemistry, bacteria, Periplasmic Proteins

Abstract

The HtrA (DegP) protein of Escherichia coli is a heat shock serine protease, essential for cell survival only at temperatures above 42 degrees C. It has been shown by genetic experiments that HtrA is an envelope protease, functioning in the periplasmic space. To clarify the cellular localization of HtrA, E. coli cells were fractionated, and HtrA was not detected by the immunoblotting technique in the periplasm or in the fraction of soluble proteins but was found in the inner membrane. The protein could be partially eluted from the total membrane fraction by a high ionic strength solution, whereas solutions affecting protein conformation released HtrA almost completely. These results, taken together with the evidence showing that HtrA functions in the periplasm, indicate that HtrA is a peripheral membrane protein, localized on the periplasmic side of the inner membrane. As the first step toward solving the problem of HtrA-membrane interactions, the structure of HtrA in the presence of phosphatidylglycerol (PG), phosphatidylethanolamine (PE), or cardiolipin (CL) was analyzed by fluorescence and Fourier-transform infrared spectroscopy. The infrared and fluorescence data indicated an interaction of HtrA with PG and CL but not with PE suspensions. Fluorescence spectroscopy revealed that this interaction was at the level of the polar head group of the phospholipid. In the PG/HtrA system, small changes were observed in the HtrA secondary structure and a remarkable decrease of the thermal stability of the protein, which suggested changes in HtrA tertiary structure. This suggestion was supported by fluorescence data that showed a shift of the fluorescence emission spectrum of HtrA tyrosine residues in the presence of PG and a reduced fluorescence intensity, phenomena not observed in the presence of PE or CL suspensions. Infrared data revealed also that the interaction of HtrA with PG leads to a protection of unfolded protein against aggregation at relatively low temperatures. The conformational changes of HtrA in the presence of PG influenced the proteolytic activity of HtrA by increasing it at the temperatures 37-45 degrees C and inhibiting it at 50-55 degrees C. CL inhibited HtrA activity at all of the temperatures tested.

Published

1997

37. Bovine α₁-acid glycoprotein, a thermostable version of its human counterpart: insights from Fourier transform infrared spectroscopy and in silico modelling

Author

Maurizio, Baldassarre, Roberta, Galeazzi, Beatrice, Maggiore, Fabio, Tanfani, and Andrea, Scirè

Subjects

Protein Folding, Protein Conformation, Protein Stability, Temperature, Orosomucoid, Hydrogen-Ion Concentration, Molecular Dynamics Simulation, Lipocalins, Protein Structure, Secondary, Spectroscopy, Fourier Transform Infrared, Animals, Humans, Cattle, Computer Simulation

Abstract

α1-Acid glycoprotein (AGP) is a plasma protein and a member of the acute phase response. AGP is known to bind and carry several biologically active compounds, as well as to down-modulate the immune system activities. In this work, the structure of bovine AGP has been investigated by Fourier-Transform infrared spectroscopy. A model structure has been obtained on the basis of human AGP and refined by molecular dynamics. In spite of the similar structure, bovine AGP shows an unexpectedly higher (∼20 °C) thermostability than its human counterpart. Inspection of the model structure has pointed out the presence of 12 ionic bridges and 2 sulphur-aromatic interactions, whereas only 6 ionic bridges were detected in human AGP. The high number (9) of glutamic acid residues involved in the ionic interactions might explain the significantly decreased thermostability measured at pH 5.5 (Tm ∼ 71 °C) with respect to pH 7.4 (Tm ∼ 81 °C), whereas thermostability of human AGP was only slightly affected by lowering the pH. As in human AGP and several other lipocalins, a temperature-induced molten globule state has been observed in the denaturation pathway of bovine AGP.

Published

2013

38. Comparison of the Structure of Wild-type HtrA Heat Shock Protease and Mutant HtrA Proteins

Author

Fabio Tanfani, Enrico Bertoli, Barbara Lipinska, Konrad Krzewski, and Joanna Skorko-Glonek

Subjects

Serine protease, Proteases, Protease, biology, medicine.medical_treatment, Mutant, Wild type, Cell Biology, bacterial infections and mycoses, complex mixtures, Biochemistry, Protein tertiary structure, Heat shock protein, biology.protein, medicine, bacteria, Denaturation (biochemistry), Molecular Biology

