Your search keyword '"Richard H Valente"' showing total 99 results

1. Isolation and molecular characterization of a major hemolymph serpin from the triatomine, Panstrongylus megistus

Author

Carlos JC Moreira, Peter J Waniek, Richard H Valente, Paulo C Carvalho, Jonas Perales, Denise Feder, Reinaldo B Geraldo, Helena C Castro, Patricia Azambuja, Norman A Ratcliffe, and Cícero B Mello

Subjects

Panstrongylus megistus, Serpin, Hemolymph, Serine protease, Cleavage sites, T. cruzi serpin modulation, Infectious and parasitic diseases, RC109-216

Abstract

Abstract Background Chagas disease kills 2.5 thousand people per year of 15 million persons infected in Latin America. The disease is caused by the protozoan, Trypanosome cruzi, and vectored by triatomine insects, including Panstrongylus megistus, an important vector in Brazil. Medicines treating Chagas disease have unpleasant side effects and may be ineffective, therefore, alternative control techniques are required. Knowledge of the T. cruzi interactions with the triatomine host needs extending and new targets/strategies for control identified. Serine and cysteine peptidases play vital roles in protozoan life cycles including invasion and entry of T. cruzi into host cells. Peptidase inhibitors are, therefore, promising targets for disease control. Methods SDS PAGE and chromatograpy detected and isolated a P. megistus serpin which was peptide sequenced by mass spectrometry. A full amino acid sequence was obtained from the cDNA and compared with other insect serpins. Reverse transcription PCR analysis measured serpin transcripts of P. megistus tissues with and without T. cruzi infection. Serpin homology modeling used the Swiss Model and Swiss-PDB viewer programmes. Results The P. megistus serpin (PMSRP1) has a ca. 40 kDa molecular mass with 404 amino acid residues. A reactive site loop contains a highly conserved hinge region but, based on sequence alignment, the normal cleavage site for serine proteases at P1-P1′ was translocated to the putative position P4′-P5′. A small peptide obtained corresponded to the C-terminal 40 amino acid region. The secondary structure of PMSRP1 indicated nine α-helices and three β-sheets, similar to other serpins. PMSRP1 transcripts occurred in all tested tissues but were highest in the fat body and hemocytes. Levels of mRNA encoding PMSRP1 were significantly modulated in the hemocytes and stomach by T. cruzi infection indicating a role for PMSRP1 in the parasite interactions with P. megistus. Conclusions For the first time, a constitutively expressed serpin has been characterized from the hemolymph of a triatomine. This opens up new research avenues into the roles of serine peptidases in the T. cruzi/P. megistus association. Initial experiments indicate a role for PMSRP1 in T. cruzi interactions with P. megistus and will lead to further functional studies of this molecule.

Published

2014

2. Interrogating the Venom of the Viperid Snake Sistrurus catenatus edwardsii by a Combined Approach of Electrospray and MALDI Mass Spectrometry.

Author

Alex Chapeaurouge, Md Abu Reza, Stephen P Mackessy, Paulo C Carvalho, Richard H Valente, André Teixeira-Ferreira, Jonas Perales, Qingsong Lin, and R Manjunatha Kini

Subjects

Medicine, Science

Abstract

The complete sequence characterization of snake venom proteins by mass spectrometry is rather challenging due to the presence of multiple isoforms from different protein families. In the present study, we investigated the tryptic digest of the venom of the viperid snake Sistrurus catenatus edwardsii by a combined approach of liquid chromatography coupled to either electrospray (online) or MALDI (offline) mass spectrometry. These different ionization techniques proved to be complementary allowing the identification a great variety of isoforms of diverse snake venom protein families, as evidenced by the detection of the corresponding unique peptides. For example, ten out of eleven predicted isoforms of serine proteinases of the venom of S. c. edwardsii were distinguished using this approach. Moreover, snake venom protein families not encountered in a previous transcriptome study of the venom gland of this snake were identified. In essence, our results support the notion that complementary ionization techniques of mass spectrometry allow for the detection of even subtle sequence differences of snake venom proteins, which is fundamental for future structure-function relationship and possible drug design studies.

