Your search keyword '"Rossi, Mose'"' showing total 83 results

1. High-level expression of Aliciclobacillus acidocaldarius thioredoxin in Pichia pastoris and Bacillus subtilis

Author

Rossi Mose, Digilio Filomena Anna, Morra Rosa, Pedone Emilia, Bartolucci Simonetta, Digilio, Fa, Morra, R, Pedone, E, Bartolucci, Simonetta, and Rossi, Mose'

Subjects

biology, Gene Expression, Bacillus subtilis, Alicyclobacillus acidocaldariu, Pichia pastori, medicine.disease_cause, biology.organism_classification, Molecular biology, Yeast, Pichia, Recombinant Proteins, Pichia pastoris, Thioredoxins, Bacterial Proteins, high-level expression, Gene expression, medicine, Bacillus subtili, Thioredoxin, Escherichia coli, Biotechnology, Thermophilic organism

Abstract

Thioredoxins are ubiquitous proteins which catalyze the reduction of disulfide bridges on target proteins and are involved in many cellular reactions. In a previous work, a thioredoxin from the thermophilic organism Aliciclobacillus acidocaldarius (Alitrx) was purified, characterized, and its gene expressed in Escherichia coli. In order to produce larger quantities of Alitrx, the protein has been expressed in the methylotrophic yeast Pichia pastoris and in the gram positive bacteria Bacillus subtilis. The growth conditions of strains showing high-level expression of Alitrx were optimized for both systems in shake-flask cultures. Active proteins were secreted in the culture media at a level of approximately 0.9 and 0.5 g/l, respectively, for P. pastoris and B. subtilis. The proteins were purified almost to homogeneity by a thermal precipitation procedure, with a 90-fold and 50-fold higher total yield with respect to that obtained with the same protein expressed in E. coli. The results indicate that either of these two systems could be utilized as a host for large-scale production of recombinant Alitrx.

Published

2003

2. Introducing transgalactosylation activity into a family 42 β-galactosidase

Author

Beatrice Cobucci-Ponzano, Maria Michela Corsaro, Andrea Strazzulli, Mosè Rossi, Sara Carillo, Emiliano Bedini, Stephen G. Withers, Gabriella Pocsfalvi, Marco Moracci, Strazzulli, Andrea, Cobucci Ponzano, Beatrice, Carillo, Sara, Bedini, Emiliano, Corsaro, MARIA MICHELA, Pocsfalvi, Gabriella, Withers, Stephen G, Rossi, Mose', and Moracci, Marco

Subjects

0301 basic medicine, Glycosylation, Alicyclobacillus, transgalactosylation, Oligosaccharides, Biochemistry, Catalysis, Substrate Specificity, 03 medical and health sciences, chemistry.chemical_compound, Hydrolysis, Catalytic Domain, chemical rescue, Glycoside hydrolase, chemistry.chemical_classification, biology, oligosaccharide synthesis, Sodium formate, thermophilic glycosidases, Mutagenesis, Active site, Glycosynthase, Oligosaccharide, beta-Galactosidase, Combinatorial chemistry, Kinetics, 030104 developmental biology, Amino Acid Substitution, chemistry, Mutation, biology.protein, Sodium azide, glycosynthase

Abstract

Chemo-enzymatic synthesis of oligosaccharides exploits the diversity of glycosidases and their ability to promote transglycosylation reactions in parallel with hydrolysis. Methods to increase the transglycosylation/hydrolysis ratio include site-directed mutagenesis and medium modification. The former approach was successful in several cases and has provided the best synthetic yields with glycosynthases-mutants at the catalytic nucleophile position that promote transglycosylation with high efficiency, but do not hydrolyze the oligosaccharide products. Several glycosidases have proven recalcitrant to this conversion, thus alternative methods to increase the transglycosylation/hydrolysis ratio by mutation would be very useful. Here we show that a mutant of a β-galactosidase from Alicyclobacillus acidocaldarius in an invariant residue in the active site of the enzymes of this family (glutamic acid 361) carries out efficient transglycosylation reactions on different acceptors only in the presence of external ions with yields up to 177-fold higher than that of the wild type. This is the first case in which sodium azide and sodium formate in combination with site-directed mutagenesis have been used to introduce transglycosylation activity into a glycosidase. These observations will hopefully guide further efforts to generate useful synthases.

Published

2017

3. Production and covalent immobilisation of the recombinant bacterial carbonic anhydrase (SspCA) onto magnetic nanoparticles

Author

Claudiu T. Supuran, Sonia Del Prete, Clemente Capasso, C.M.A. Barone, Mosè Rossi, Giovanni Sansone, Daniela Vullo, Rosa Perfetto, Perfetto, Rosa, del Prete, Sonia, Vullo, Daniela, Sansone, Giovanni, Barone, CARMELA MARIA ASSUNTA, Rossi, Mose, Supuran, Claudiu T., and Capasso, Clemente

Subjects

immobilised enzyme, magnetic nanoparticles, metalloenzyme, magnetic nanoparticle, 01 natural sciences, Catalysis, law.invention, Gram-Negative Chemolithotrophic Bacteria, law, Carbonic anhydrase, Drug Discovery, Enzyme kinetics, Magnetite Nanoparticles, Carbonic Anhydrases, Thermostability, Pharmacology, chemistry.chemical_classification, metalloenzymes, biology, 010405 organic chemistry, Chemistry, Thermophile, lcsh:RM1-950, General Medicine, Recombinant Proteins, thermostability, 0104 chemical sciences, 010404 medicinal & biomolecular chemistry, Enzyme, lcsh:Therapeutics. Pharmacology, Biochemistry, Covalent bond, biology.protein, Recombinant DNA, high cell density, Research Paper

Abstract

Carbonic anhydrases (CAs; EC 4.2.1.1) are metalloenzymes with a pivotal potential role in the biomimetic CO2 capture process (CCP) because these biocatalysts catalyse the simple but physiologically crucial reaction of carbon dioxide hydration to bicarbonate and protons in all life kingdoms. The CAs are among the fastest known enzymes, with kcat values of up to 106 s−1 for some members of the superfamily, providing thus advantages when compared with other CCP methods, as they are specific for CO2. Thermostable CAs might be used in CCP technology because of their ability to perform catalysis in operatively hard conditions, typical of the industrial processes. Moreover, the improvement of the enzyme stability and its reuse are important for lowering the costs. These aspects can be overcome by immobilising the enzyme on a specific support. We report in this article that the recombinant thermostable SspCA (α-CA) from the thermophilic bacterium Sulfurihydrogenibium yellowstonense can been heterologously produced by a high-density fermentation of Escherichia coli cultures, and covalently immobilised onto the surface of magnetic Fe3O4 nanoparticles (MNP) via carbodiimide activation reactions. Our results demonstrate that using a benchtop bioprocess station and strategies for optimising the bacterial growth, it is possible to produce at low cost a large amount SspCA. Furthermore, the enzyme stability and storage greatly increased through the immobilisation, as SspCA bound to MNP could be recovered from the reaction mixture by simply using a magnet or an electromagnetic field, due to the strong ferromagnetic properties of Fe3O4.

Published

2017

4. Diversity of bacteria and archaea from two shallow marine hydrothermal vents from Vulcano Island

Author

Jenny M. Blamey, Nils-Kåre Birkeland, Christian Schäfers, Yoshizumi Ishino, Elizaveta A. Bonch-Osmolovskaya, Robert M. Kelly, Reinhard Sterner, Mosè Rossi, Michael Thomm, Tairo Oshima, Frank T. Robb, Don A. Cowan, Patrick Forterre, Garabed Antranikian, Jennifer A. Littlechild, Marcel Suleiman, Helena Santos, Peter Schönheit, Michael J. Danson, Michael W. W. Adams, Kenneth M. Noll, Milton S. da Costa, Marco Moracci, Jürgen Wiegel, Rudolf K. Thauer, Simonetta Bartolucci, Karl O. Stetter, Antranikian, Garabed, Suleiman, Marcel, Schäfers, Christian, Adams, Michael W. W, Bartolucci, Simonetta, Blamey, Jenny M, Birkeland, Nils Kåre, Bonch Osmolovskaya, Elizaveta, da Costa, Milton S, Cowan, Don, Danson, Michael, Forterre, Patrick, Kelly, Robert, Ishino, Yoshizumi, Littlechild, Jennifer, Moracci, Marco, Noll, Kenneth, Oshima, Tairo, Robb, Frank, Rossi, Mose', Santos, Helena, Schönheit, Peter, Sterner, Reinhard, Thauer, Rudolf, Thomm, Michael, Wiegel, Jürgen, and Stetter, Karl Otto

Subjects

0301 basic medicine, 030106 microbiology, Hydrothermal marine shallow vent, Marine Biology, Hydrothermal marine shallow vents, Microbiology, 03 medical and health sciences, Hydrothermal Vents, Microbial ecology, Staphylothermus, Sulfurimonas, RNA, Ribosomal, 16S, Botany, Diversity, biology, Bacteria, Ecology, General Medicine, biology.organism_classification, Palaeococcus, Archaea, Hyperthermophile, 030104 developmental biology, Italy, Molecular Medicine, Hyperthermophiles, Thermococcus, Hydrothermal vent

Abstract

To obtain new insights into community compositions of hyperthermophilic microorganisms, defined as having optimal growth temperatures of 80 degrees C and above, sediment and water samples were taken from two shallow marine hydrothermal vents (I and II) with temperatures of 100 degrees C at Vulcano Island, Italy. A combinatorial approach of denaturant gradient gel electrophoresis (DGGE) and metagenomic sequencing was used for microbial community analyses of the samples. In addition, enrichment cultures, growing anaerobically on selected polysaccharides such as starch and cellulose, were also analyzed by the combinatorial approach. Our results showed a high abundance of hyperthermophilic archaea, especially in sample II, and a comparable diverse archaeal community composition in both samples. In particular, the strains of the hyperthermophilic anaerobic genera Staphylothermus and Thermococcus, and strains of the aerobic hyperthermophilic genus Aeropyrum, were abundant. Regarding the bacterial community, e-Proteobacteria, especially the genera Sulfurimonas and Sulfurovum, were highly abundant. The microbial diversity of the enrichment cultures changed significantly by showing a high dominance of archaea, particularly the genera Thermococcus and Palaeococcus, depending on the carbon source and the selected temperature.

Published

2017

5. Sequence Analysis, Kinetic Constants, and Anion Inhibition Profile of the Nacrein-Like Protein (CgiNAP2X1) from the Pacific Oyster Magallana gigas (Ex-Crassostrea gigas)

Author

Sonia Del Prete, Clemente Capasso, Giovanni Sansone, Claudiu T. Supuran, Rosa Perfetto, Daniela Vullo, C.M.A. Barone, Mosè Rossi, Perfetto, Rosa, Del Prete, Sonia, Vullo, Daniela, Sansone, Giovanni, Barone, CARMELA MARIA ASSUNTA, Rossi, Mose', Supuran, Claudiu T, and Capasso, Clemente

Subjects

Anions, Bicarbonate, carbonic anhydrase, Pharmaceutical Science, anion inhibitors, anion inhibitor, phylogeny, 01 natural sciences, Article, chemistry.chemical_compound, Carbonic anhydrase, Drug Discovery, Animals, nacrein-like protein, signal peptide, Enzyme kinetics, Phenylboronic acid, molluskan, kinetic constants, lcsh:QH301-705.5, Pharmacology, Toxicology and Pharmaceutics (miscellaneous), Peptide sequence, Sulfamide, Carbonic Anhydrases, chemistry.chemical_classification, Pacific Ocean, biology, 010405 organic chemistry, kinetic constant, Phenylarsonic acid, Ostreidae, 0104 chemical sciences, Kinetics, 010404 medicinal & biomolecular chemistry, Enzyme, lcsh:Biology (General), chemistry, Biochemistry, Mollusca, biology.protein

Abstract

The carbonic anhydrase (CA, EC 4.2.1.1) superfamily of metalloenzymes catalyzes the hydration of carbon dioxide to bicarbonate and protons. The catalytically active form of these enzymes incorporates a metal hydroxide derivative, the formation of which is the rate-determining step of catalytic reaction, being affected by the transfer of a proton from a metal-coordinated water molecule to the environment. Here, we report the cloning, expression, and purification of a particular CA, i.e., nacrein-like protein encoded in the genome of the Pacific oyster Magallana gigas (previously known as Crassostrea gigas). Furthermore, the amino acid sequence, kinetic constants, and anion inhibition profile of the recombinant enzyme were investigated for the first time. The new protein, CgiNAP2X1, is highly effective as catalyst for the CO₂ hydration reaction, based on the measured kinetic parameters, i.e., kcat = 1.0 × 10⁶ s(-1) and kcat/KM = 1.2 × 10⁸ M(-1)·s(-1). CgiNAP2X1 has a putative signal peptide, which probably allows an extracellular localization of the protein. The inhibition data demonstrated that the best anion inhibitors of CgiNAP2X1 were diethyldithiocarbamate, sulfamide, sulfamate, phenylboronic acid and phenylarsonic acid, which showed a micromolar affinity for this enzyme, with KIs in the range of 76-87 μM. These studies may add new information on the physiological role of the molluskan CAs in the biocalcification processes.