Abstract

The HtrA protease of Escherichia coli, identical with the DegP protease, is a 48-kDa heat shock protein, indispensable for bacterial survival only at temperatures above 42 °C. Proteolytic activity of HtrA is inhibited by diisopropyl fluorophosphate, suggesting that HtrA is a serine protease. We have recently found that mutational alteration of serine in position 210 of the mature HtrA or of histidine in position 105 totally eliminated proteolytic activity of HtrA. However, little was known about the consequences of the mutations on HtrA conformation. In this work, Fourier transform infrared spectroscopy has been used to examine the conformation in aqueous solution of wild-type HtrA and mutant HtrAS210 and HtrAH105 proteins. The spectra were collected at different temperatures in order to gain information also on the thermal stability of the three proteins. The analysis of HtrA protein spectrum, by resolution-enhancement methods, revealed that β-sheet is the major structural element of the conformation of HtrA. Deconvoluted as well as second derivative spectra of wild-type HtrA and mutant HtrAS210 and HtrAH105 collected at 20 °C were identical, indicating no differences in the secondary structure of these proteins. The analysis of spectra obtained at different temperatures revealed a maximum of protein denaturation within 65–70 °C for wild-type HtrA as well as for the HtrAS210 and HtrAH105 mutant proteins. However, the thermal denaturation pattern of wild-type HtrA revealed a lower cooperativity in the denaturation process as compared to the mutant proteins which instead behaved similarly. These data suggest that the mutations in HtrA protein induced minor changes in the tertiary structure of the protein (most likely located at the mutation sites). Our results strongly support the idea that Ser210 and His105 may represent two elements of the active-site triad (Ser, His, and Asp), found in most serine proteases. We have also found that in vitro, in the range from 37 to 55 °C, the proteolytic activity of HtrA rapidly increased with temperature and that HtrA activity remained unchanged for at least 4 h at 45 °C.

Published

1995

39. Quinolinic Aminoxyl Protects Albumin Against Peroxyl Radical Mediated Damage

Author

Fabio Tanfani, Jacek Kaczor, Kamil Jankowski, Andrzej Matuszkiewics, Elisabetta Damiani, Patricia Carloni, Dorota Kulawiak, Michal Wozniak, and Lucedio Greci

Subjects

Nitroxide mediated radical polymerization, Antioxidant, biology, Chemistry, medicine.medical_treatment, Electron Spin Resonance Spectroscopy, Albumin, A protein, Serum Albumin, Bovine, General Medicine, Photochemistry, Protein oxidation, Biochemistry, Antioxidants, Peroxides, Cyclic N-Oxides, Peroxyl radicals, Quinolines, medicine, biology.protein, Bovine serum albumin, Oxidation-Reduction

Abstract

A study of peroxyl radical-mediated bovine serum albumin oxidation in the presence of the quinolinic aminoxyl 1,2-dihydro-2,2-diphenyl-4-ethoxy-quinoline-1-oxyl (QAO) was carried out in order to test its efficiency as a protein antioxidant. Albumin oxidation was induced by the tert-butylhydroperoxide/PbO2 system. The extent of protein oxidation, measured by monitoring the formation of carbonyl groups, was considerably reduced in the presence of QAO. ESR measurements were carried out to confirm the consumption of the nitroxide during oxidation and its incorporation in the protein. The data obtained indicate that the quinolinic aminoxyl function can be used as an effective antioxidant in biological systems.

Published

1994

40. Characterization of thymoquinone binding to human α₁-acid glycoprotein

Author

Giulio, Lupidi, Emidio, Camaioni, Hamal, Khalifé, Luca, Avenali, Elisabetta, Damiani, Fabio, Tanfani, and Andrea, Scirè

Subjects

Models, Molecular, Binding Sites, Spectrometry, Fluorescence, Spectroscopy, Fourier Transform Infrared, Benzoquinones, Humans, Plant Oils, Thermodynamics, Hydrogen Bonding, Nigella sativa, Orosomucoid, Protein Binding

Abstract

Thymoquinone (TQ) is the main bioactive component isolated from Nigella sativa essential oil and seeds and has been used for the treatment of inflammations, liver disorders, arthritis, and is of great importance as a promising therapeutic drug for different diseases including cancer. This paper reports the first experimental evidence on binding of TQ to human α(1)-acid glycoprotein (AGP), an important drug-binding glycoprotein in human plasma, which affects pharmacokinetic properties of various therapeutic agents. The interaction of TQ with AGP has been characterized by Fourier transform infrared (FTIR) and fluorescence spectroscopy, as well as by molecular docking experiments. FTIR spectroscopy showed that the binding of TQ to AGP slightly increases its thermal stability and shifts the existence of a molten globule-like state observed in a previous study to higher temperature. The binding constants K(a); the number of binding sites n; and the corresponding thermodynamic parameters ΔG, ΔH, and ΔS at different temperatures were calculated through fluorescence spectroscopy. Fluorescence quenching experiments indicated that TQ binding involves hydrophobic interactions and to a lower extent hydrogen bonds, in agreement with molecular docking experiments. The data on binding ability of TQ to AGP represent basic information for the TQ pharmacokinetics such as drug metabolism and distribution in the body.