Published

2015

3. Comparison of phylogeny, venom composition and neutralization by antivenom in diverse species of bothrops complex.

Author

Leijiane F Sousa, Carolina A Nicolau, Pedro S Peixoto, Juliana L Bernardoni, Sâmella S Oliveira, José Antonio Portes-Junior, Rosa Helena V Mourão, Isa Lima-dos-Santos, Ida S Sano-Martins, Hipócrates M Chalkidis, Richard H Valente, and Ana M Moura-da-Silva

Subjects

Arctic medicine. Tropical medicine, RC955-962, Public aspects of medicine, RA1-1270

Abstract

In Latin America, Bothrops snakes account for most snake bites in humans, and the recommended treatment is administration of multispecific Bothrops antivenom (SAB--soro antibotrópico). However, Bothrops snakes are very diverse with regard to their venom composition, which raises the issue of which venoms should be used as immunizing antigens for the production of pan-specific Bothrops antivenoms. In this study, we simultaneously compared the composition and reactivity with SAB of venoms collected from six species of snakes, distributed in pairs from three distinct phylogenetic clades: Bothrops, Bothropoides and Rhinocerophis. We also evaluated the neutralization of Bothrops atrox venom, which is the species responsible for most snake bites in the Amazon region, but not included in the immunization antigen mixture used to produce SAB. Using mass spectrometric and chromatographic approaches, we observed a lack of similarity in protein composition between the venoms from closely related snakes and a high similarity between the venoms of phylogenetically more distant snakes, suggesting little connection between taxonomic position and venom composition. P-III snake venom metalloproteinases (SVMPs) are the most antigenic toxins in the venoms of snakes from the Bothrops complex, whereas class P-I SVMPs, snake venom serine proteinases and phospholipases A2 reacted with antibodies in lower levels. Low molecular size toxins, such as disintegrins and bradykinin-potentiating peptides, were poorly antigenic. Toxins from the same protein family showed antigenic cross-reactivity among venoms from different species; SAB was efficient in neutralizing the B. atrox venom major toxins. Thus, we suggest that it is possible to obtain pan-specific effective antivenoms for Bothrops envenomations through immunization with venoms from only a few species of snakes, if these venoms contain protein classes that are representative of all species to which the antivenom is targeted.

Published

2013

4. The antioxidant role of xanthurenic acid in the Aedes aegypti midgut during digestion of a blood meal.

Author

Vitor L A Lima, Felipe Dias, Rodrigo D Nunes, Luiza O Pereira, Tiago S R Santos, Luciana B Chiarini, Tadeu D Ramos, Bernardo J Silva-Mendes, Jonas Perales, Richard H Valente, and Pedro L Oliveira

Subjects

Medicine, Science

Abstract

In the midgut of the mosquito Aedes aegypti, a vector of dengue and yellow fever, an intense release of heme and iron takes place during the digestion of a blood meal. Here, we demonstrated via chromatography, light absorption and mass spectrometry that xanthurenic acid (XA), a product of the oxidative metabolism of tryptophan, is produced in the digestive apparatus after the ingestion of a blood meal and reaches milimolar levels after 24 h, the period of maximal digestive activity. XA formation does not occur in the White Eye (WE) strain, which lacks kynurenine hydroxylase and accumulates kynurenic acid. The formation of XA can be diminished by feeding the insect with 3,4-dimethoxy-N-[4-(3-nitrophenyl)thiazol-2-yl] benzenesulfonamide (Ro-61-8048), an inhibitor of XA biosynthesis. Moreover, XA inhibits the phospholipid oxidation induced by heme or iron. A major fraction of this antioxidant activity is due to the capacity of XA to bind both heme and iron, which occurs at a slightly alkaline pH (7.5-8.0), a condition found in the insect midgut. The midgut epithelial cells of the WE mosquito has a marked increase in occurrence of cell death, which is reversed to levels similar to the wild type mosquitoes by feeding the insects with blood supplemented with XA, confirming the protective role of this molecule. Collectively, these results suggest a new role for XA as a heme and iron chelator that provides protection as an antioxidant and may help these animals adapt to a blood feeding habit.