Published

2017

6. Translational recoding in archaea

Author

Mosè Rossi, Beatrice Cobucci-Ponzano, Marco Moracci, Cobucci Ponzano, Beatrice, Rossi, Mose', and Moracci, Marco

Subjects

Archaeal Proteins, Pseudogene, Pyrrolysine, Programmed frameshifting, Biology, Microbiology, Ribosome, Stop codon readthrough, chemistry.chemical_compound, Archaeal Protein, Genetics, chemistry.chemical_classification, Translational frameshift, Selenocysteine, Lysine, Frameshifting, Ribosomal, General Medicine, Ribosomal RNA, Archaea, Stop codon, Amino acid, chemistry, Hyperthermophiles, Molecular Medicine, Gene expression, Pseudogenes

Abstract

Translational recoding includes a group of events occurring during gene translation, namely stop codon readthrough, programmed +/- 1 frameshifting, and ribosome bypassing, which have been found in organisms from all domains of life. They serve to regulate protein expression at translational level and represent a relatively less known exception to the traditional central 'dogma' of biology that information flows as DNA -> RNA -> protein and that it is stored in a co-linear way between the 5'-> 3' of nucleic acids and N -> C-terminal of polypeptides. In archaea, in which translational recoding regulates the decoding of the 21st and the 22nd amino acids selenocysteine and pyrrolysine, respectively, only one case of programmed -1 frameshifting has been reported so far and further examples, although promising, have not been confirmed yet. We here summarize the current state-of-the-art of this field that, especially in archaea, has relevant implications for the physiology of life in extreme environments and for the origin of life.

Published

2012

7. Glycosynthases in Biocatalysis

Author

Andrea Strazzulli, Mosè Rossi, Beatrice Cobucci-Ponzano, Marco Moracci, Cobucci Ponzano, Beatrice, Strazzulli, Andrea, Rossi, Mose', and Moracci, Marco

Subjects

Glycan, biology, Glycobiology, Chemistry, Carbohydrate synthesis, General Chemistry, Glycosynthase, Combinatorial chemistry, glycoconjugates, biotransformations, carbohydrate synthesis, glycobiology, Biocatalysis, biology.protein, Organic chemistry, Glycoside hydrolase, glycoproteins

Abstract

Glycosynthases, engineered glycoside hydrolases that are able to synthesize glycans in quantitative yields without hydrolyzing them, are among the most interesting tools for the chemoenzymatic synthesis of carbohydrates that have been made available so far. From their invention in 1998, these enzymes have been developed enormously and demonstrated to be convenient alternatives to the more expensive glycosyltransferase. Glycosynthases have been proved to be efficient catalysts for the synthesis of oligosaccharides, polysaccharides, and glycoconjugates of various lengths containing different monosaccharides bound through alpha- and beta-linkages, which have interesting applications. In this review we describe the impact that glycosynthases have had on the biocatalysis and biosynthesis of carbohydrates through the description of the novel activities produced and of the development of the glycosynthase-based process. In addition, we summarize the approaches that, according to the current literature, can be adopted to produce novel glycosynthase activities and to improve the existing process.

Published

2011

8. Role of Tryptophan 95 in substrate specificity and structural stability of Sulfolobus solfataricus alcohol dehydrogenase

Author

Luciana Esposito, Angela Pennacchio, Adriana Zagari, Mosè Rossi, Carlo A. Raia, Pennacchio, A., Esposito, L., Zagari, Adriana, Rossi, Mose', and Raia, C. A.

Subjects

Models, Molecular, Protein Denaturation, Protein Conformation, Stereochemistry, Archaeal Proteins, ved/biology.organism_classification_rank.species, Crystallography, X-Ray, Microbiology, Cofactor, Genes, Archaeal, Substrate Specificity, Structural stability, Oxidoreductase, Catalytic Domain, Enzyme Stability, Coenzyme binding, Alcohol dehydrogenase, chemistry.chemical_classification, biology, Chemistry, ved/biology, Sulfolobus solfataricus, Temperature, Tryptophan, Alcohol Dehydrogenase, Active site, Substrate (chemistry), General Medicine, Hydrogen-Ion Concentration, Sulfolobu, NAD, Recombinant Proteins, Kinetics, Spectrometry, Fluorescence, Amino Acid Substitution, Mutagenesis, Site-Directed, biology.protein, Molecular Medicine, NAD+ kinase

Abstract

A mutant of the thermostable NAD(+)-dependent (S)-stereospecific alcohol dehydrogenase from Sulfolobus solfataricus (SsADH) which has a single substitution, Trp95Leu, located at the substrate binding pocket, was fully characterized to ascertain the role of Trp95 in discriminating between chiral secondary alcohols suggested by the wild-type SsADH crystallographic structure. The Trp95Leu mutant displays no apparent activity with short-chain primary and secondary alcohols and poor activity with aromatic substrates and coenzyme. Moreover, the Trp --> Leu substitution affects the structural stability of the archaeal ADH, decreasing its thermal stability without relevant changes in secondary structure. The double mutant Trp95Leu/Asn249Tyr was also purified to assist in crystallographic analysis. This mutant exhibits higher activity but decreased affinity toward aliphatic alcohols, aldehydes as well as NAD(+) and NADH compared to the wild-type enzyme. The crystal structure of the Trp95Leu/Asn249Tyr mutant apo form, determined at 2.0 A resolution, reveals a large local rearrangement of the substrate site with dramatic consequences. The Leu95 side-chain conformation points away from the catalytic metal center and the widening of the substrate site is partially counteracted by a concomitant change of Trp117 side chain conformation. Structural changes at the active site are consistent with the reduced activity on substrates and decreased coenzyme binding.

Published

2009

9. Inhibition of translesion DNA polymerase by archaeal reverse gyrase

Author

Anna Valenti, Giuseppe Perugino, Maria Ciaramella, Takehiko Nohmi, Mosè Rossi, Valenti, Anna, Perugino, Giuseppe, Nohmi, Takehiko, Rossi, Mosè, Ciaramella, Maria, Valenti, A., Perugino, G., Takehiko, N., Rossi, Mose', and M. Ciaramella M.

Subjects

biology, DNA polymerase, ved/biology, DNA damage, Sulfolobus solfataricus, ved/biology.organism_classification_rank.species, DNA polymerase beta, Genome Integrity, Repair and Replication, Sulfolobus solfataricu, DNA gyrase, chemistry.chemical_compound, DNA Topoisomerases, Type I, chemistry, Biochemistry, Genetics, biology.protein, DNA supercoil, DNA Polymerase beta, DNA, Polymerase, DNA Damage

Abstract

Reverse gyrase is a unique DNA topoisomerase endowed with ATP-dependent positive supercoiling activity. It is typical of microorganisms living at high temperature and might play a role in maintenance of genome stability and repair. We have identified the translesion DNA polymerase SsoPolY/Dpo4 as one partner of reverse gyrase in the hyperthermophilic archaeon Sulfolobus solfataricus. We show here that in cell extracts, PolY and reverse gyrase co-immunoprecipitate with each other and with the single strand binding protein, SSB. The interaction is confirmed in vitro by far-western and Surface Plasmon Resonance. In functional assays, reverse gyrase inhibits PolY, but not the S. solfataricus B-family DNA polymerase PolB1. Mutational analysis shows that inhibition of PolY activity depends on both ATPase and topoisomerase activities of reverse gyrase, suggesting that the intact positive supercoiling activity is required for PolY inhibition. In vivo, reverse gyrase and PolY are degraded after induction of DNA damage. Inhibition by reverse gyrase and degradation might act as a double mechanism to control PolY and prevent its potentially mutagenic activity when undesired. Inhibition of a translesion polymerase by topoisomerase-induced modification of DNA structure may represent a previously unconsidered mechanism of regulation of these two-faced enzymes.

Published

2009

10. Structural determinants of the high thermal stability of SsoPox from the hyperthermophilic archaeon Sulfolobus solfataricus

Author

Jérôme Dupuy, Luigia Merone, Paola Carullo, Pompea Del Vecchio, Mosè Rossi, Giuseppe Graziano, Giuseppe Manco, Bertrand Fournier, Mikael Elias, Daniel Rochu, Eric Chabrière, Luigi Mandrich, Patrick Masson, P., Del Vecchio, M., Elia, L., Merone, G., Graziano, J., Dupuy, L., Mandrich, P., Carullo, B., Fournier, D., Rochu, Rossi, Mose', Masson, E., Chabriere E, G., Manco, DEL VECCHIO, POMPEA GIUSEPPINA GRAZIA, Carullo, Paola, P., Masson, E., Chabiere, and G. M. A. N. C., O.

Subjects

Models, Molecular, Circular dichroism, Protein Conformation, Stereochemistry, Archaeal Proteins, Quaternary structure organization, Static Electricity, ved/biology.organism_classification_rank.species, Biology, Microbiology, Protein structure, Hyperthermophilic enzyme - Conformational stability - Salt bridge, Thermostability, ved/biology, Circular Dichroism, Sulfolobus solfataricus, Sulfolobaceae, General Medicine, biology.organism_classification, Spectrometry, Fluorescence, Biochemistry, Molecular Medicine, Spectrophotometry, Ultraviolet, Protein quaternary structure, Sulfolobales, Agrobacterium radiobacter

Abstract

Organophosphates (OPs) constitute the largest class of insecticides used worldwide and certain of them are potent nerve agents. Consequently, enzymes degrading organophosphates are of paramount interest, as they could be used as bioscavengers and biodecontaminants. Looking for a stable OPs catalyst, able to support industrial process constraints, a hyperthermophilic phosphotriesterase (known as SsoPox) was isolated from the archaeon Sulfolobus solfataricus and was found to be highly thermostable. The solved 3D structure revealed that SsoPox is a noncovalent dimer, with lactonase activity against “quorum sensing signals”, and therefore could represent also a potential weapon against certain pathogens. The structural basis of the high thermostability of SsoPox has been investigated by performing a careful comparison between its structure and that of two mesophilic phosphotriesterases (PTEs) from P. diminuta and A. radiobacter. In addition, the conformational stability of SsoPox against the denaturing action of temperature and GuHCl has been determined by means of circular dichroism and fluorescence measurements. The data suggest that the two fundamental differences between SsoPox and the mesophilic counterparts are: (a) a larger number of surface salt bridges, also involved in complex networks; (b) a tighter quaternary structure due to an optimization of the interactions at the interface between the two monomers.

Published

2009

11. Reverse gyrase and genome stability in hyperthermophilic organisms

Author

Anna Valenti, Giuseppe Perugino, Anna D'Amaro, Maria Ciaramella, Mosè Rossi, Perugino, Giuseppe, Valenti, Anna, D'Amaro, Anna, Rossi, Mosè, Ciaramella, Maria, Perugino, G., Valenti, A., D'Amaro A, A., Rossi, Mose', and M. C. i. a. r. a. m. e. l. l. a. .

Subjects

Genetics, DNA Repair, Topoisomerase, Linking number, Biology, Archaea, Biochemistry, DNA gyrase, Genomic Instability, Protein Structure, Tertiary, Methyl methanesulfonate, symbols.namesake, chemistry.chemical_compound, DNA Topoisomerases, Type I, Species Specificity, chemistry, symbols, biology.protein, DNA supercoil, A-DNA, Function (biology), DNA

Abstract

Reverse gyrase is a DNA topoisomerase that is peculiar in many aspects: it has the unique ability to introduce positive supercoils into DNA molecules; it comprises a type IA topoisomerase fused to a helicase-like domain; although it is a type IA topoisomerase, its reaction is ATP-dependent; and it is the only hyperthermophile-specific protein. All these features have made reverse gyrase the subject of biochemical, structural and functional studies, although they have not shed complete light on the evolution, mechanism and function of this distinctive enzyme. In the present article, we review the latest progress on structure–function relationships of reverse gyrase, and discuss old and recent data linking reverse gyrase to DNA stability, protection and repair in hyperthermophilic organisms. Abbreviations: dsDNA, double-stranded DNA; EM, electron microscopy; Lk, linking number; MMS, methyl methanesulfonate; SF2, superfamily 2; SSB, single-stranded DNA-binding protein; ssDNA, single-stranded DNA

Published

2009

12. Evidence that the xylanase activity from Sulfolobus solfataricus Oα is encoded by the endoglucanase precursor gene (sso1354) and characterization of the associated cellulase activity

Author

Immacolata Fiume, Marco Moracci, Mosè Rossi, Alessandra Esposito, Alessandra Morana, Alfonso Giovane, Luisa Maurelli, Maurelli, L., Giovane, A., Esposito, A., Moracci, M., Fiume, I., Rossi, Mose', Morana, A., Maurelli, Luisa, Giovane, Alfonso, Esposito, Alessandra, Moracci, Marco, Fiume, Immacolata, and Morana, Alessandra

Subjects

glycoprotein, Archaeal Proteins, Molecular Sequence Data, ved/biology.organism_classification_rank.species, Cellobiose, Cellulase, Xylose, Endo-1,4-beta Xylanase, Microbiology, Mass Spectrometry, Substrate Specificity, Hydrolysis, chemistry.chemical_compound, Peptide Fragment, Archaeal Protein, Glycoside hydrolase, Amino Acid Sequence, Membrane Protein, Conserved Sequence, Kinetic, xylanase, Endo-1,4-beta Xylanases, Sequence Homology, Amino Acid, biology, Chemistry, ved/biology, Sulfolobus solfataricus, Membrane Proteins, General Medicine, Sulfolobus solfataricu, Xylan, Peptide Fragments, Kinetics, Biochemistry, Carboxymethylcellulose Sodium, Chromatography, Gel, biology.protein, Xylanase, Thermodynamics, Molecular Medicine, agricultural waste, Sequence Alignment

Abstract

Sulfolobus solfataricus strain Oalpha was previously isolated for its ability to grow on minimal medium supplemented with xylan as a carbon source. The strain exhibited thermostable xylanase activity but several attempts to identify the gene encoding for the activity failed. Further studies showed that the xylanase displayed activity on carboxymethylcellulose (CMC) and the new activity was characterized. It exhibited an optimal temperature and pH of 95 degrees C and 3.5, respectively, and a half-life of 53 min at 95 degrees C. The enzyme, which was demonstrated to be glycosylated, hydrolyzed CMC in an endo-manner releasing cellobiose and other cello-oligomers. Analysis of the tryptic fragments by tandem mass spectrometry led to identification of the endoglucanase precursor, encoded by the sso1354 gene, as the protein possessing dual activity. The efficiency of the SSO1354 protein in degrading cellulosic and hemicellulosic fractions contained in agronomic residues was tested at low pH and high temperature. Cellulose and xylan were degraded to glucose and xylose at 90 degrees C, pH 4 by an enzyme mix consisting of SSO1354 and additional glycosyl hydrolases from S. solfataricus Oalpha. Given its role in saccharification processes requiring high temperatures and acidic environments, SSO1354 represents an interesting candidate for the utilization of agro-industrial waste for fuel production.