Published

2011

41. Importance of pH and disulfide bridges on the structural and binding properties of human α₁-acid glycoprotein

Author

Andrea, Scirè, Maurizio, Baldassarre, Giulio, Lupidi, and Fabio, Tanfani

Subjects

Structure-Activity Relationship, Protein Conformation, Temperature, Humans, Disulfides, Orosomucoid, Hydrogen-Ion Concentration, Ligands

Abstract

Human α(1)-acid glycoprotein (AGP) is an acute phase plasma glycoprotein containing two disulfide bridges. As a member of the lipocalin superfamily, it binds and transports several basic and neutral ligands, but a number of other activities have also been described. Thanks to its binding properties, AGP is also a good candidate for the development of biosensors and affinity chromatography media, and in this context detailed structural information is needed. The structural properties of AGP at different p(2)Hs and under reducing conditions were analysed by FT-IR spectroscopy. The obtained data indicate that AGP, when denatured, does not aggregate at neutral or basic p(2)Hs whilst it does at acidic p(2)Hs. Under reducing conditions the protein is remarkably less thermostable than its oxidized counterpart and presents an enhanced tendency to aggregate, even at neutral p(2)H. A heat-induced molten globule-like state (MG) was detected at 55 °C at p(2)H 7.4 and 5.5. At p(2)H 4.5 the MG occurred at 45 °C with an onset of formation at 40 °C. The MG was not observed under reducing conditions. A lower affinity of chlorpromazine and progesterone for the MG formed at p(2)H 4.5 and 40 °C was observed, suggesting that ligand(s) may be released near the negative surfaces of biological membranes. Furthermore, the reduced AGP displays an enhanced affinity for progesterone, indicating the importance of disulfide bonds for the binding capacity of AGP.

Published

2011

42. Indolinonic and quinolinic aminoxyls as protectants against oxidative stress

Author

Fabio Tanfani, Jerzy Popinigis, Michal Wozniak, Jedrzej Antosiewicz, Lucedio Greci, Enrico Bertoli, Elisabetta Damiani, and Stanislaw Przybylski

Subjects

Indoles, Antioxidant, Linolenic Acids, Linolenic acid, medicine.medical_treatment, chemistry.chemical_element, medicine.disease_cause, Biochemistry, Oxygen, Antioxidants, Cyclic N-Oxides, Lipid peroxidation, chemistry.chemical_compound, Oxygen Consumption, Malondialdehyde, Physiology (medical), medicine, Organic chemistry, Micelles, Hydrogen-Ion Concentration, chemistry, Peroxyl radicals, Quinolines, Lipid Peroxidation, Oxidation-Reduction, Oxidative stress, Nuclear chemistry

Abstract

A study on thermally and peroxyl radical induced oxidation of linolenic acid micelles in the presence of different concentrations of aminoxyls was carried out in order to test their efficiency as antioxidants in lipid peroxidation. The extent of peroxidation was measured by the malondialdehyde (MDA) produced and by oxygen consumption evaluated using an oxygraph. The results obtained indicate that indolinonic and quinolinic aminoxyls synthesized by us could be used as effective antioxidants in biological systems.

Published

1993

43. The interaction of phospholipid bilayers with pig heart AMP deaminase: Fourier-transform infrared spectroscopic and kinetic studies

Author

M M Zydowo, J Purzycka-Preis, Fabio Tanfani, E Kossowska, Michal Wozniak, E. Tartaglini, and Enrico Bertoli

Subjects

1,2-Dipalmitoylphosphatidylcholine, Spectrophotometry, Infrared, Swine, AMP deaminase activity, Adenylyl Imidodiphosphate, Lipid Bilayers, Phospholipid, Synthetic membrane, Biochemistry, Protein Structure, Secondary, AMP Deaminase, chemistry.chemical_compound, Adenosine Triphosphate, Phosphatidylcholine, Animals, Molecular Biology, Phospholipids, Liposome, Fourier Analysis, Myocardium, AMP deaminase, Biological membrane, Cell Biology, Kinetics, Membrane, chemistry, Phosphatidylcholines, lipids (amino acids, peptides, and proteins), Research Article