Published

2012

5. 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

6. Proteomics reveals disturbances in the immune response and energy metabolism of monocytes from patients with septic shock

Author

Giselle Villa Flor Brunoro, Helder I. Nakaya, Monique R.O. Trugilho, Patrícia T. Bozza, Richard H. Valente, Fernando A. Bozza, Pedro Mendes de Azambuja Rodrigues, and Mariana Araujo-Pereira

Subjects

0301 basic medicine, Male, Proteomics, Immunopathogenesis, Science, Immunology, Pathogenesis, Monocytes, Article, Proinflammatory cytokine, Sepsis, Cohort Studies, 03 medical and health sciences, 0302 clinical medicine, Immune system, Downregulation and upregulation, Immunopathology, medicine, Humans, Prospective Studies, Aged, Aged, 80 and over, Inflammation, Multidisciplinary, Septic shock, business.industry, Monocyte, Histocompatibility Antigens Class II, Immunity, PROTEÔMICA, Middle Aged, medicine.disease, Shock, Septic, 030104 developmental biology, medicine.anatomical_structure, Case-Control Studies, Cytokines, Medicine, Female, Immunocompetence, business, Energy Metabolism, Infection, 030217 neurology & neurosurgery

Abstract

Sepsis results from a dyshomeostatic response to infection, which may lead to hyper or hypoimmune states. Monocytes are central regulators of the inflammatory response, but our understanding of their role in the genesis and resolution of sepsis is still limited. Here, we report a comprehensive exploration of monocyte molecular responses in a cohort of patients with septic shock via proteomic profiling. The acute stage of septic shock was associated with an impaired inflammatory phenotype, indicated by the down-regulation of MHC class II molecules and proinflammatory cytokine pathways. Simultaneously, there was an up-regulation of glycolysis enzymes and a decrease in proteins related to the citric acid cycle and oxidative phosphorylation. On the other hand, the restoration of immunocompetence was the hallmark of recovering patients, in which an upregulation of interferon signaling pathways was a notable feature. Our results provide insights into the immunopathology of sepsis and propose that, pending future studies, immunometabolism pathway components could serve as therapeutic targets in septic patients.

Published

2021

7. Platelet proteome reveals features of cell death, antiviral response and viral replication in covid-19

Author

Monique R. O. Trugilho, Isaclaudia G. Azevedo-Quintanilha, João S. M. Gesto, Emilly Caroline S. Moraes, Samuel C. Mandacaru, Mariana M. Campos, Douglas M. Oliveira, Suelen S. G. Dias, Viviane A. Bastos, Marlon D. M. Santos, Paulo C. Carvalho, Richard H. Valente, Eugenio D. Hottz, Fernando A. Bozza, Thiago Moreno L. Souza, Jonas Perales, and Patrícia T. Bozza

Subjects

Cancer Research, Cellular and Molecular Neuroscience, Immunology, Cell Biology

Abstract

Coronavirus disease 2019 (COVID-19) has affected over 400 million people worldwide, leading to 6 million deaths. Among the complex symptomatology of COVID-19, hypercoagulation and thrombosis have been described to directly contribute to lethality, pointing out platelets as an important SARS-CoV-2 target. In this work, we explored the platelet proteome of COVID-19 patients through a label-free shotgun proteomics approach to identify platelet responses to infection, as well as validation experiments in a larger patient cohort. Exclusively detected proteins (EPs) and differentially expressed proteins (DEPs) were identified in the proteomic dataset and thus classified into biological processes to map pathways correlated with pathogenesis. Significant changes in the expression of proteins related to platelet activation, cell death, and antiviral response through interferon type-I were found in all patients. Since the outcome of COVID-19 varies highly among individuals, we also performed a cross-comparison of proteins found in survivors and nonsurvivors. Proteins belonging to the translation pathway were strongly highlighted in the nonsurvivor group. Moreover, the SARS-CoV-2 genome was fully sequenced in platelets from five patients, indicating viral internalization and preprocessing, with CD147 as a potential entry route. In summary, platelets play a significant role in COVID-19 pathogenesis via platelet activation, antiviral response, and disease severity.

Published

2022

8. DiagnoMass: A proteomics hub for pinpointing discriminative spectral clusters

Author

Marlon D.M. Santos, Amanda C. Camillo-Andrade, Diogo B. Lima, Tatiana A.C.B. Souza, Juliana de S. da G. Fischer, Richard H. Valente, Fabio C. Gozzo, Valmir C. Barbosa, Carlos Batthyany, Julia Chamot-Rooke, Rosario Duran, and Paulo C. Carvalho