Published

2008

13. Structural analysis of the Sulfolobus solfataricus MCM protein N-terminal domain†

Author

Francesca M. Pisani, Wei Liu, Rudolf Ladenstein, Biagio Pucci, Mosè Rossi, Liu, W., Pucci, B., Rossi, Mose', Pisani, F. M., and Ladenstein, R.

Subjects

Models, Molecular, Methanobacteriaceae, Protein subunit, Archaeal Proteins, ved/biology.organism_classification_rank.species, Molecular Sequence Data, Crystallography, X-Ray, Protein Structure, Secondary, chemistry.chemical_compound, Bacterial Proteins, Structural Biology, Genetics, Amino Acid Sequence, Binding site, Sequence Deletion, Binding Sites, biology, ved/biology, Sulfolobus solfataricus, DNA Helicases, Helicase, biology.organism_classification, MCM Protein, Sulfolobus, Protein Structure, Tertiary, DNA-Binding Proteins, Protein Subunits, Zinc, Biochemistry, chemistry, Structural Homology, Protein, Nucleic acid, biology.protein, Biophysics, DNA

Abstract

The Mini-Chromosome Maintenance (MCM) proteins are candidates of replicative DNA helicase in eukarya and archaea. Here we report a 2.8 A crystal structure of the N-terminal domain (residues 1-268) of the Sulfolobus solfataricus MCM (Sso MCM) protein. The structure reveals single-hexameric ring-like architecture, at variance from the protein of Methanothermobacter thermoautotrophicus (Mth). Moreover, the central channel in Sso MCM seems significantly narrower than the Mth counterpart, which appears to more favorably accommodate single-stranded DNA than double-stranded DNA, as supported by DNA-binding assays. Structural analysis also highlights the essential role played by the zinc-binding domain in the interaction with nucleic acids and allows us to speculate that the Sso MCM N-ter domain may function as a molecular clamp to grasp the single-stranded DNA passing through the central channel. On this basis possible DNA unwinding mechanisms are discussed.

Published

2008

14. A novel DNA helicase with strand-annealing activity from the crenarchaeon Sulfolobus solfataricus

Author

Francesca M. Pisani, Mariarita De Felice, Valentina Aria, Mariarosaria De Falco, Biagio Pucci, Luca Esposito, Mosè Rossi, De Felice, M., Aria, V., Esposito, L., De Falco, M., Pucci, B., Rossi, Mose', and Pisani, F. M.

Subjects

DNA recombination, ved/biology.organism_classification_rank.species, DNA helicase, Biochemistry, Catalysis, Substrate Specificity, law.invention, chemistry.chemical_compound, Adenosine Triphosphate, law, Annealing activity, Molecular Biology, biology, ved/biology, Hydrolysis, Circular bacterial chromosome, Sulfolobus solfataricus, DNA Helicases, DNA replication, Helicase, DNA, Cell Biology, Archaea, DNA-pairing activity, chemistry, biology.protein, Recombinant DNA, Primase, Dimerization, genome stability, Research Article, Protein Binding

Abstract

To protect their genetic material cells adopt different mechanisms linked to DNA replication, recombination and repair. Several proteins function at the interface of these DNA transactions. In the present study, we report on the identification of a novel archaeal DNA helicase. BlastP searches of the Sulfolobus solfataricus genome database allowed us to identify an open reading frame (SSO0112, 875 amino acid residues) having sequence similarity with the human RecQ5β. The corresponding protein, termed Hel112 by us, was produced in Escherichia coli in soluble form, purified to homogeneity and characterized. Gel-filtration chromatography and glycerol-gradient sedimentation analyses revealed that Hel112 forms monomers and dimers in solution. Biochemical characterization of the two oligomeric species revealed that only the monomeric form has an ATP-dependent 3′–5′ DNA-helicase activity, whereas, unexpectedly, both the monomeric and dimeric forms possess DNA strand-annealing capability. The Hel112 monomeric form is able to unwind forked and 3′-tailed DNA structures with high efficiency, whereas it is almost inactive on blunt-ended duplexes and bubble-containing molecules. This analysis reveals that S. solfataricus Hel112 shares some enzymatic features with the RecQ-like DNA helicases and suggests potential cellular functions of this protein.

Published

2007

15. 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

16. Novel thermophilic hemicellulases for the conversion of lignocellulose for second generation biorefineries

Author

Beatrice Cobucci-Ponzano, Mosè Rossi, Giuseppe Masturzo, Rosa Giglio, Roberta Iacono, Andrea Strazzulli, Marco Moracci, Cobucci Ponzano, Beatrice, Strazzulli, Andrea, Iacono, Roberta, Masturzo, Giuseppe, Giglio, Rosa, Rossi, Mose', and Moracci, Marco

Subjects

Bioconversion, CAZy, Hot Temperature, Alicyclobacillus, Glycoside Hydrolases, Thermophilic enzymes, Firmicute, Glycoside Hydrolase, Firmicutes, Bacterial Protein, Bioengineering, Biology, Xylose, Endo-1,4-beta Xylanase, Lignin, Biochemistry, Applied Microbiology and Biotechnology, Substrate Specificity, chemistry.chemical_compound, Bioma, Bacterial Proteins, Biofuel, Glucuronoxylan, Enzyme Stability, Hemicellulose, Glycoside hydrolase, Biomass, Biotransformation, chemistry.chemical_classification, White chemistry, Alicyclobacillu, Endo-1,4-beta Xylanases, Thermophile, Medicine (all), Biocatalysi, Recombinant Protein, biology.organism_classification, Recombinant Proteins, Thermophilic enzyme, chemistry, Genes, Bacterial, Biofuels, Biocatalysis, Xylanase, Caldicellulosiruptor saccharolyticus, Biotechnology

Abstract

The biotransformation of lignocellulose biomasses into fermentable sugars is a very complex procedure including, as one of the most critical steps, the (hemi) cellulose hydrolysis by specific enzymatic cocktails. We explored here, the potential of stable glycoside hydrolases from thermophilic organisms, so far not used in commercial enzymatic preparations, for the conversion of glucuronoxylan, the major hemicellulose of several energy crops. Searches in the genomes of thermophilic bacteria led to the identification, efficient production, and detailed characterization of novel xylanase and a-glucuronidase from Alicyclobacillus acidocaldarius (G1-110-XA and GH67-GA, respectively) and a alpha-glucuronidase from Caldicellulosiruptor saccharolyticus (GH67-GC). Remarkably, GH10-XA, if compared to other thermophilic xylanases from this family, coupled good specificity on beechwood xylan and the best stability at 65 degrees C (3.5 days). In addition, GH67-GC was the most stable alpha-glucuronidases from this family and the first able to hydrolyse both aldouronic acid and aryl-alpha-glucuronic acid substrates. These enzymes, led to the very efficient hydrolysis of beechwood xylan by using 7- to 9-fold less protein (concentrations

Published

2015

17. The human GINS complex binds to and specifically stimulates human DNA polymerase α‐primase

Author

Mariarita De Felice, Mariarosaria De Falco, Francesca M. Pisani, Ulrich Hübscher, Mosè Rossi, Elena Ferrari, De Falco, M, Ferrari, E, De Felice, M, Rossi, Mose', Hubscher, U, and Pisani, F. M.

Subjects

GINS, DNA polymerase, Scientific Report, DNA replication, Biochemistry, genome dynamics, law.invention, chemistry.chemical_compound, ATP Binding Cassette Transporter, Subfamily B, Member 3, law, Escherichia coli, Genetics, Humans, ATP Binding Cassette Transporter, Subfamily B, Member 2, Protein Precursors, Molecular Biology, Polymerase, DNA primase, biology, DNA, Surface Plasmon Resonance, DNA Polymerase I, Molecular biology, Peptide Fragments, Recombinant Proteins, Cell biology, Protein Subunits, chemistry, Recombinant DNA, biology.protein, ATP-Binding Cassette Transporters, Primase, DNA polymerase I

Abstract

The eukaryotic GINS complex has an essential role in the initiation and elongation phases of genome duplication. It is composed of four paralogous subunits--Sld5, Psf1, Psf2 and Psf3--which are ubiquitous and evolutionarily conserved in eukaryotic organisms. Here, we report the biochemical characterization of the human GINS complex (hGINS). The four hGINS subunits were coexpressed in Escherichia coli in a highly soluble form and purified as a complex. hGINS was shown to interact directly with the heterodimeric human DNA primase, by using either surface plasmon resonance measurements or by immunoprecipitation experiments carried out with anti-hGINS antibodies. The DNA polymerase alpha-primase synthetic activity was specifically stimulated by hGINS on various primed DNA templates. The significance of these findings is discussed in view of the molecular dynamics at the human replication fork.

Published

2006

18. A Novel Member of the Protein Disulfide Oxidoreductase Family from Aeropyrum pernix K1: Structure, Function and Electrostatics

Author

Simonetta Bartolucci, Carlo Pedone, Giuseppina De Simone, Emma Langella, Katia D'Ambrosio, Mosè Rossi, Emilia Pedone, K., D'Ambrosio, E., Pedone, E., Langella, D., DE SIMONE, Rossi, Mose', Pedone, Carlo, and Bartolucci, Simonetta

Subjects

Protein family, Static Electricity, Protein Disulfide-Isomerases, Crystallography, X-Ray, Thioredoxin fold, Protein Structure, Secondary, Structure-Activity Relationship, Structural Biology, Oxidoreductase, protein disulfide oxidoreductase, Animals, Insulin, Aeropyrum pernix, Cysteine, Disulfides, Protein disulfide-isomerase, Molecular Biology, chemistry.chemical_classification, Binding Sites, biology, Chemistry, Protein Disulfide Reductase (Glutathione), Aeropyrum, Hydrogen-Ion Concentration, biology.organism_classification, Biochemistry, Cattle, Protein folding, Thioredoxin, Oxidation-Reduction, thioredoxin fold

Abstract

The formation of disulfide bonds between cysteine residues is a rate-limiting step in protein folding. To control this oxidative process, different organisms have developed different systems. In bacteria, disulfide bond formation is assisted by the Dsb protein family; in eukarya, disulfide bond formation and rearrangement are catalyzed by PDI. In thermophilic organisms, a potential key role in disulfide bond formation has recently been ascribed to a new cytosolic Protein Disulphide Oxidoreductase family whose members have a molecular mass of about 26 kDa and are characterized by two thioredoxin folds comprising a CXXC active site motif each. Here we report on the functional and structural characterization of ApPDO, a new member of this family, which was isolated from the archaeon Aeropyrum pernix K1. Functional studies have revealed that ApPDO can catalyze the reduction, oxidation and isomerization of disulfide bridges. Structural studies have shown that this protein has two CXXC active sites with fairly similar geometrical parameters typical of a stable conformation. Finally, a theoretical calculation of the cysteine pKa values has suggested that the two active sites have similar functional properties and each of them can impart activity to the enzyme. Our results are evidence of functional similarity between the members of the Protein Disulphide Oxidoreductase family and the eukaryotic enzyme PDI. However, as the different three-dimensional features of these two biological systems strongly suggest significantly different mechanisms of action, further experimental studies will be needed to make clear how different three-dimensional structures can result in systems with similar functional behavior.

Published

2006

19. Identification and Characterization of a Novel Bacterial Sulfite Oxidase with No Heme Binding Domain from Deinococcus radiodurans

Author

Giovanni D’Errico, Francesco La Cara, Anna Di Salle, Raffaele Cannio, Mosè Rossi, D'Errico, G, DI SALLE, A, LA CARA, F, Rossi, Mose', and Cannio, R.

Subjects

Models, Molecular, Heme binding, Molecular Sequence Data, Heme, medicine.disease_cause, Microbiology, Gene product, Open Reading Frames, chemistry.chemical_compound, Bacterial Proteins, Sulfite oxidase, medicine, Deinococcus, Amino Acid Sequence, Molecular Biology, Escherichia coli, Peptide sequence, Gene, biology, Sulfite Oxidase, Deinococcus radiodurans, Chromosomes, Bacterial, biology.organism_classification, Enzymes and Proteins, Molecular biology, Recombinant Proteins, chemistry, Genes, Bacterial, bacteria, Sequence Alignment

Abstract

An open reading frame ( draSO ) encoding a putative sulfite oxidase (SO) was identified in the sequence of chromosome II of Deinococcus radiodurans ; the predicted gene product showed significant amino acid sequence homology to several bacterial and eukaryotic SOs, such as the biochemically and structurally characterized enzyme from Arabidopsis thaliana . Cloning of the Deinococcus SO gene was performed by PCR amplification from the bacterial genomic DNA, and heterologous gene expression of a histidine-tagged polypeptide was obtained in a molybdopterin-overproducing strain of Escherichia coli . The recombinant protein was purified to homogeneity by nickel chelating affinity chromatography, and its main kinetic and chemical physical parameters were determined. Northern blot and enzyme activity analyses indicated that draSO gene expression is constitutive in D. radiodurans and that there is no increase upon exposure to thiosulfate and/or molybdenum(II).