Abstract

The interaction of pig heart AMP deaminase with different chemical species of phosphatidylcholine and with natural plasma membranes has been investigated. Phospholipids added to the system either as natural biological membranes (plasma membrane vesicles) or in the form of liposomes containing unsaturated phosphatidylcholine considerably enhanced AMP deaminase activity. The secondary structure of pig heart AMP deaminase in the absence and in the presence of dioleoyl phosphatidylcholine and dipalmitoyl phosphatidylcholine liposomes was investigated by Fourier-transform infrared spectroscopy. Quantitative analysis of the amide I band showed that the enzyme contains 45% beta-sheets, 28% alpha-helix, 16% turns and 11% non-ordered structure. In the presence of dioleoyl phosphatidylcholine liposomes, the beta/alpha content ratio decreased; this decrease was dependent on the amount of lipid added. This phenomenon was not observed in the case of dipalmitoyl phosphatidylcholine liposomes. These data suggest a possible role for membrane phospholipids in the regulation of AMP deaminase activity.

Published

1993

44. On the use of 1,3-diphenylisobenzofuran (DPBF). Reactions with carbon and oxygen centered radicals in model and natural systems

Author

Pierluigi Stipa, Elisabetta Damiani, Lucedio Greci, Fabio Tanfani, Michal Wozniak, E. Tartaglini, and Patricia Carloni

Subjects

chemistry.chemical_compound, chemistry, Bicyclic molecule, Singlet oxygen, Radical, Alkoxy group, Molecule, Reactivity (chemistry), General Chemistry, Photochemistry, Catalysis, Adduct

Abstract

1,3-diphenylisobenzofuran (DPBF) is a fluorescent molecule which possesses a highly specific reactivity towards singlet oxygen (1O2) forming an endoperoxide which decomposes to give 1,2-dibenzoylbenzene. This reaction between DPBF and 1O2 can be followed by measuring the decrease in fluorescence intensity of DPBF. In order to check the specificity of DPBF toward free radicals a series of experiments was carried out in Triton-X micelles and in natural systems (rat liver microsomes), in which DPBF was reacted with hydroxy (HO•), alkyloxy (RO•), alkylperoxy (ROO•), and C-centered radicals (2-cyanoisopropyl radical). In all cases, the DPBF is rapidly transformed to 1,2-dibenzoylbenzene in the case of O-centered radicals and to the corresponding adduct in the case of 2-cyanoisopropyl radical. The experiments in the model systems were also carried out from the chemical point of view and the reaction products were isolated and identified. From the results obtained, it should be stressed that DPBF must be used with caution in complex biological systems for the detection of 1O2, as it also reacts with different radical species.

Published

1993

45. The role of the L2 loop in the regulation and maintaining the proteolytic activity of HtrA (DegP) protein from Escherichia coli

Author

Tomasz Koper, Barbara Lipinska, Anna Sobiecka-Szkatula, Fabio Tanfani, Donata Figaj, Artur Giełdoń, Andrea Scirè, Jerzy Ciarkowski, and Joanna Skorko-Glonek

Subjects

DNA, Bacterial, Models, Molecular, Protein Denaturation, Hot Temperature, Protein Conformation, Biophysics, Virulence, Biology, medicine.disease_cause, Biochemistry, Protein structure, Valine, Catalytic Domain, Spectroscopy, Fourier Transform Infrared, medicine, Escherichia coli, Protein Structure, Quaternary, Molecular Biology, Heat-Shock Proteins, DNA Primers, Sequence Deletion, Base Sequence, Escherichia coli Proteins, Serine Endopeptidases, Regulatory loop, Recombinant Proteins, Amino Acid Substitution, Mutagenesis, Site-Directed, bacteria, Mutant Proteins, Periplasmic Proteins, Plasmids