Subjects

Biophysics, Biochemistry

Published

2023

9. Atrazine, desethylatrazine (DEA) and desisopropylatrazine (DIA) degradation by Pleurotus ostreatus INCQS 40310

Author

Keysson Vieira Fernandes, Julia Finamor Carvalho, Aline Ramalho Brandão Pereira, Raquel de Oliveira Lopes, Patrícia Maia Pereira, Manuela da Silva, Richard H. Valente, Viridiana Santana Ferreira-Leitão, and Alexandre da Silva de França

Subjects

0106 biological sciences, biology, 010405 organic chemistry, Sugar cane, Biodegradation, biology.organism_classification, 01 natural sciences, Biochemistry, Catalysis, 0104 chemical sciences, chemistry.chemical_compound, chemistry, 010608 biotechnology, Degradation (geology), Atrazine, Pleurotus ostreatus, Food science, Biotechnology

Abstract

Atrazine is the most common herbicide applied in crops of economic relevance, such as sugar cane, soybean, and corn. Atrazine and its derivatives desethylatrazine (DEA) and desisopropylatrazine (DI...

Published

2020

10. Glycolytic profile shift and antioxidant triggering in symbiont-free and H2O2-resistant Strigomonas culicis

Author

Richard H. Valente, Paulo C. Carvalho, Geovane Dias-Lopes, Jonas Perales, Giselle Villa Flor Brunoro, Vítor Ennes-Vidal, Claudia M. d’Avila-Levy, Rubem Figueiredo Sadok Menna-Barreto, and Ana Cristina S. Bombaça

Subjects

0301 basic medicine, Hexokinase, Chemistry, fungi, Metabolism, Oxidative phosphorylation, Pentose phosphate pathway, medicine.disease_cause, Biochemistry, 03 medical and health sciences, Aposymbiotic, chemistry.chemical_compound, 030104 developmental biology, 0302 clinical medicine, Gluconeogenesis, Physiology (medical), medicine, Glycolysis, 030217 neurology & neurosurgery, Oxidative stress

Abstract

During their life cycle, trypanosomatids are exposed to stress conditions and adapt their energy and antioxidant metabolism to colonize their hosts. Strigomonas culicis is a monoxenous protist found in invertebrates with an endosymbiotic bacterium that completes essential biosynthetic pathways for the trypanosomatid. Our research group previously generated a wild-type H2O2-resistant (WTR) strain that showed improved mitochondrial metabolism and antioxidant defenses, which led to higher rates of Aedes aegypti infection. Here, we assess the biological contribution of the S. culicis endosymbiont and reactive oxygen species (ROS) resistance to oxidative and energy metabolism processes. Using high-throughput proteomics, several proteins involved in glycolysis and gluconeogenesis, the pentose phosphate pathway and glutathione metabolism were identified. The results suggest that ROS resistance decreases glucose consumption and indicate that the metabolic products from gluconeogenesis are key to supplying the protist with high-energy and reducing intermediates. Our hypothesis was confirmed by biochemical assays showing opposite profiles for glucose uptake and hexokinase and pyruvate kinase activity levels in the WTR and aposymbiotic strains, while the enzyme glucose-6P 1-dehydrogenase was more active in both strains. Regarding the antioxidant system, ascorbate peroxidase has an important role in H2O2 resistance and may be responsible for the high infection rates previously described for A. aegypti. In conclusion, our data indicate that the energy-related and antioxidant metabolic processes of S. culicis are modulated in response to oxidative stress conditions, providing new perspectives on the biology of the trypanosomatid-insect interaction as well as on the possible impact of resistant parasites in accidental human infection.

Published

2020

11. Molecular Architecture of the Antiophidic Protein DM64 and its Binding Specificity to Myotoxin II From Bothrops asper Venom

Author

Barbara S. Soares, Surza Lucia G. Rocha, Viviane A. Bastos, Diogo B. Lima, Paulo C. Carvalho, Fabio C. Gozzo, Borries Demeler, Tayler L. Williams, Janelle Arnold, Amy Henrickson, Thomas J. D. Jørgensen, Tatiana A. C. B. Souza, Jonas Perales, Richard H. Valente, Bruno Lomonte, Francisco Gomes-Neto, and Ana Gisele C. Neves-Ferreira

Subjects

Veneno de serpiente, QH301-705.5, antiophidic activity, immunoglobulin fold, Biochemistry, Genetics and Molecular Biology (miscellaneous), Biochemistry, toxin neutralisation, protein inhibitor, cross-linking (XL), structural biology, Biology (General), Molecular Biology, snake envenomation, mass spectrometry