Published

2006

20. Reversion of protein aggregation mediated by Sso7d in cell extracts of Sulfolobus solfataricus

Author

Mosè Rossi, Annamaria Guagliardi, Lucia Mancusi, Guagliardi, Annamaria, A., Mancusi, and Rossi, Mose'

Subjects

Hot Temperature, Archaeal Proteins, ved/biology.organism_classification_rank.species, Protein aggregation, medicine.disease_cause, Biochemistry, DNA-binding protein, Sulfolobus, chemistry.chemical_compound, Adenosine Triphosphate, ATP hydrolysis, medicine, Molecular Biology, Escherichia coli, biology, ved/biology, Hydrolysis, Sulfolobus solfataricus, Cell Biology, biology.organism_classification, DNA-Binding Proteins, Enzyme Activation, Solubility, chemistry, Chaperone (protein), biology.protein, Adenosine triphosphate, Glucosidases, Research Article, Molecular Chaperones

Abstract

In eukaryotic cells and in Escherichia coli, reversion of protein aggregation is mediated by the network of chaperones belonging to Hsp70 and Hsp100 families [Weibezahn, Bukau and Mogk (2004) Microb. Cell Fact. 3, 1–12]. The thermophilic prokaryotes of the archaea domain lack homologues of these chaperone families, and the mechanisms they use to rescue aggregated proteins are unknown [Macario, Malz and Conway de Macario (2004) Front. Biosci. 9, 1318–1332]. In the present study, we show that stable protein aggregates can be detected in extracts of starved cells of the thermophilic archaeon Sulfolobus solfataricus, and that the protein Sso7d interacts with the aggregates and mediates the disassembly of the aggregates and the re-activation of insolubilized β-glycosidase in the presence of ATP hydrolysis. Furthermore, we report that heat-induced protein aggregates in extracts of exponential cells of S. solfataricus contain Sso7d that rescues insolubilized proteins in the presence of ATP hydrolysis. Results of these experiments performed in cell extracts are consistent with an in vivo role of Sso7d in reverting protein aggregation.

Published

2004

21. Identification of a GDP-mannose pyrophosphorylase gene from Sulfolobus solfataricus

Author

Simonetta Bartolucci, Silvana Sacchetti, Raffaele Cannio, Mosè Rossi, Sacchetti, Silvana, Bartolucci, Simonetta, Rossi, Mose', and Cannio, R.

Subjects

Guanosine Diphosphate Mannose, Sequence analysis, Recombinant Fusion Proteins, Molecular Sequence Data, ved/biology.organism_classification_rank.species, Saccharomyces cerevisiae, RNA, Archaeal, Biology, medicine.disease_cause, Catalysis, Gene Expression Regulation, Enzymologic, Substrate Specificity, Sulfolobus, Mannose metabolism, Affinity chromatography, Genetics, medicine, GDP-mannose pyrophosphorylase, Amino Acid Sequence, Escherichia coli, Peptide sequence, Glutathione Transferase, Mannosephosphates, Base Sequence, Sequence Homology, Amino Acid, ved/biology, Sulfolobus solfataricus, Sequence Analysis, DNA, General Medicine, biology.organism_classification, Nucleotidyltransferases, Molecular biology, Open reading frame, DNA, Archaeal, Biochemistry, Electrophoresis, Polyacrylamide Gel, Guanosine Triphosphate, Gene Expression Regulation, Archaeal

Abstract

An open reading frame (ORF) encoding a putative GDP-mannose pyrophosphorylase (SsoGMPP) was identified on the genome sequence of Sulfolobus solfataricus P2, the predicted gene product showing high amino acid sequence homology to several archaeal, bacterial, and eukaryal GDP-mannose pyrophosphorylases such as guanidine diphosphomannose pyrophosphorylases (GMPPs) from Saccharomyces cerevisiae and Arabidopsis thaliana. The sequence was PCR amplified from genomic DNA of S. solfataricus P2 and heterologous gene expression obtained as a fusion to glutathione S-transferase in Escherichia coli, under conditions suitable to reduce the formation of inclusion bodies. Specific assays performed at 60 degrees C revealed the presence of the archaeal synthesizing GDP-mannose enzyme activity in the cell extracts of the transformed E. coli. As a positive control, the same assays were performed at the mesophilic enzyme optimum temperature on the already characterized yeast recombinant GMPP. The recombinant protein was purified to homogeneity by glutathione sepharose affinity chromatography and its thermophilic nature could be verified. The enzyme was definitively identified by demonstrating its capability to catalyze also the reverse reaction of pyrophosphorolysis and, most interestingly, its high specificity for synthesizing GDP-mannose.

Published

2004

22. Applications in Biocatalysis of Glycosyl Hydrolases from the Hyperthermophilic ArchaeonSulfolobus solfataricus

Author

Barbara Di Lauro, Marco Moracci, Assunta Giordano, Giuseppe Perugino, Mosè Rossi, Beatrice Cobucci-Ponzano, Antonio Trincone, Marialuisa Mazzone, Cobucci Ponzano, Beatrice, Perugino, Giuseppe, Trincone, Antonio, Mazzone, Marialuisa, DI LAURO, Barbara, Giordano, Assunta, Rossi, Mose', and Moracci, Marco

Subjects

chemistry.chemical_classification, biology, Chemistry, ved/biology, Sulfolobus solfataricus, ved/biology.organism_classification_rank.species, Sulfolobaceae, Glycosynthase, Oligosaccharide, biology.organism_classification, Biochemistry, Catalysis, Molecular recognition, Biocatalysis, Glycoside hydrolase, Energy source, Biotechnology

Abstract

Carbohydrates serve as structural components and en- ergy sources of cells. More interestingly, however, these biomolecules are involved in a variety of molecular recognition processes in intercellular communication and signal transduction such as cell adhesion, differ- entiation, development and regulation. For these rea- sons, great interest has arisen in carbohydrate-based pharmaceuticals and on the development of techniques for the analysis and synthesis of oligosaccharides. In this respect, enzymes involved in carbohydrates hydrolysis and modification are increasingly being utilised for the bioconversion of sugars, for the synthesis of oligosac- charides with potential application, and for the charac- terisation of carbohydrate compounds of unknown structure. In this review, the enzymology and the applications of three glycosyl hydrolases from the archaeon Sulfolobus solfataricus are described. In particular, we focus on the enzymological properties of a b-glycosidase, an a-xylo- sidase, and an a-fucosidase; their exploitation in oligo- saccharides synthesis will be also described.

Published

2003

23. Transcriptional Regulation of the Gene Encoding an Alcohol Dehydrogenase in the Archaeon Sulfolobus solfataricus Involves Multiple Factors and Control Elements

Author

Simonetta Bartolucci, Mosè Rossi, Raffaele Cannio, Gabriella Fiorentino, Fiorentino, G, Cannio, R, Rossi, Mose', Bartolucci, Simonetta, Fiorentino, Gabriella, R., Cannio, and M., Rossi

Subjects

Transcriptional Activation, Transcription, Genetic, 5' Flanking Region, Archaeal Proteins, TATA box, Molecular Sequence Data, ved/biology.organism_classification_rank.species, 5' flanking region, DNA Footprinting, Biology, Microbiology, Sulfolobus, Transcriptional regulation, Promoter Regions, Genetic, Molecular Biology, Transcription factor, Gene, Regulation of gene expression, Base Sequence, ved/biology, Sulfolobus solfataricus, Alcohol Dehydrogenase, Meeting Presentations, Promoter, TATA Box, DNA binding protein, Culture Media, DNA-Binding Proteins, DNA, Archaeal, Biochemistry, Benzaldehydes, Gene Expression Regulation, Archaeal, Transcription Factors

Abstract

A transcriptionally active region has been identified in the 5′ flanking region of the alcohol dehydrogenase gene of the crenarchaeon Sulfolobus solfataricus through the evaluation of the activity of putative transcriptional regulators and the role of the region upstream of the gene under specific metabolic circumstances. Electrophoretic mobility shift assays with crude extracts revealed protein complexes that most likely contain TATA box-associated factors. When the TATA element was deleted from the region, binding sites for both DNA binding proteins, such as the small chromatin structure-modeling Sso7d and Sso10b (Alba), and transcription factors, such as the repressor Lrs14, were revealed. To understand the molecular mechanisms underlying the substrate-induced expression of the adh gene, the promoter was analyzed for the presence of cis -acting elements recognized by specific transcription factors upon exposure of the cell to benzaldehyde. Progressive dissection of the identified promoter region restricted the analysis to a minimal responsive element (PAL) located immediately upstream of the transcription factor B-responsive element-TATA element, resembling typical bacterial regulatory sequences. A benzaldehyde-activated transcription factor (Bald) that specifically binds to the PAL cis -acting element was also identified. This protein was purified from heparin-fractionated extracts of benzaldehyde-induced cells and was shown to have a molecular mass of ∼16 kDa. The correlation between S. solfataricus adh gene activation and benzaldehyde-inducible occupation of a specific DNA sequence in its promoter suggests that a molecular signaling mechanism is responsible for the switch of the aromatic aldehyde metabolism as a response to environmental changes.

Published

2003

24. Modification of the enantioselectivity of two homologous thermophilic carboxylesterases from Alicyclobacillus acidocaldarius and Archaeoglobus fulgidus by random mutagenesis and screening

Author

Gianluca Ottolina, Mosè Rossi, Giuseppe Manco, Giovanna Adamo, Elena Giosuè, Giacomo Carrea, Manco, G., Carrea, G., Giosue, E., Ottolina, G., Adamo, G., and Rossi, Mose'

Subjects

Models, Molecular, Mutant, Bacillus, Polymerase Chain Reaction, Microbiology, Esterase, Substrate Specificity, DNA Primers, chemistry.chemical_classification, Base Sequence, biology, Thermophile, Mutagenesis, Archaeoglobus fulgidus, Active site, Substrate (chemistry), Stereoisomerism, General Medicine, Enzyme, Biochemistry, chemistry, biology.protein, Molecular Medicine, Carboxylic Ester Hydrolases

Abstract

The esterase genes est2 from Alicyclobacillus acidocaldarius and AF1716 from Archaeoglobus fulgidus were subjected to error-prone PCR in an effort to increase the low enantioselectivity of the corresponding enzymes EST2 and AFEST, respectively. The model substrate ( RS)- p-nitrophenyl-2-chloropropionate was chosen to produce ( S)-2-chloropropionic acid, an important intermediate in the synthesis of some optically pure compounds, such as the herbicide mecoprop. In the case of EST2, a single mutant, Leu212Pro, was obtained showing a slightly enhanced preference toward the ( S) substrate; in the case of AFEST, a double mutant, Leu101Ile/Asp117Gly, was obtained showing an increased preference in the opposite direction. The 3-D structures of the EST2 and AFEST enzymes were analyzed by molecular modeling to determine the effects of the mutations. Mutations were positioned differently in the structures, but in both cases caused small modifications around the active site and in the oxyanion loop.

Published

2002

25. A low-resolution 3D model of the tetrameric alcohol dehydrogenase from Sulfolobus solfataricus

Author

Pier Luigi Martelli, Rita Casadio, Carlo A. Raia, Mosè Rossi, Antonietta Giordano, Casadio, R., Martelli, P. L., Giordano, A., Rossi, Mose', and Raia, C. A.

Subjects

Models, Molecular, Molecular Sequence Data, ved/biology.organism_classification_rank.species, Bioengineering, Biochemistry, Sulfolobus, Ion, chemistry.chemical_compound, Residue (chemistry), Amino Acid Sequence, Protein Structure, Quaternary, Molecular Biology, Zinc ion binding, Alcohol dehydrogenase, Binding Sites, biology, ved/biology, Chemistry, Thermophile, Sulfolobus solfataricus, Alcohol Dehydrogenase, NAD, Zinc, Crystallography, Cross-Linking Reagents, Monomer, biology.protein, Threading (protein sequence), Sequence Alignment, Biotechnology

Abstract

We describe the computation of a model of the thermophilic NAD-dependent homotetrameric alcohol dehydrogenase from the archaeon Sulfolobus solfataricus (SsADH). Modeling is based on the knowledge that each monomer contains two Zn ions with catalytic and structural function, respectively. In the database of known structures, proteins with similar functions are either dimers containing two zinc ions per monomer or tetramers with one zinc ion per monomer. In any case, the sequence identity of the target to the possible templates is low. A threading procedure is therefore developed which includes constraints taking into account residue conservation both at the zinc ion binding and at the monomer-monomer interaction sites in the tetrameric unit. The model is consistent with previously reported data. Furthermore, cross-linking experiments are described which support the computed tetrameric model.

Published

2002

26. The identification and molecular characterization of the first archaeal bifunctional exo-beta-glucosidase/N-acetyl-beta-glucosaminidase demonstrate that family GH116 is made of three functionally distinct subfamilies

Author

Ferrara M.C., Cobucci-Ponzano B., Carpentieri A., Henrissat, Rossi M., Amoresano A., Moracci M., Ferrara, Mc, Cobucci Ponzano, B, Carpentieri, Andrea, Henrissat, B, Rossi, Mose', Amoresano, Angela, and Moracci, Marco

Subjects

Glycan, CAZy, Molecular Sequence Data, ved/biology.organism_classification_rank.species, Biophysics, Biochemistry, Substrate Specificity, Tandem Mass Spectrometry, Crenarchaeota, Catalytic Domain, Amino Acid Sequence, Cloning, Molecular, Molecular Biology, Phylogeny, chemistry.chemical_classification, Sequence Homology, Amino Acid, biology, Chemistry, Glycobiology, ved/biology, Thermophile, Sulfolobus solfataricus, biology.organism_classification, Recombinant Proteins, beta-N-Acetylhexosaminidases, Sulfolobus, Enzyme, Multigene Family, biology.protein, Chromatography, Liquid

Abstract

Background ?-N-acetylhexosaminidases, which are involved in a variety of biological processes including energy metabolism, cell proliferation, signal transduction and in pathogen-related inflammation and autoimmune diseases, are widely distributed in Bacteria and Eukaryotes, but only few examples have been found in Archaea so far. However, N-acetylgluco- and galactosamine are commonly found in the extracellular storage polymers and in the glycans decorating abundantly expressed glycoproteins from different Crenarchaeota Sulfolobus sp., suggesting that ?-N-acetylglucosaminidase activities could be involved in the modification/recycling of these cellular components. Methods A thermophilic ?-N-acetylglucosaminidase was purified from cellular extracts of S. solfataricus, strain P2, identified by mass spectrometry, and cloned and expressed in E. coli. Glycosidase assays on different strains of S. solfataricus, steady state kinetic constants, substrate specificity analysis, and the sensitivity to two inhibitors of the recombinant enzyme were also reported. Results A new ?-N-acetylglucosaminidase from S. solfataricus was unequivocally identified as the product of gene sso3039. The detailed enzymatic characterization demonstrates that this enzyme is a bifunctional ?-glucosidase/?-N-acetylglucosaminidase belonging to family GH116 of the carbohydrate active enzyme (CAZy) classification. Conclusions This study allowed us to propose that family GH116 is composed of three subfamilies, which show distinct substrate specificities and inhibitor sensitivities. General significance The characterization of SSO3039 allows, for the first time in Archaea, the identification of an enzyme involved in the metabolism ?-N-acetylhexosaminide, an essential component of glycoproteins in this domain of life, and substantially increases our knowledge on the functional role and phylogenetic relationships amongst the GH116 CAZy family members. © 2013 Elsevier B.V. All rights reserved.