Abstract

The aim of this study was to characterize the role of particular elements of the regulatory loop L2 in the activation process and maintaining the proteolytic activity of HtrA (DegP) from Escherichia coli . We measured the effects of various mutations introduced to the L2 loop’s region (residues 228–238) on the stability of HtrA molecule and its proteolytic activity. We demonstrated that most mutations affected the activity of HtrA. In the case of the following substitutions: L229N, N235I, I238N, the proteolytic activity was undetectable. Thus, the majority of interactions mediated by the studied amino-acid residues seem to play important role in maintaining the active conformation. Formation of contacts between the apical parts (residues 231–234) of the L2 loops within the HtrA trimer, in particular the residues D232, was shown to play a crucial role in the activation process of HtrA. Stabilization of these intermolecular interactions by substitution of D232 with valine caused a stimulation of proteolytic activity whereas deletion of this region abolished the activity. Since the pathogenic E. coli strains require active HtrA for virulence, the apical part of L2 is of particular interest in terms of structure-based drug design for treatment E. coli infections.

Published

2010

46. CHARACTERIZATION OF THE MOLECULAR ORGANIZATION AND STRUCTURAL STABILITY OF AN ARGININE-BINDING PROTEIN IN Thermotoga maritima

Author

Andrea, Sciré, Marabotti, Anna, Maria, Staiano, Luisa, Iozzino, Luchansky, Matthew S., Der, Bryan S., Dattelbaum, Jonathan D., Fabio, Tanfani, and Sabato, D’Auria

Published

2010

47. Amino acid transport in thermophiles: characterization of an arginine-binding protein in Thermotoga maritima. 2. Molecular organization and structural stability

Author

Maria Staiano, Anna Marabotti, Bryan S. Der, Andrea Scirè, Fabio Tanfani, Matthew S. Luchansky, Sabato D'Auria, Luisa Iozzino, and Jonathan D. Dattelbaum

Subjects

Models, Molecular, Arginine, COMPUTATIONAL DESIGN, Molecular Sequence Data, Biological Transport, Active, Molecular Dynamics Simulation, Protein Structure, Secondary, TRANSFORM INFRARED-SPECTROSCOPY, ABC TRANSPORTERS, Bacterial Proteins, Spectroscopy, Fourier Transform Infrared, GENETICALLY-ENGINEERED PROTEIN, Thermotoga maritima, Amino Acid Sequence, Amino Acids, Molecular Biology, Peptide sequence, chemistry.chemical_classification, biology, CONSTRUCTION, Protein Stability, Systems Biology, Protein dynamics, Binding protein, Hydrogen-Ion Concentration, Ligand (biochemistry), biology.organism_classification, Amino acid, Biochemistry, chemistry, Structural Homology, Protein, Thermodynamics, Carrier Proteins, Arginine binding, Biotechnology

Abstract

ABC transport systems provide selective passage of metabolites across cell membranes and typically require the presence of a soluble binding protein with high specificity to a specific ligand. In addition to their primary role in nutrient gathering, the binding proteins associated with bacterial transport systems have been studied for their potential to serve as design scaffolds for the development of fluorescent protein biosensors. In this work, we used Fourier transform infrared spectroscopy and molecular dynamics simulations to investigate the physicochemical properties of a hyperthermophilic binding protein from Thermotoga maritima. We demonstrated preferential binding for the polar amino acid arginine and experimentally monitored the significant stabilization achieved upon binding of ligand to protein. The effect of temperature, pH, and detergent was also studied to provide a more complete picture of the protein dynamics. A protein structure model was obtained and molecular dynamic experiments were performed to investigate and couple the spectroscopic observations with specific secondary structural elements. The data determined the presence of a buried beta-sheet providing significant stability to the protein under all conditions investigated. The specific amino acid residues responsible for arginine binding were also identified. Our data on dynamics and stability will contribute to our understanding of bacterial binding protein family members and their potential biotechnological applications.

Published

2010

48. Thymoquinone, a potential therapeutic agent of Nigella sativa, binds to site I of human serum albumin

Author

Elisabetta Damiani, Emidio Camaioni, G. De Sanctis, Andrea Scirè, Kh Khalife, Fabio Tanfani, and Giulio Lupidi

Subjects

Models, Molecular, Circular dichroism, Stereochemistry, Serum albumin, Pharmaceutical Science, Thymoquinone, Nigella sativa, Human serum albumin, Drug-protein complex, FT-IR, Fluorescence quenching, Molecular modelling and docking, Protein Structure, Secondary, Hydrophobic effect, chemistry.chemical_compound, In vivo, Drug Discovery, Spectroscopy, Fourier Transform Infrared, medicine, Benzoquinones, Humans, Binding site, Serum Albumin, Pharmacology, Binding Sites, biology, Chemistry, Binding constant, body regions, Spectrometry, Fluorescence, Complementary and alternative medicine, embryonic structures, biology.protein, Molecular Medicine, medicine.drug