Abstract

DM64 is a toxin-neutralizing serum glycoprotein isolated from Didelphis aurita, an ophiophagous marsupial naturally resistant to snake envenomation. This 64 kDa antitoxin targets myotoxic phospholipases A2, which account for most local tissue damage of viperid snakebites. We investigated the noncovalent complex formed between native DM64 and myotoxin II, a myotoxic phospholipase-like protein from Bothrops asper venom. Analytical ultracentrifugation (AUC) and size exclusion chromatography indicated that DM64 is monomeric in solution and binds equimolar amounts of the toxin. Attempts to crystallize native DM64 for X-ray diffraction were unsuccessful. Obtaining recombinant protein to pursue structural studies was also challenging. Classical molecular modeling techniques were impaired by the lack of templates with more than 25% sequence identity with DM64. An integrative structural biology approach was then applied to generate a three-dimensional model of the inhibitor bound to myotoxin II. I-TASSER individually modeled the five immunoglobulin-like domains of DM64. Distance constraints generated by cross-linking mass spectrometry of the complex guided the docking of DM64 domains to the crystal structure of myotoxin II, using Rosetta. AUC, small-angle X-ray scattering (SAXS), molecular modeling, and molecular dynamics simulations indicated that the DM64-myotoxin II complex is structured, shows flexibility, and has an anisotropic shape. Inter-protein cross-links and limited hydrolysis analyses shed light on the inhibitor’s regions involved with toxin interaction, revealing the critical participation of the first, third, and fifth domains of DM64. Our data showed that the fifth domain of DM64 binds to myotoxin II amino-terminal and beta-wing regions. The third domain of the inhibitor acts in a complementary way to the fifth domain. Their binding to these toxin regions presumably precludes dimerization, thus interfering with toxicity, which is related to the quaternary structure of the toxin. The first domain of DM64 interacts with the functional site of the toxin putatively associated with membrane anchorage. We propose that both mechanisms concur to inhibit myotoxin II toxicity by DM64 binding. The present topological characterization of this toxin-antitoxin complex constitutes an essential step toward the rational design of novel peptide-based antivenom therapies targeting snake venom myotoxins. Fundação Oswaldo Cruz/[INOVA GC VPPCB-007-FIO-18-2-9]/Fiocruz/Brasil Fundação de Amparo à Pesquisa do Estado do Rio de Janeiro/[APQ1 E-6/010.001929/2019]/FAPERJ/Brasil Conselho Nacional de Desenvolvimento Científico e Tecnológico/[Universal 426290/2018-6]/CNPq/Brasil National Institutes of Health/[GM120600]/NIH/Estados Unidos National Science Foundation/[NSF-ACI-1339649]/NSF/Estados Unidos San Diego Supercomputer Center/[TG-MCB070039N]/SDSC/Estados Unidos Texas Advanced Computing Center/[TG457201]/TACC/Estados Unidos UCR::Vicerrectoría de Investigación::Unidades de Investigación::Ciencias de la Salud::Instituto Clodomiro Picado (ICP)

Published

2022

12. Revisiting Jatropha curcas Monomeric Esterase: A Dienelactone Hydrolase Compatible with the Electrostatic Catapult Model

Author

Deborah Antunes, Denise M. G. Freire, Richard H. Valente, Marcos Gustavo Araujo Schwarz, and Gabriela Coelho Brêda

Subjects

Models, Molecular, Proteomics, esterase, Cations, Divalent, Static Electricity, Jatropha curcas L, Jatropha, Biochemistry, Esterase, dienelactone hydrolase, Microbiology, Article, Substrate Specificity, Hydrolysis, Catalytic Domain, Catalytic triad, Organic chemistry, Amino Acid Sequence, Isoelectric Point, Molecular Biology, chemistry.chemical_classification, Analysis of Variance, biology, Chemistry, Esterases, Temperature, Stereoisomerism, Hydrogen-Ion Concentration, biology.organism_classification, QR1-502, Enzyme, Biocatalysis, Biodiesel production, Proteolysis, Solvents, Carboxylic Ester Hydrolases, Jatropha curcas, seed, Cysteine