Published

2014

27. Identification and molecular characterization of an endoglucanase gene, celS , from the extremely thermophilic archaeon Sulfolobus solfataricus

Author

Danila Limauro, Simonetta Bartolucci, Mosè Rossi, Gabriella Fiorentino, Raffaele Cannio, Limauro, Danila, Cannio, R., Fiorentino, Gabriella, Rossi, Mose', and Bartolucci, Simonetta

Subjects

Molecular Sequence Data, ved/biology.organism_classification_rank.species, Biology, Microbiology, Genes, Archaeal, Sulfolobus, Gene product, Cellulase, Amino Acid Sequence, Cloning, Molecular, Gene, ved/biology, Sulfolobus solfataricus, Temperature, Glycosyl hydrolase, General Medicine, Sulfolobus solfataricu, biology.organism_classification, Molecular biology, Open reading frame, Biochemistry, Thermotoga maritima, Pyrococcus furiosus, Molecular Medicine, Sequence Alignment, Sequence Analysis, Thermotoga neapolitana

Abstract

A genomic region upstream of the alcohol dehydrogenase ( Ssadh ) gene was cloned and sequenced from a library of Sulfolobus solfataricus MT4 strain. The isolated 4,040-bp DNA fragment revealed an open reading frame ( celS ), lying in the opposite direction to Ssadh , which showed significant similarity to endo - β -1,4-glucanases from Pyrococcus furiosus , Thermotoga maritima , and Thermotoga neapolitana . celS was shown to be a functional gene in vivo: a specific celS mRNA was detected by primer extension analysis showing a unique initiation transcription site coinciding with the ATG translation initiation codon. The specific gene product was detected as an extracellular cellulase after enzyme staining by carboxymethyl cellulose (CMC) SDS-PAGE, showing a molecular weight in agreement with that deduced from the open reading frame. Depending on growth conditions, different levels of cellulase activity and specific celS transcript were detected, revealing an inductive effect of CMC and suggesting a repressive role of glucose.

Published

2001

28. Thermoadaptation of a mesophilic hygromycin B phosphotransferase by directed evolution in hyperthermophilic Archaea: selection of a stable genetic marker for DNA transfer into Sulfolobus solfataricus

Author

Patrizia Contursi, Simonetta Bartolucci, Raffaele Cannio, Mosè Rossi, R., Cannio, Contursi, Patrizia, Rossi, Mose', and Bartolucci, Simonetta

Subjects

Genetic Markers, ved/biology.organism_classification_rank.species, Adaptation, Biological, Gene Expression, Genetica manipolativa, "genetic marker", Biology, medicine.disease_cause, Microbiology, Sulfolobus, chemistry.chemical_compound, Transformation, Genetic, Cotransformation, Extrachromosomal DNA, Escherichia coli, medicine, Termoadattamento, "shuttle vector", Trasformazione, Gene, Sulfolobus shibatae, Base Sequence, Sistemi genetici, ved/biology, Sulfolobus solfataricus, Temperature, General Medicine, Directed evolution, Molecular biology, "thermostability", Phosphotransferases (Alcohol Group Acceptor), chemistry, Genes, Bacterial, Mutation, Fuselloviridae, "Hygromycin B phosphotransferase", "thermophilicity", Molecular Medicine, Directed Molecular Evolution, "gene expression", Hygromycin B, Plasmids

Abstract

A mutated version of the hygromycin B phosphotransferase (hph mut ) gene from Escherichia coli, isolated by directed evolution at 75°C in transformants of a thermophilic strain of Sulfolobus solfataricus, was characterized with respect to its genetic stability in both the original mesophilic and the new thermophilic hosts. This gene was demonstrated to be able to express the hygromycin B resistance phenotype and to be steadily maintained and propagated also in other, more thermophilic strains of S. solfataricus, i.e., up to 82°C. Furthermore, it may be transferred to S. solfataricus cells by cotransformation with pKMSD48, another extrachromosomal element derived from the virus SSV1 of Sulfolobus shibatae, without any loss of stability and without affecting the replication and infectivity of this viral DNA. The hph mut and the wild-type gene products were expressed at higher levels in E. coli and purified by specific affinity chromatography on immobilized hygromycin B. Comparative characterization revealed that the mutant enzyme had acquired significant thermoresistance and displayed higher thermal activity with augmented catalytic efficiency.

Published

2001

29. Thermophilic glycosynthases for oligosaccharides synthesis

Author

Mosè Rossi, Andrea Strazzulli, Beatrice Cobucci-Ponzano, Giuseppe Perugino, Marco Moracci, Cobucci Ponzano, Beatrice, Perugino, Giuseppe, Strazzulli, Andrea, Rossi, Mose', Moracci, Marco, Cobucci-Ponzano, Beatrice, and Rossi, Mosè

Subjects

chemistry.chemical_classification, Glycosylation, Hot Temperature, biology, Glycobiology, Glycoconjugate, Thermophile, beta-Glucosidase, Glycoside Hydrolase, Regioselectivity, Enzyme Assay, Oligosaccharide, Sulfolobus solfataricu, Mutagenesi, chemistry, Biochemistry, Glycosyltransferase, Mutation, biology.protein, Stereoselectivity, Glycoside hydrolase, Thermotoga maritima, Cloning, Molecular

Abstract

Glycosynthases are engineered glycoside hydrolases that in suitable reaction conditions promote the synthesis of oligosaccharides with exquisite stereoselectivity and enhanced regioselectivity, if compared to traditional chemical methods. This approach was demonstrated to be successful in a number of cases including β-glycosynthases acting at the termini or within an oligosaccharide chain ( exo - and endo -glycosynthases, respectively) and, more recently, α-glycosynthases. This led to the production of a vast repertoire of products that include poly- and oligosaccharides, glycoconjugates, and glycopeptides. These molecules can be used as ligands of glycoside hydrolases, for the characterization of therapeutic enzymes, and as leads of drugs for the pharmaceutical industry. In this panorama, hyperthermophilic organisms, which thrive at temperatures as high as 80 °C, which usually impede the growth of other living forms, have been used in the development of interesting novel glycosynthases. In fact, the extreme stability of these catalysts to extremes of pH and high concentrations of organics has allowed the exploration of novel reaction conditions, revealing new avenues for enzyme-catalyzed oligosaccharide synthesis.

Published

2012

30. Gene cloning andprotein expression of ?-glutamyltranspeptidases from Thermus thermophilus and Deinococcus radiodurans: comparison of molecular and structural properties withmesophilic counterparts

Author

Mosè Rossi, Francesco La Cara, Immacolata Castellano, Antonello Merlino, Anna Di Salle, Castellano, I., Di Salle, A., Merlino, Antonello, Rossi, Mose', and La Cara, F.

Subjects

Molecular adaptation, Protein family, Protein Conformation, Glutamine, Molecular Sequence Data, Molecular cloning, Microbiology, Thermus thermophilu, Protein structure, Deinococcus radiodurans, Extremophile, Hydrolase, Extreme environment, Amino Acid Sequence, Cloning, Molecular, Peptide sequence, Phylogeny, biology, Sequence Homology, Amino Acid, Hydrolysis, Thermus thermophilus, Temperature, General Medicine, gamma-Glutamyltransferase, Hydrogen-Ion Concentration, biology.organism_classification, Glutathione, Recombinant Proteins, Protein Structure, Tertiary, Gamma-glutamyltranspeptidase, Biochemistry, Molecular Medicine, Deinococcus, Plasmids

Abstract

Gamma-Glutamyltranspeptidase (³-GT) is an ubiquitous enzyme that catalyzes the hydrolysis of ³-glutamyl bonds in glutathione and glutamine and the transfer of the released ³-glutamyl group to amino acids or short peptides. ³-GTs from extremophiles, bacteria adapted to live in hostile environments, were selected as model systems to study the molecular underpinnings of their adaptation to extreme conditions and to find out special properties of potential biotechnological interest. Here, we report the cloning, expression and purification of two members of ³-GT family from two different extremophilic species, Thermus thermophilus (TtGT) and Deinococcus radiodurans (DrGT); the first is an aerobic eubacterium, growing at high temperatures (50-82°C), the second is a polyextremophile, as it tolerates radiations, cold, dehydration, vacuum, and acid. TtGT and DrGT were both synthesized as precursor proteins of 59-60 kDa, undergoing an intramolecular auto-cleavage to yield two subunits of 40 and 19-20 kDa, respectively. However, like the ³-GT from Geobacillus thermodenitrificans, but differently from the other characterized bacterial and eukaryotic ³-GTs, the two new extremophilic enzymes displayed ³-glutamyl hydrolase, but not transpeptidase activity in the 37-50°C temperature range, pH 8.0. The comparison of sequences and structural models of these two proteins with experimental-determined structures of other known mesophilic ³-GTs suggests that the extremophilic members of this protein family have found a common strategy to adapt to different hostile environments. Moreover, a phylogenetic analysis suggests that ³-GTs displaying only ³-glutamyl hydrolase activity could represent the progenitors of the bacterial and eukaryotic counterparts.

Published

2011

31. Functional characterization and high-throughput proteomic analysis of interrupted genes in the archaeon Sulfolobus solfataricus

Author

Dario Benelli, Diem Tran, Emmanuel Perrodou, Lucia Guzzini, Eric J. Mathur, Jun Sun, Odile Lecompte, Beatrice Cobucci-Ponzano, Jing Wei, Mosè Rossi, Marco Moracci, Paola Londei, Laboratoire des sciences de l'ingénieur, de l'informatique et de l'imagerie (ICube), École Nationale du Génie de l'Eau et de l'Environnement de Strasbourg (ENGEES)-Université de Strasbourg (UNISTRA)-Institut National des Sciences Appliquées - Strasbourg (INSA Strasbourg), Institut National des Sciences Appliquées (INSA)-Institut National des Sciences Appliquées (INSA)-Institut National de Recherche en Informatique et en Automatique (Inria)-Les Hôpitaux Universitaires de Strasbourg (HUS)-Centre National de la Recherche Scientifique (CNRS)-Matériaux et Nanosciences Grand-Est (MNGE), Université de Strasbourg (UNISTRA)-Université de Haute-Alsace (UHA) Mulhouse - Colmar (Université de Haute-Alsace (UHA))-Institut National de la Santé et de la Recherche Médicale (INSERM)-Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS)-Université de Strasbourg (UNISTRA)-Université de Haute-Alsace (UHA) Mulhouse - Colmar (Université de Haute-Alsace (UHA))-Institut National de la Santé et de la Recherche Médicale (INSERM)-Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS)-Réseau nanophotonique et optique, Université de Strasbourg (UNISTRA)-Université de Haute-Alsace (UHA) Mulhouse - Colmar (Université de Haute-Alsace (UHA))-Centre National de la Recherche Scientifique (CNRS)-Université de Strasbourg (UNISTRA)-Centre National de la Recherche Scientifique (CNRS), Cobucci Ponzano, Beatrice, Guzzini, Lucia, Benelli, Dario, Londei, Paola, Perrodou, Emmanuel, Lecompte, Odile, Tran, Diem, Sun, Jun, Wei, Jing, Mathur, Eric J, Rossi, Mose', and Moracci, Marco

Subjects

High-Throughput Screening Assay, Proteomics, Proteome, Pseudogene, Archaeal Proteins, ved/biology.organism_classification_rank.species, Molecular Sequence Data, Programmed frameshifting, Biology, Biochemistry, Genome, Peptide Mapping, Genes, Archaeal, Tandem Mass Spectrometry, Archaeal Protein, Gene expression, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, Amino Acid Sequence, Gene, Genetics, Base Sequence, ved/biology, Reverse Transcriptase Polymerase Chain Reaction, Sulfolobus solfataricus, Proteomic, gene expression, kae1/bud32, programmed frameshifting, pseudogenes, sui-1, translational recoding, General Chemistry, Sulfolobus solfataricu, High-Throughput Screening Assays, Transketolase, Pseudogenes, Chromatography, Liquid

Abstract

Sequenced genomes often reveal interrupted coding sequences that complicate the annotation process and the subsequent functional characterization of the genes. In the past, interrupted genes were generally considered to be the result of sequencing errors or pseudogenes, that is, gene remnants with little or no biological importance. However, recent lines of evidence support the hypothesis that these coding sequences can be functional; thus, it is crucial to understand whether interrupted genes are expressed in vivo. We addressed this issue by experimentally demonstrating the existence of functional disrupted genes in archaeal genomes. We discovered previously unknown disrupted genes that have interrupted homologues in distantly related species of archaea. The combination of a RT-PCR strategy with shotgun proteomics demonstrates that interrupted genes in the archaeon Sulfolobus solfataricus are expressed in vivo. In addition, the sequence of the peptides determined by LCMSMS and experiments of in vitro translation allows us to identify a gene expressed by programmed -1 frameshifting. Our findings will enable an accurate reinterpretation of archaeal interrupted genes shedding light on their function and on archaeal genome evolution.