Abstract

Thymoquinone (TQ) is the main constituent of Nigella sativa essential oil which shows promising in vitro and in vivo antineoplastic growth inhibition against various tumor cell lines. Because of the increasing interest to test it in pre-clinical and clinical researches for assessing its health benefits, we here evaluate the interactions between TQ and human serum albumin (HSA), a possible carrier of this drug in vivo. Binding to HSA was studied using different spectroscopic techniques. Fourier transform infrared (FT-IR) and circular dichroism (CD) spectroscopies suggest that the association between TQ and HSA does not affect the secondary structure of HSA. Using fluorescence spectroscopy, one mole of TQ was found to bind one mole of HSA with a binding constant of 2.39 +/- 0.2 10(4)M(-1). At 25 degrees C (pH 7.4), van't Hoff's enthalpy and entropy that accompany the binding were found to be -10.24 kJ/mol(-1) and 45 J/mol(-1)K(-1) respectively. The thermodynamic analysis of the TQ-HSA complex formation shows that the binding process is enthalpy driven and spontaneous, and that hydrophobic interactions are the predominant intermolecular forces stabilizing the complex. Furthermore, displacement experiments using warfarin and ibuprofen indicate that TQ could bind to site I of HSA, which is also in agreement with the results of the molecular modeling study.

Published

2010

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

Author

Fabio Tanfani, Ardesio Floridi, Enrico Bertoli, Carlo Fini, and Gianni Albertini

Subjects

Male, Nitrilotriacetic Acid, Spectrophotometry, Infrared, Protein Conformation, Protein subunit, Biophysics, Analytical chemistry, Infrared spectroscopy, chemistry.chemical_element, Zinc, Biochemistry, chemistry.chemical_compound, Semen, Structural Biology, Metalloprotein, Animals, Denaturation (biochemistry), Fourier transform infrared spectroscopy, 5'-Nucleotidase, Molecular Biology, Protein secondary structure, chemistry.chemical_classification, Fourier Analysis, Nitrilotriacetic acid, Dithiothreitol, Crystallography, chemistry, Cattle

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

50. Wild-type and mutant bovine odorant-binding proteins to probe the role of the quaternary structure organization in the protein thermal stability

Author

Fabio Tanfani, Andrea Scirè, Roberta Crescenzo, Sabato D'Auria, Vincenzo Aurilia, Anna Marabotti, and Maria Staiano

Subjects

Models, Molecular, Spectrophotometry, Infrared, Odorant binding, Molecular Conformation, Receptors, Odorant, Biochemistry, Hydrophobic effect, Molecular dynamics, Protein structure, Spectroscopy, Fourier Transform Infrared, Animals, Computer Simulation, Protein Structure, Quaternary, biology, Chemistry, MD, Wild type, Temperature, General Chemistry, Lipocalins, Protein Structure, Tertiary, FT-IR, Crystallography, Odorant-binding protein, Mutation, biology.protein, Protein quaternary structure, Cattle, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

The exploration of events taking place at different timescales and affecting the structural and dynamics properties of proteins, such as the interactions of proteins with ligands and the subunits association/ dissociation, must necessarily be performed by using different methodologies, each of which specialized to highlight the different phenomena that occur when proteins are exposed to chemical or physical stress. In this work, we investigated the structure and dynamics of the wild-type bovine odorant-binding protein (wt-bOBP), which is a domain-swapped dimeric protein, and the triple mutant deswapped monomeric form of the protein (m-bOBP) to shed light on the role of the quaternary and tertiary structural organization in the protein thermal stability. Difference infrared spectra, 2D-IR correlation spectroscopy and molecular dynamics simulations were used to probe the effect of heating on protein structure and dynamics in microsecond and nanoseconds temporal ranges, respectively. The obtained results show that there is a heating-induced transition toward a less structured state in m-bOBP, that it is detectable around 70-80 degrees C. On the contrary, in wt-bOBP this transition is almost negligible, and changes are detectable in the protein spectra in the range of temperature between 75 and 85 degrees C. A detailed 3D inspection of the structure of the two proteins that takes into the account the spectroscopic results indicates that (a) ion pairs and hydrophobic interactions appear to be the major determinants responsible for the protein stability and (b) the protein intersubunit interactions confer an increased resistance toward the thermal stress.

Published

2009