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8 results on '"Ana G. C. Neves-Ferreira"'

1. Simple, efficient and thorough shotgun proteomic analysis with PatternLab V

Author

Marlon D. M. Santos, Diogo B. Lima, Juliana S. G. Fischer, Milan A. Clasen, Louise U. Kurt, Amanda Caroline Camillo-Andrade, Leandro C. Monteiro, Priscila F. de Aquino, Ana G. C. Neves-Ferreira, Richard H. Valente, Monique R. O. Trugilho, Giselle V. F. Brunoro, Tatiana A. C. B. Souza, Renata M. Santos, Michel Batista, Fabio C. Gozzo, Rosario Durán, John R. Yates, Valmir C. Barbosa, and Paulo C. Carvalho

Subjects
General Biochemistry, Genetics and Molecular Biology
Published
2022

2. Simple, efficient and thorough shotgun proteomic analysis with PatternLab V

Author

Marlon D M, Santos, Diogo B, Lima, Juliana S G, Fischer, Milan A, Clasen, Louise U, Kurt, Amanda Caroline, Camillo-Andrade, Leandro C, Monteiro, Priscila F, de Aquino, Ana G C, Neves-Ferreira, Richard H, Valente, Monique R O, Trugilho, Giselle V F, Brunoro, Tatiana A C B, Souza, Renata M, Santos, Michel, Batista, Fabio C, Gozzo, Rosario, Durán, John R, Yates, Valmir C, Barbosa, and Paulo C, Carvalho

Subjects
Proteomics, Tandem Mass Spectrometry, Proteins, Databases, Protein, Software
Abstract

Shotgun proteomics aims to identify and quantify the thousands of proteins in complex mixtures such as cell and tissue lysates and biological fluids. This approach uses liquid chromatography coupled with tandem mass spectrometry and typically generates hundreds of thousands of mass spectra that require specialized computational environments for data analysis. PatternLab for proteomics is a unified computational environment for analyzing shotgun proteomic data. PatternLab V (PLV) is the most comprehensive and crucial update so far, the result of intensive interaction with the proteomics community over several years. All PLV modules have been optimized and its graphical user interface has been completely updated for improved user experience. Major improvements were made to all aspects of the software, ranging from boosting the number of protein identifications to faster extraction of ion chromatograms. PLV provides modules for preparing sequence databases, protein identification, statistical filtering and in-depth result browsing for both labeled and label-free quantitation. The PepExplorer module can even pinpoint de novo sequenced peptides not already present in the database. PLV is of broad applicability and therefore suitable for challenging experimental setups, such as time-course experiments and data handling from unsequenced organisms. PLV interfaces with widely adopted software and community initiatives, e.g., Comet, Skyline, PEAKS and PRIDE. It is freely available at http://www.patternlabforproteomics.org .

Published
2021

4. The interaction of the antitoxin DM43 with a snake venom metalloproteinase analyzed by mass spectrometry and surface plasmon resonance

Author

Guilherme D, Brand, Rune, Salbo, Thomas J D, Jørgensen, Carlos, Bloch, Elisabetta, Boeri Erba, Carol V, Robinson, Isabelle, Tanjoni, Ana M, Moura-da-Silva, Peter, Roepstorff, Gilberto B, Domont, Jonas, Perales, Richard H, Valente, and Ana G C, Neves-Ferreira

Subjects
Molecular Weight, Kinetics, Immobilized Proteins, Multiprotein Complexes, Crotalid Venoms, Metalloendopeptidases, Blood Proteins, Surface Plasmon Resonance, Hydrophobic and Hydrophilic Interactions, Mass Spectrometry
Abstract