Published

2010

32. Biochemical and structural properties of gamma-glutamyl transpeptidase from Geobacillus thermodenitrificans: an enzyme specialized in hydrolase activity

Author

Francesco La Cara, Immacolata Castellano, Mosè Rossi, Antonello Merlino, Castellano, I, Merlino, Antonello, Rossi, Mose', and La Cara, F.

Subjects

N-terminal nucleophile hydrolase, Thermophilic enzymes, Protein subunit, Molecular Sequence Data, glutamyltranspeptidase, Biochemistry, chemistry.chemical_compound, Geobacillus thermodenitrifican, Geobacillus thermoglucosidasius, Enzyme Stability, Hydrolase, Amino Acid Sequence, DNA Primers, Thermostability, chemistry.chemical_classification, Base Sequence, Sequence Homology, Amino Acid, biology, Hydrolysis, Temperature, Geobacillus, gamma-Glutamyl Hydrolase, gamma-Glutamyltransferase, General Medicine, Glutathione, Hydrogen-Ion Concentration, biology.organism_classification, Heterotetramer, Thermophilic enzyme, Amino acid, Molecular Weight, Gamma-glutamyltranspeptidase, Kinetics, Geobacillus thermodenitrificans, Enzyme, chemistry, Biocatalysis, Mutagenesis, Site-Directed, Electrophoresis, Polyacrylamide Gel

Abstract

Gamma-glutamyltranspeptidases (gamma-GTs) catalyze the transfer of the gamma-glutamyl moiety of glutathione and related gamma-glutamyl amides to water (hydrolysis) or to amino acids and peptides (transpeptidation) and play a key role in glutathione metabolism. Recently, gamma-GTs have been considered attractive pharmaceutical targets for cancer and useful tools to produce gamma-glutamyl compounds. To find out gamma-GTs with special properties we have chosen microorganisms belonging to Geobacillus species which are source of several thermostable enzymes of potential interest for biotechnology. gamma-GT from Geobacillus thermodenitrificans (GthGT) was cloned, expressed in Escherichia coli, purified to homogeneity and characterized. The enzyme, synthesized as a precursor homotetrameric protein of 61-kDa per subunit, undergoes an internal post-translational cleavage of the 61 kDa monomer into 40- and 21-kDa shorter subunits, which are then assembled into an active heterotetramer composed of two 40- and two 21-kDa subunits. The kinetic characterization of the hydrolysis reaction using L-glutamic acid gamma-(4-nitroanilide) as the substrate reveals that the active enzyme has K(m) 7.6 microM and V(max) 0.36 micromol min/mg. The optimum pH and temperature for the hydrolysis activity are 7.8 and 52 degrees C, respectively. GthGT hydrolyses the physiological antioxidant glutathione, suggesting an involvement of the enzyme in the cellular defense mechanism against oxidative stress. Unlike other gamma-GTs, the mutation of the highly conserved catalytic nucleophile, Thr353, abolishes the post-translational cleavage of the pro-enzyme, but does not completely block the hydrolytic action. Furthermore, GthGT does not show any transpeptidase activity, suggesting that the enzyme is a specialized gamma-glutamyl hydrolase. The GthGT homology-model structure reveals peculiar structural features, which should be responsible for the different functional properties of the enzyme and suggests the structural bases of protein thermostability.

Published

2010

33. First Archaeal PEPB-Serine Protease Inhibitor from Sulfolobus Solfataricus with Non-Canonical Amino Acid Sequence in the Reactive-Site Loop

Author

Mosè Rossi, Michele Saviano, Giuliana Catara, Marta Gogliettino, Gianna Palmieri, Emma Langella, Palmieri, G, Catara, G, Saviano, M, Langella, E, Gogliettino, M, and Rossi, Mose'

Subjects

Proteomics, ved/biology.organism_classification_rank.species, Molecular Sequence Data, Molecular Conformation, Phosphatidylethanolamine Binding Protein, Biology, Biochemistry, Mass Spectrometry, Serine proteinases, Basic research, Catalytic Domain, Escherichia coli, Chymotrypsin, Homology modeling, Amino Acid Sequence, Peptide sequence, Reactive site, Serine protease, Serine protease inhibitor, Sequence Homology, Amino Acid, ved/biology, Kazal-type serine protease inhibitor domain, Sulfolobus solfataricus, Serine Endopeptidases, General Chemistry, Archaea, Kinetics, protease binding site, protease inhibitor family, biology.protein, PEBP

Abstract

The specific inhibition of serine proteinases, which are crucial switches in many important physiological processes, is of great value both for basic research and for therapeutic applications. In this study, we report the molecular cloning of the sso0767 gene from Sulfolobus solfataricus, and the functional characterization of its product, SsCEI, which represents the first archaeal phosphatidylethanolamine-binding protein (PEBP)-serine proteinase inhibitor, reported to date. SsCEI is a monomer protein with a molecular mass of 19.0 kDa and a pI of 6.7, which is able to inhibit the serine proteases alpha-chymotrypsin and elastase with K(i) values of 0.08 and 0.1 microM, respectively. Moreover SsCEI is extremely resistant to both thermal inactivation and proteolytic attack suggesting compact folding of the protein. Within the I51 family, the archaeal inhibitor shows strong similarity to the human and murine members. The three-dimensional model of SsCEI revealed a general beta-fold and the presence of an anion-binding pocket, the hallmark of the PEBP family. Moreover SsCEI binds the cognate proteases according to a common, substrate-like standard mechanism. Point mutation experiments supported the prediction of the protease-binding site located on the surface at the C- terminal region of the protein. Interestingly, searches based on preidentified structural reactive loop motifs revealed the occurrence of a sequence (T123-N130) that is not represented in all serine-protease inhibitor families. This unique motif may provide new insights into both the inhibitor/protease binding mode and the specific biological functions of SsCEI within the PEBP family.

Published

2009

34. The prefoldin of the crenarchaeon Sulfolobus solfataricus

Author

Maria Ciaramella, Alessandra Napoli, Mosè Rossi, Anna Valenti, Anna D'Amaro, D'Amaro, A, Valenti, A, Napoli, A, Rossi, Mose', Ciaramella, M., D'Amaro, A., Valenti, A., and Napoli, A.

Subjects

Archaeal Proteins, ved/biology.organism_classification_rank.species, Molecular Sequence Data, medicine.disease_cause, Biochemistry, Sulfolobus, Structural Biology, medicine, Amino Acid Sequence, Cloning, Molecular, Escherichia coli, biology, Base Sequence, ved/biology, Sulfolobus solfataricus, General Medicine, biology.organism_classification, Hyperthermophile, Prefoldin, Chaperone (protein), biology.protein, Gene Expression Regulation, Archaeal, Sequence Alignment, Archaea, Molecular Chaperones

Abstract

Prefoldin is a hetero-hexameric ATP-independent chaperone, shared by eukaryotes and archaea, which binds non-native proteins preventing them from aggregation. We report the identification and characterization in vivo and in vitro of the first prefoldin from a crenarchaeon, the hyperthermophile Sulfolobus solfataricus. A functional complex was obtained either co-expressing the alpha- and beta-prefoldin subunits in Escherichia coli, or incubating at high temperature the separately expressed subunits. In S. solfataricus, prefoldin expression and apparent molecular weight were not affected by either heat or cold shock.

Published

2008

35. A novel thermoacidophilic cellulase from Alicyclobacillus acidocaldarius

Author

Mauro Rossi, F. La Cara, Luisa Maurelli, A. Esposito, Giuseppe Ruggiero, Elena Ionata, Alessandra Morana, Morana, A., Esposito, A., Maurelli, M., Ruggiero, G., Ionata, E., Rossi, Mose', and La Cara, F.

Subjects

glycoprotein, Alicyclobacillus acidocaldarius, Cellulase, Gram-Positive Endospore-Forming Bacteria, Polysaccharide, Biochemistry, Chromatography, Affinity, Substrate Specificity, chemistry.chemical_compound, Structural Biology, carboxymethylcellulose, Polyacrylamide gel electrophoresis, chemistry.chemical_classification, biology, Temperature, General Medicine, Hydrogen-Ion Concentration, biology.organism_classification, Electrophoresis, Monomer, Enzyme, chemistry, biology.protein, Chromatography, Gel, Electrophoresis, Polyacrylamide Gel, Ultracentrifuge, Ultracentrifugation, Bacteria

Abstract

A novel cellulase was isolated from the thermoacidophilic bacterium Alicyclobacillus acidocaldarius ATCC27009 grown in medium containing carboxymethylcellulose. The enzyme is a glycosylated monomer of 56.2 kDa, relatively thermostable, with optimal pH and temperature of 4.0 and 65 degrees C, respectively. Enzymatic assays on several polysaccharides demonstrated that CelG was specific for carboxymethylcellulose.

Published

2008

36. A novel keratinase from Clostridium sporogenes bv. pennavorans bv. nov., a thermotolerant organism isolated from solfataric muds

Author

G. Bianconi, Mauro Rossi, Yoshimi Benno, F. La Cara, F. Canganella, Antonio Capasso, Mitsuo Sakamoto, Elena Ionata, Ionata, E, Canganella, F, Bianconi, G, Benno, Y, Sakamoto, M, Capasso, A, Rossi, Mose', and La Cara, F.

Subjects

animal structures, Clostridium sporogenes, Biology, Microbiology, Clostridia, keratinase, Bacterial Proteins, RNA, Ribosomal, 16S, Animals, Anaerobiosis, feathers degradation, Phylogeny, Soil Microbiology, chemistry.chemical_classification, Clostridium, Molecular mass, Hydrolysis, Temperature, food and beverages, Ribosomal RNA, Feathers, Hydrogen-Ion Concentration, biology.organism_classification, Molecular Weight, RNA, Bacterial, Enzyme, Keratinase, chemistry, Italy, Culture Media, Conditioned, biology.protein, Soil microbiology, Chickens, clostridia, Bacteria, Peptide Hydrolases

Abstract

A bacterium which can grow on chicken feathers and which exhibits keratinolytic activity was isolated from solfataric muds. It was classified as belonging to the genus Clostridium and closely related to C. sporogenes. Based on its unique capability to degrade chicken feathers, it was designated as Clostridium sporogenes bv. pennavorans bv. nov. The keratinase purified from the culture supernatant is a monomer of 28.7kDa molecular mass. The enzyme is relatively thermostable and is active over a broad range of temperature and pH. Specific enzymatic assays demonstrate that keratinase can act on a large variety of soluble and insoluble protein substrates.

Published

2008

37. Purification and characterization of a novel recombinant highly enantioselective ,short-chain NAD(H)-dependent alcohol dehydrogenase from Thermus thermophilus

Author

Angela Pennacchio, Francesco La Cara, Francesco Secundo, Biagio Pucci, Carlo A. Raia, Mosè Rossi, Pennacchio, A., Pucci, B., Secundo, F., La Cara, F., Rossi, Mose', and Raia, C. A.

Subjects

Hot Temperature, Molecular Sequence Data, Dehydrogenase, Reductase, Applied Microbiology and Biotechnology, Cofactor, Substrate Specificity, Enzyme Stability, Escherichia coli, Amino Acid Sequence, Enzymology and Protein Engineering, Enantiomeric excess, Alcohol dehydrogenase, chemistry.chemical_classification, Ecology, biology, Thermus thermophilus, Alcohol Dehydrogenase, Stereoisomerism, NAD, biology.organism_classification, Recombinant Proteins, Kinetics, Enzyme, Biochemistry, chemistry, biology.protein, NAD+ kinase, Sequence Alignment, Food Science, Biotechnology

Abstract

The gene encoding a novel alcohol dehydrogenase (ADH) that belongs to the short-chain dehydrogenase/reductase (SDR) superfamily was identified in the extremely thermophilic, halotolerant gram-negative eubacterium Thermus thermophilus HB27. The T. thermophilus ADH gene ( adh Tt ) was heterologously overexpressed in Escherichia coli , and the protein (ADH Tt ) was purified to homogeneity and characterized. ADH Tt is a tetrameric enzyme consisting of identical 26,961-Da subunits composed of 256 amino acids. The enzyme has remarkable thermophilicity and thermal stability, displaying activity at temperatures up to ∼73°C and a 30-min half-inactivation temperature of ∼90°C, as well as good tolerance to common organic solvents. ADH Tt has a strict requirement for NAD(H) as the coenzyme, a preference for reduction of aromatic ketones and α-keto esters, and poor activity on aromatic alcohols and aldehydes. This thermophilic enzyme catalyzes the following reactions with Prelog specificity: the reduction of acetophenone, 2,2,2-trifluoroacetophenone, α-tetralone, and α-methyl and α-ethyl benzoylformates to ( S )-(−)-1-phenylethanol (>99% enantiomeric excess [ee]), ( R )-α-(trifluoromethyl)benzyl alcohol (93% ee), ( S )-α-tetralol (>99% ee), methyl ( R )-(−)-mandelate (92% ee), and ethyl ( R )-(−)-mandelate (95% ee), respectively, by way of an efficient in situ NADH-recycling system involving 2-propanol and a second thermophilic ADH. This study further supports the critical role of the D37 residue in discriminating NAD(H) from NADP(H) in members of the SDR superfamily.

Published

2008

38. The alpha-L-fucosidase from Sulfolobus solfataricus

Author

Marco Moracci, Beatrice Cobucci-Ponzano, Fiorella Conte, Mosè Rossi, Cobucci Ponzano, Beatrice, Conte, Fiorella, Rossi, Mose', and Moracci, Marco

Subjects

Hot Temperature, Archaeal Proteins, ved/biology.organism_classification_rank.species, Microbiology, Catalysis, Catalysi, Archaeal Protein, Catalytic triad, chemical rescue, Glycoside hydrolase, glycoside hydrolase, alpha-L-Fucosidase, Binding Sites, biology, ved/biology, Sulfolobus solfataricus, Interrupted gene, Binding Site, Active site, Frameshifting, Ribosomal, Sulfolobaceae, General Medicine, Sulfolobus solfataricu, biology.organism_classification, Biochemistry, Models, Chemical, catalytic triad, biology.protein, acid/base, Molecular Medicine, nucleophile, Sulfolobales, Archaea

Abstract

Glycoside hydrolases form hyperthermophilic archaea are interesting model systems for the study of catalysis at high temperatures and, at the moment, their detailed enzymological characterization is the only approach to define their role in vivo. Family 29 of glycoside hydrolases classification groups alpha-L: -fucosidases involved in a variety of biological events in Bacteria and Eukarya. In Archaea the first alpha-L: -fucosidase was identified in Sulfolobus solfataricus as interrupted gene expressed by programmed -1 frameshifting. In this review, we describe the identification of the catalytic residues of the archaeal enzyme, by means of the chemical rescue strategy. The intrinsic stability of the hyperthermophilic enzyme allowed the use of this method, which resulted of general applicability for beta and alpha glycoside hydrolases. In addition, the presence in the active site of the archaeal enzyme of a triad of catalytic residues is a rather uncommon feature among the glycoside hydrolases and suggested that in family 29 slightly different catalytic machineries coexist.

Published

2008

39. A proteomic approach to study Escherichia coli acetyl esyterase interactors unveil a sequence motif involved in protein-protein interactions

Author

Andrea Scaloni, Giuseppe Manco, Chiara D'Ambrosio, Mosè Rossi, Luigi Mandrich, D. '. A. m. b. r. o. s. i., O., Mandrich, L., Rossi, Mose', Scaloni, A., and Manco, G.

Subjects

Lipopolysaccharides, Proteomics, Structural similarity, Amino Acid Motifs, Biology, medicine.disease_cause, Biochemistry, Mass Spectrometry, Protein–protein interaction, Structural Biology, Escherichia coli, Consensus sequence, medicine, Protein Interaction Domains and Motifs, Maltose, Escherichia coli Proteins, Cystathionine gamma-Lyase, Computational Biology, General Medicine, Repressor Proteins, Regulon, Proteome, Mutagenesis, Site-Directed, Acetylesterase, Sequence motif, Metabolic Networks and Pathways, Protein Binding

Abstract

E. coli acetyl esterase (Aes) and beta-cysthationase (MalY) interact, probably with the same mechanism, with the N-terminus of transcriptional activator of maltose regulon (MalT). In order to investigate the basic mechanism of this interaction, we used both a proteomic and a bioinformatic approach. Affinity-based mass spectrometry experiments with purified Aes protein as bait allowed to fish twenty-three, apparently specific, interactors from crude extracts of E. coli cells grown in different conditions. The group of interactors appeared quite heterogeneous, comprising Aes itself, some molecular chaperons, metabolic enzymes, and several proteins of unknown function. Among the identified proteins, two are in some way related to the maltose metabolism and two are related to the lipopolysaccharide metabolism. By superposing the structures of the Alicyclobacillus acidocaldarius EST2, an Aes homolog, and MalY, a region of structural similarity was discovered that allowed detecting a short stretch of nine residues with sequence similarity among EST2, AES and MalY. Degenerated sequence consensuses derived from the alignment were used to analyse the E. coli proteome in the Swiss Prot database and permitted to retrieve sequences of Aes interactors already known or detected in this study. Most of these interactors (14 out of 25) contain the expected consensus. A site-directed mutant of Aes R179A made in the consensus sequence resulted in complete loss of interaction. Based on the analysis of the available three-dimensional structures and mutagenic and structural data inferred from literature, we predict a role of this motif in protein-protein interaction.

Published

2008

40. Fluorescence correlation spectroscopy assay for gliadin in food

Author

Sabato D'Auria, Mosè Rossi, Antonio Varriale, Beniamino Barbieri, Mauro Rossi, Ewald Terpetschnig, Maria Staiano, Varriale, A, Rossi, Mose', Staiano, M, Terpetschnig, E, Barbieri, B, Rossi, M, and D'Auria, S.

Subjects

Glutens, Fluorescence spectrometry, Peptide, Fluorescence correlation spectroscopy, Sensitivity and Specificity, digestive system, Gliadin, Fluorescence spectroscopy, Analytical Chemistry, Mice, chemistry.chemical_compound, Antibody Specificity, Animals, Fluorescein, GLUTEN, Immunoassay, chemistry.chemical_classification, Detection limit, Mice, Inbred BALB C, Chromatography, biology, CELIAC-DISEASE, Reproducibility of Results, nutritional and metabolic diseases, Fluoresceins, Gluten, digestive system diseases, Spectrometry, Fluorescence, chemistry, Biochemistry, Immunoglobulin G, biology.protein, Food Analysis

Abstract

Gliadin proteins are primarily responsible for celiac disease. As gliadin is a complex mixture of proteins difficult to solubilize and to extract from food, it is difficult to develop an assay capable of accurate quantization of gliadin in food for celiac patients. In this work, we present an advanced fluorescence assay for the detection of traces of gliadin in food. The described assay is based on measurement of the fluctuations of fluorescein-labeled gliadin peptides (GP) in a focused laser beam in the absence and in the presence of anti-GP antibodies. A competitive assay based on the utilization of unlabeled GP was developed. The obtained results indicate that the combination of high-avidity IgG antibodies together with the innovative fluorescence immunoassay strategy resulted in a gluten detection limit of 0.006 ppm, which it is much lower than the values reported in the literature.

Published

2007

41. MarR-like transcriptional regulator involved in the detoxification of aromatic compounds in Sulfolobus solfataricus

Author

Raffaele Cannio, Gabriella Fiorentino, Mosè Rossi, Raffaele Ronca, Simonetta Bartolucci, Fiorentino, Gabriella, Ronca, Raffaele, Cannio, R, Rossi, Mose', and Bartolucci, Simonetta

Subjects

Transcription, Genetic, Operon, archaea, Archaeal Proteins, Molecular Sequence Data, ved/biology.organism_classification_rank.species, DNA Footprinting, Electrophoretic Mobility Shift Assay, RNA, Archaeal, Biology, Microbiology, Escherichia coli, Transcriptional regulation, Gene Regulation, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Promoter Regions, Genetic, Molecular Biology, Gene, Regulator gene, transcriptional regulator, Regulation of gene expression, Sequence Homology, Amino Acid, ved/biology, Sulfolobus solfataricus, Promoter, Gene Expression Regulation, Bacterial, Sulfolobus solfataricu, Blotting, Northern, Recombinant Proteins, DNA-Binding Proteins, Repressor Proteins, DNA, Archaeal, Biochemistry, Regulatory sequence, Benzaldehydes, Protein Binding

Abstract

A DNA binding protein, BldR, was identified in the crenarchaeon Sulfolobus solfataricus as a protein 5- to 10-fold more abundant in cells grown in the presence of toxic aldehydes; it binds to regulatory sequences located upstream of an alcohol dehydrogenase gene (Sso2536). BldR is homologous to bacterial representatives of the MarR (multiple antibiotic resistance) family of transcriptional regulators that mediate response to multiple environmental stresses. Transcriptional analysis revealed that the bldR gene was transcribed in a bicistronic unit composed of the genes encoding the transcriptional regulator (Sso1352) and a putative multidrug transporter (Sso1351) upstream. By homology to bacterial counterparts, the bicistron was named the mar -like operon. The level of mar -like operon expression was found to be increased at least 10-fold in response to chemical stress by aromatic aldehydes. Under the same growth conditions, similar enhanced in vivo levels of Sso2536 gene transcript were also measured. The gene encoding BldR was expressed in E. coli , and the recombinant protein was purified to homogeneity. DNA binding assays demonstrated that the protein is indeed a transcription factor able to recognize site specifically both the Sso2536 and mar -like promoters at sites containing palindromic consensus sequences. Benzaldehyde, the substrate of ADH Ss , stimulates DNA binding of BldR at both promoters. The role of BldR in the auto-activation as well as in the regulation of the Sso2536 gene, together with results of increased operon and gene expression under conditions of exposure to aromatic aldehydes, indicates a novel coordinate regulatory mechanism in cell defense against stress by aromatic compounds.

Published

2007

42. Modular organization of the Sulfolobus solfataricus mini-chromosome maintenance protein

Author

Monia Rocco, Mariarita De Felice, Francesco Esposito, Mariarosaria De Falco, Mosè Rossi, Francesca M. Pisani, Luca Esposito, Biagio Pucci, Pucci, B, DE FELICE, M, Rocco, M, Esposito, F, DE FALCO, M, Esposito, L, Rossi, Mose', and Pisani, Fm

Subjects

Archaeal Proteins, ved/biology.organism_classification_rank.species, Biochemistry, Models, Biological, chemistry.chemical_compound, Structure-Activity Relationship, Protein structure, Minichromosome maintenance, MCM complex, Amino Acid Sequence, Molecular Biology, Sequence Deletion, Adenosine Triphosphatases, biology, ved/biology, Oligonucleotide, Sulfolobus solfataricus, DNA Helicases, Helicase, Cell Biology, DNA Replication Fork, Recombinant Proteins, Protein Structure, Tertiary, DNA-Binding Proteins, chemistry, biology.protein, DNA

Abstract

Mini-chromosome maintenance (MCM) proteins form ring-like hexameric complexes that are commonly believed to act as the replicative DNA helicase at the eukaryotic/archaeal DNA replication fork. Because of their simplified composition with respect to the eukaryotic counterparts, the archaeal MCM complexes represent a good model system to use in analyzing the structural/functional relationships of these important replication factors. In this study the domain organization of the MCM-like protein from Sulfolobus solfataricus (Sso MCM) has been dissected by trypsin partial proteolysis. Three truncated derivatives of Sso MCM corresponding to protease-resistant domains were produced as soluble recombinant proteins and purified: the N-terminal domain (N-ter, residues 1-268); a fragment comprising the AAA+ and C-terminal domains (AAA+-C-ter, residues 269-686); and the C-terminal domain (C-ter, residues 504-686). All of the purified recombinant proteins behaved as monomers in solution as determined by analytical gel filtration chromatography, suggesting that the polypeptide chain integrity is required for stable oligomerization of Sso MCM. However, the AAA+-C-ter derivative, which includes the AAA+ motor domain and retains ATPase activity, was able to form dimers in solution when ATP was present, as analyzed by size exclusion chromatography and glycerol gradient sedimentation analyses. Interestingly, the AAA+-C-ter protein could displace oligonucleotides annealed to M13 single-stranded DNA although with a reduced efficiency in comparison with the full-sized Sso MCM. The implications of these findings for understanding the DNA helicase mechanism of the MCM complex are discussed.

Published

2007

43. Biochemical evidence of a physical interaction between Sulfolobus solfataricus B-family and Y-family DNA polymerases

Author

Francesca M. Pisani, Biagio Pucci, Mariarosaria De Falco, Mariarita De Felice, Petr Grúz, Luca Esposito, Takehiko Nohmi, Mosè Rossi, Barbara Medagli, De Felice, M., Medagli, B., Esposito, L., De Falco, M., Pucci, B., Rossi, Mose', Gruz, P., Nohmi, T., and Pisani, F. M.

Subjects

DNA polymerase, Archaeal Proteins, DNA polymerase II, ved/biology.organism_classification_rank.species, DNA-Directed DNA Polymerase, DNA replication, Microbiology, DNA polymerase delta, Protein Structure, Secondary, Genome, Archaeal, Genome stability, Translesion synthesis, biology, ved/biology, Sulfolobus solfataricus, General Medicine, Base excision repair, Processivity, Surface Plasmon Resonance, Archaea, Biochemistry, Coding strand, biology.protein, Molecular Medicine, DNA Damage, Protein Binding

Abstract

The hyper-thermophilic archaeon Sulfolobus solfataricus possesses two functional DNA polymerases belonging to the B-family (Sso DNA pol B1) and to the Y-family (Sso DNA pol Y1). Sso DNA pol B1 recognizes the presence of uracil and hypoxanthine in the template strand and stalls synthesis 3-4 bases upstream of this lesion ("read-ahead" function). On the other hand, Sso DNA pol Y1 is able to synthesize across these and other lesions on the template strand. Herein we report evidence that Sso DNA pol B1 physically interacts with DNA pol Y1 by surface plasmon resonance measurements and immuno-precipitation experiments. The region of DNA pol B1 responsible for this interaction has been mapped in the central portion of the polypeptide chain (from the amino acid residue 482 to 617), which includes an extended protease hyper-sensitive linker between the N- and C-terminal modules (amino acid residues Asn482-Ala497) and the alpha-helices forming the "fingers" sub-domain (alpha-helices R, R' and S). These results have important implications for understanding the polymerase-switching mechanism on the damaged template strand during genome replication in S. solfataricus.

Published

2007

44. Temperature modulates binding specificity and affinity of the D-trehalose/D-maltose-binding protein from the hyperthermophilic archaeon Thermococcus litoralis

Author

Mosè Rossi, Sabato D'Auria, Petr Herman, Annalisa Vitale, Jaroslav Vecer, Maria Staiano, Ivan Barvík, Herman, P, Barvik, I. J. r., Staiano, M, Vitale, A, Vecer, J, Rossi, Mose', and D'Auria, S.