DM43 is a circulating dimeric antitoxin isolated from Didelphis aurita, a South American marsupial naturally immune to snake envenomation. This endogenous inhibitor binds non-covalently to jararhagin, the main hemorrhagic metalloproteinase from Bothrops jararaca snake venom, and efficiently neutralizes its toxicity. The aim of this study was to apply mass spectrometry (MS) and surface plasmon resonance (SPR) to improve the molecular characterization of this heterocomplex. The stoichiometry of the interaction was confirmed by nanoelectrospray ionization-quadrupole-time-of-flight MS; from native solution conditions, the complex showed a molecular mass of ~94 kDa, indicating that one molecule of jararhagin (50 kDa) interacts with one monomer of DM43 (43 kDa). Although readily observed in solution, the dimeric structure of the inhibitor was barely preserved in the gas phase. This result suggests that, in contrast to the toxin-antitoxin complex, hydrophobic interactions are the primary driving force for the inhibitor dimerization. For the real-time interaction analysis, the toxin was captured on a sensor chip derivatized with the anti-jararhagin monoclonal antibody MAJar 2. The sensorgrams obtained after successive injections of DM43 in a concentration series were globally fitted to a simple bimolecular interaction, yielding the following kinetic rates for the DM43/jararhagin interaction: k(a) = 3.54 ± 0.03 × 10(4) M(-1) s(-1) and k(d) = 1.16 ± 0.07 × 10(-5) s(-1), resulting in an equilibrium dissociation constant (K(D) ) of 0.33 ± 0.06 nM. Taken together, MS and SPR results show that DM43 binds to its target toxin with high affinity and constitute the first accurate quantitative study on the extent of the interaction between a natural inhibitor and a metalloproteinase toxin, with unequivocal implications for the use of this kind of molecule as template for the rational development of novel antivenom therapies.

Published
2012

5. Functional analysis of DM64, an antimyotoxic protein with immunoglobulin-like structure from Didelphis marsupialis serum

Author

Surza L G, Rocha, Bruno, Lomonte, Ana G C, Neves-Ferreira, Monique R O, Trugilho, Inácio de L M, Junqueira-de-Azevedo, Paulo L, Ho, Gilberto B, Domont, José M, Gutiérrez, and Jonas, Perales

Subjects
DNA, Complementary, Molecular Sequence Data, Immunoglobulins, Phospholipases A, Mice, Crotalid Venoms, Animals, Humans, Bothrops, Protease Inhibitors, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Gene Library, Glycoproteins, Base Sequence, Dose-Response Relationship, Drug, Sequence Homology, Amino Acid, Hydrolysis, Metalloendopeptidases, Blood Proteins, Opossums, Protein Structure, Tertiary, Phospholipases A2, Liver, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Electrophoresis, Polyacrylamide Gel, Isoelectric Focusing
Abstract

Bothrops snake venoms are known to induce local tissue damage such as hemorrhage and myonecrosis. The opossum Didelphis marsupialis is resistant to these snake venoms and has natural venom inhibitors in its plasma. The aim of this work was to clone and study the chemical, physicochemical and biological properties of DM64, an antimyotoxic protein from opossum serum. DM64 is an acidic protein showing 15% glycosylation and with a molecular mass of 63 659 Da when analysed by MALDI-TOF MS. It was cloned and the amino acid sequence was found to be homologous to DM43, a metalloproteinase inhibitor from D. marsupialis serum, and to human alpha1B-glycoprotein, indicating the presence of five immunoglobulin-like domains. DM64 neutralized both the in vivo myotoxicity and the in vitro cytotoxicity of myotoxins I (mt-I/Asp49) and II (mt-II/Lys49) from Bothrops asper venom. The inhibitor formed noncovalent complexes with both toxins, but did not inhibit the PLA2 activity of mt-I. Accordingly, DM64 did not neutralize the anticoagulant effect of mt-I nor its intracerebroventricular lethality, effects that depend on its enzymatic activity, and which demonstrate the dissociation between the catalytic and toxic activities of this Asp49 myotoxic PLA2. Furthermore, despite its similarity with metalloproteinase inhibitors, DM64 presented no antihemorrhagic activity against Bothrops jararaca or Bothrops asper crude venoms, and did not inhibit the fibrinogenolytic activity of jararhagin or bothrolysin. This is the first report of a myotoxin inhibitor with an immunoglobulin-like structure isolated and characterized from animal blood.

Published
2002

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