Subjects

Models, Molecular, Archaeal Proteins, Biophysics, macromolecular substances, Biochemistry, Fluorescence spectroscopy, Analytical Chemistry, law.invention, Maltose-binding protein, chemistry.chemical_compound, law, Thermococcus litoralis, Maltose, Molecular Biology, Binding selectivity, Thermostability, biology, Chemistry, Temperature, Trehalose, biology.organism_classification, Thermococcus, carbohydrates (lipids), Spectrometry, Fluorescence, biology.protein, Recombinant DNA, Biosensor, Protein Binding

Abstract

We investigated the effect of temperature on the binding specificity of the recombinant d-trehalose/d-maltose-binding protein from the hyperthermophilic archaeon Thermococcus litoralis (TMBP). Importantly, we found that TMBP can bind d-glucose (Glc). The Glc binding was characterized by means of fluorescence spectroscopy in the temperature range of 25 degrees C-85 degrees C. Our results show that at 25 degrees C the binding of Glc to TMBP is well represented by a bimodal model with apparent K(d) of 20 muM and approximately 3-8 mM for the first and the second binding step, respectively. At 60 degrees C the binding of Glc to TMBP is represented by a simple hyperbolic model with an apparent K(d) value of about 40 muM. Finally, at 85 degrees C Glc did not bind to TMBP. Molecular dynamics (MD) simulations were used to shed light on the molecular mechanism of the Glc binding. Our results suggest that after proper fluorescent labeling TMBP can be used as a highly thermostable and non-consuming analyte biosensor for monitoring the level of glucose in fluids (e.g. human blood) where other sugars are not present.

Published

2007

45. Molecular adaptation strategies to high temperature and thermal denaturation mechanism of the D-Trehalose/D-Maltose-binding protein from the hyperthermophilic archaeon Thermococcus litoralis

Author

Alberto Schiraldi, Alberto Barbiroli, Dimitrios Fessas, Maria Staiano, Anna Marabotti, Sabato D'Auria, Mosè Rossi, Antonio Varriale, Fessas, D, Staiano, M, Barbiroli, A, Marabotti, A, Schiraldi, A, Varriale, A, Rossi, Mose', and Dauria, S.

Subjects

Models, Molecular, Protein Denaturation, Adaptation, Biological, Crystallography, X-Ray, Biochemistry, Maltose-Binding Proteins, law.invention, chemistry.chemical_compound, Maltose-binding protein, GLOBULAR-PROTEINS, Protein structure, Structural Biology, law, Settore BIO/10 - Biochimica, CRYSTAL-STRUCTURE, Denaturation (biochemistry), TRANSPORT-SYSTEM, Thermococcus litoralis, Molecular Biology, Settore CHIM/02 - Chimica Fisica, Thermostability, biology, Calorimetry, Differential Scanning, Temperature, Trehalose, Maltose, biology.organism_classification, Protein Structure, Tertiary, BETA-GLYCOSIDASE, Thermococcus, chemistry, Recombinant DNA, biology.protein, SULFOLOBUS-SOLFATARICUS, Carrier Proteins

Abstract

The D-trehalose/D-maltose-binding protein (TMBP), a monomeric protein of 48 kDa, is one component of the trehalose and maltose uptake system. In the hyperthermophilic archaeon T. litoralis this is mediated by a protein-dependent ATP-binding cassette system transporter. The gene coding for a thermostable TMBP from the archaeon T. litoralis has been cloned, and the recombinant protein has been expressed in E. coli. The recombinant TMBP has been purified to homogeneity and characterized. It exhibits the same functional and structural properties as the native one. In fact, it is highly thermostable and binds both trehalose and maltose with high affinity. In this work we used differential scanning calorimetry studies together with a detailed analysis, at the molecular level, of the three-dimensional protein structure to shed light on the basis of the high thermostability exhibited by the recombinant TMBP from the archaeon T. litoralis. The obtained data suggest that the presence of trehalose does not change the overall mechanism of the denaturation of this protein but it selectively modifies the stability of the TMBP structural domains. Proteins 2007. © 2007 Wiley-Liss, Inc.

Published

2007

46. Identification of the first archaeal oligopeptide-binding protein from the hyperthermophile Aeropyrum pernix

Author

Gennaro Marino, Gianna Palmieri, Annarita Casbarra, Mosè Rossi, Silvia Onesti, Giuliana Catara, Antonio Capasso, Immacolata Fiume, Palmieri, G, Casbarra, A, Fiume, I, Catara, G, Capasso, A, Marino, Gennaro, Onesti, S, and Rossi, Mose'

Subjects

Proteomics, MALDI Mass Spectrometry, Hot Temperature, Archaeal Proteins, Molecular Sequence Data, ATP-binding cassette transporter, Oligopeptide transport, Peptide Mapping, Microbiology, Genes, Archaeal, Aeropyrum pernix, Bacterial Proteins, Oligopeptide binding protein, Genome, Archaeal, Amino Acid Sequence, Isoelectric Point, Peptide sequence, Oligopeptide, biology, Binding protein, Aeropyrum, General Medicine, biology.organism_classification, Archaea, Hyperthermophile, Molecular Weight, Biochemistry, Molecular Medicine, ATP-Binding Cassette Transporters, ABC transport, Carrier Proteins, Oligopeptides, Oligopeptide binding

Abstract

The archaeon Aeropyrum pernix grows optimally at 90 degrees C and derives energy primarily from aerobic degradation of complex proteinaceous substrates. The ability of these nutrients to sustain growth is generally associated with the presence of oligopeptide transport systems, such as the well-known protein-dependent ATP-binding cassette (ABC) transporters. This study is concerned with the isolation and characterisation of the first archaeal oligopeptide-binding protein (OppA(Ap)) from the extracellular medium of A. pernix. The protein shows a pI of 3.9 and a molecular mass of about 90 kDa under native conditions. By using a proteomic approach, the OppA(Ap)-encoding gene was identified (APE1583) and about 55% of the protein amino-acid sequence was validated. The extracellular purified protein was able to efficiently bind oligopeptide substrates such as Xenopsin. The amount of a liganded peptide to OppA(Ap) was about 70% at 90 degrees C using a 1/100 (w/w) OppA(Ap)/substrate ratio. Sequence comparisons showed a weak but significant similarity of OppA(Ap) with bacterial oligopeptide binding proteins. Furthermore, APE1583 neighbouring genes encode for the cognate components of an ABC transport system, suggesting that these ORFs are organised in an operon-like structure, with OppA(Ap )as the extracellular component for the uptake of oligopeptides.

Published

2006

47. The gene of an archaeal alpha-L-fucosidase is expressed by translational frameshifting

Author

Angela Flagiello, Mosè Rossi, Piero Pucci, Dario Benelli, Marco Moracci, Paola Londei, Fiorella Conte, Beatrice Cobucci-Ponzano, Maria Chiara Monti, COBUCCI PONZANO, B, Conte, F, Benelli, D, Londei, P, Flagiello, A, Monti, Maria, Pucci, Pietro, Rossi, Mose', and Moracci, Marco

Subjects

archaea, ved/biology.organism_classification_rank.species, Regulatory site, medicine.disease_cause, Escherichia coli, Genetics, medicine, split genes, Fucosidase, Frameshift Mutation, Molecular Biology, Gene, alpha-L-Fucosidase, recoding, Translational frameshift, biology, ved/biology, Sulfolobus solfataricus, Frameshifting, Ribosomal, Stop codon, Open reading frame, programmed frameshifting, gene expression, biology.protein, Gene Expression Regulation, Archaeal

Abstract

The standard rules of genetic translational decoding are altered in specific genes by different events that are globally termed recoding. In Archaea recoding has been unequivocally determined so far only for termination codon readthrough events. We study here the mechanism of expression of a gene encoding for a alpha-l-fucosidase from the archaeon Sulfolobus solfataricus (fucA1), which is split in two open reading frames separated by a -1 frameshifting. The expression in Escherichia coli of the wild-type split gene led to the production by frameshifting of full-length polypeptides with an efficiency of 5%. Mutations in the regulatory site where the shift takes place demonstrate that the expression in vivo occurs in a programmed way. Further, we identify a full-length product of fucA1 in S.solfataricus extracts, which translate this gene in vitro by following programmed -1 frameshifting. This is the first experimental demonstration that this kind of recoding is present in Archaea.

Published

2006

48. Characterization of a multifunctional Protein Disulfide Oxidoreductase from Sulfolobus solfataricus

Author

Mosè Rossi, Emilia Pedone, Danila Limauro, Simonetta Bartolucci, Romina D'Alterio, Pedone, E, Limauro, Danila, Dalterio, R, Rossi, Mose', and Bartolucci, Simonetta

Subjects

redox site, Time Factors, Thioredoxin reductase, Molecular Sequence Data, ved/biology.organism_classification_rank.species, thioredoxin system, Isomerase, Reductase, Biology, Biochemistry, Oxidoreductase, Amino Acid Sequence, Cysteine, Disulfides, Protein disulfide-isomerase, Molecular Biology, Fluorescent Dyes, chemistry.chemical_classification, thermophile, ved/biology, Sulfolobus solfataricus, Protein Disulfide Reductase (Glutathione), Ferredoxin-thioredoxin reductase, Cell Biology, Sulfolobus solfataricu, chemistry, protein disulfide oxidoreductases (PDO), Thioredoxin, Sequence Alignment, Molecular Chaperones

Abstract

A potential role in disulfide bond formation in the intracellular proteins of thermophilic organisms has recently been ascribed to a new family of protein disulfide oxidoreductases (PDOs). We report on the characterization of SsPDO, isolated from the hyperthermophilic archaeon Sulfolobus solfataricus. SsPDO was cloned and expressed in Escherichia coli. We revealed that SsPDO is the substrate of a thioredoxin reductase in S. solfataricus (K(M) 0.3 microm) and not thioredoxins (TrxA1 and TrxA2). SsPDO/S. solfataricus thioredoxin reductase constitute a new thioredoxin system in aerobic thermophilic archaea. While redox (reductase, oxidative and isomerase) activities of SsPDO point to its central role in the biochemistry of cytoplasmic disulfide bonds, chaperone activities also on an endogenous substrate suggest a potential role in the stabilization of intracellular proteins. Northern and western analysis have been performed in order to analyze the response to the oxidative stress.

Published

2006

49. Characterization of the Sulfolobus host-SSV2 virus interaction

Author

Qunxin She, Susanne L. Jensen, Simonetta Bartolucci, Patrizia Contursi, Mosè Rossi, Tiziana Aucelli, Contursi, Patrizia, Jensen, S, Aucelli, Tiziana, Rossi, Mose', Bartolucci, Simonetta, and She, Q.

Subjects

Archaeal Viruses, DNA Replication, Virus Integration, ved/biology.organism_classification_rank.species, Integration, Fuselloviridae, Virus Replication, Microbiology, Virus, Sulfolobus, chemistry.chemical_compound, Gene, Genetics, Integrases, biology, ved/biology, Host (biology), Archaeal viru, Sulfolobus solfataricus, General Medicine, Provirus, biology.organism_classification, DNA, Archaeal, chemistry, Molecular Medicine, DNA

Abstract

The Sulfolobus spindle virus, SSV2, encodes a tyrosine integrase which furthers provirus formation in host chromosomes. Consistently with the prediction made during sequence analysis, integration was found to occur in the downstream half of the tRNA(Gly) (CCC) gene. In this paper we report the findings of a comparative study of SSV2 physiology in the natural host, Sulfolobus islandicus REY15/4, versus the foreign host, Sulfolobus solfataricus, and provide evidence of differently regulated SSV2 life cycles in the two hosts. In fact, whereas a significant induction of SSV2 replication takes place during the growth of the natural host REY15/4, the cellular content of SSV2 DNA remains fairly low throughout the incubation of the foreign host. The accumulation of episomal DNA in the former case cannot be traced to decreased packaging activity because of a simultaneous increase in the virus titre in the medium. In addition, the interaction between SSV2 and its natural host is characterized by the concurrence of host growth inhibition and the induction of viral DNA replication. When this virus-host interaction was investigated using S. islandicus REY15A, a strain which is closely related to the natural host, it was found that the SSV2 replication process was induced in the same way as in the natural host REY15/4.

Published

2006

50. A new kumamolisin-like protease from Alicyclobacillus acidocaldarius: an enzyme active under extreme acidic conditions

Author

Giuliana Catara, Giovanna Maria, Giuseppe Ruggiero, Antonio Capasso, Gianna Palmieri, Immacolata Fiume, Filippo Iuliano, Mosè Rossi, Catara, G, Fiume, I, Iuliano, F, Maria, G, Ruggiero, G, Palmieri, G, Capasso, A, and Rossi, Mose'

Subjects

chemistry.chemical_classification, Proteases, Protease, biology, Chemistry, medicine.medical_treatment, collagenolytic protease, Substrate (chemistry), protease substrate specificity, biology.organism_classification, Biochemistry, Catalysis, law.invention, Enzyme, Biotransformation, law, renewable wastes, medicine, Recombinant DNA, Specific activity, biotransformation, recombinant enzyme, Bacteria, Biotechnology

Abstract

A new serine-carboxyl proteinase, called kumamolisin-ac, was purified from the thermoacidophilic bacterium Alicyclobacillus acidocaldarius. The enzyme is a monomeric protein of 45 kDa, active over a wide temperature range (5.0–70°C) and extremely acidic pHs (1.0–4.0), showing maximal proteolytic activity at pH 2.0 and 60°C. Interestingly, kumamolisin-ac displayed a significant proteolytic activity even at 5°C, thus suggesting a sort of cold-adaptation for this enzyme. The protease was remarkably stable at high temperatures (t1/2 at 80°C, 10h, pH 2.0) and over a broad range of pH (2.0–7.0). Substrate analysis indicated that kumamolisin-ac was active on a variety of macromolecular substrates, such as haemoglobin, hide powder azure, and azocoll. In particular, a high specific activity was detected towards collagen. The corresponding gene was cloned, expressed and the recombinant protease, was found to be homologous to proteases of the ‘S53’ family. From the high identity with kumamolisin and kumamolisin-As, known as collagenolytic proteases, kumamolisin-ac can be considered as the third collagenolytic affiliate within the ‘S53’ family. Cleavage specificity investigation of kumamolisin-ac revealed a unique primary cleavage site in bovine insulin B-chain, whereas a broad specificity was detected using bovine alpha-globin as substrate. Thus, kumamolisin-ac could represent an attractive candidate for industrial-scale biopeptide production under thermoacidophilic conditions.

Published

2006