Abstract

Jatropha curcas contains seeds with a high oil content, suitable for biodiesel production. After oil extraction, the remaining mass can be a rich source of enzymes. However, data from the literature describing physicochemical characteristics for a monomeric esterase from the J. curcas seed did not fit the electrostatic catapult model for esterases/lipases. We decided to reevaluate this J. curcas esterase and extend its characterization to check this apparent discrepancy and gain insights into the enzyme’s potential as a biocatalyst. After anion exchange chromatography and two-dimensional gel electrophoresis, we identified the enzyme as belonging to the dienelactone hydrolase family, characterized by a cysteine as the nucleophile in the catalytic triad. The enzyme displayed a basic optimum hydrolysis pH of 9.0 and an acidic pI range, in contrast to literature data, making it well in line with the electrostatic catapult model. Furthermore, the enzyme showed low hydrolysis activity in an organic solvent-containing medium (isopropanol, acetonitrile, and ethanol), which reverted when recovering in an aqueous reaction mixture. This enzyme can be a valuable tool for hydrolysis reactions of short-chain esters, useful for pharmaceutical intermediates synthesis, due to both its high hydrolytic rate in basic pH and its stability in an organic solvent.

Published

2021

13. Molecular Architecture of the Antiophidic Protein DM64 and its Binding Specificity to Myotoxin II From

Author

Barbara S, Soares, Surza Lucia G, Rocha, Viviane A, Bastos, Diogo B, Lima, Paulo C, Carvalho, Fabio C, Gozzo, Borries, Demeler, Tayler L, Williams, Janelle, Arnold, Amy, Henrickson, Thomas J D, Jørgensen, Tatiana A C B, Souza, Jonas, Perales, Richard H, Valente, Bruno, Lomonte, Francisco, Gomes-Neto, and Ana Gisele C, Neves-Ferreira

Abstract

DM64 is a toxin-neutralizing serum glycoprotein isolated from

Published

2021

14. Leveraging the partition selection bias to achieve a high-quality clustering of mass spectra

Author

Diogo B. Lima, Richard H. Valente, Julia Chamot-Rooke, Mathieu Dupré, Louise U. Kurt, André R.F. Silva, Carolina Alves Nicolau, Marlon D.M. Santos, Paulo C. Carvalho, Valmir C. Barbosa, Fiocruz Paraná - Instituto Carlos Chagas / Carlos Chagas Institute [Curitiba, Brésil] (ICC), Fundação Oswaldo Cruz / Oswaldo Cruz Foundation (FIOCRUZ), Réseau International des Instituts Pasteur (RIIP)-Réseau International des Instituts Pasteur (RIIP), Leibniz Forschungsinstitut für Molekulare Pharmakolgie = Leibniz Institute for Molecular Pharmacology [Berlin, Allemagne] (FMP), Leibniz Association, Spectrométrie de Masse pour la Biologie – Mass Spectrometry for Biology (UTechS MSBio), Institut Pasteur [Paris] (IP)-Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS)-Université Paris Cité (UPCité), Instituto Oswaldo Cruz / Oswaldo Cruz Institute [Rio de Janeiro] (IOC), Centre de Recherche en Cancérologie et Immunologie Nantes-Angers (CRCINA), Université d'Angers (UA)-Université de Nantes (UN)-Institut National de la Santé et de la Recherche Médicale (INSERM)-Centre National de la Recherche Scientifique (CNRS)-Centre hospitalier universitaire de Nantes (CHU Nantes), Instituto Alberto Luiz Coimbra de Pós-Graduação e Pesquisa de Engenharia (COPPE-UFRJ), Universidade Federal do Rio de Janeiro (UFRJ), Universidade Federal do Estado do Rio de Janeiro (UNIRIO), A.R.F.S., L.U.K., M.D.M.S. and V.C.B. acknowledge support from Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES). A.R.F.S. acknowledges Instituto Carlos Chagas (ICC). D.B.L., M.D. and J.C.R. acknowledge Institut Pasteur, CNRS, the Agence Nationale de la Recherche (project ANR-15-CE18-0021) and the European Joint Programme One Health EJP from the European Union's Horizon 2020 research and innovation programme (Grant Agreement 773830) for financial support. R.H.V., V.C.B. and P.C.C. acknowledge support from Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq). V.C.B. acknowledges a BBP grant from Fundação Carlos Chagas Filho de Amparo à Pesquisa do Estado do Rio de Janeiro (FAPERJ)., ANR-15-CE18-0021,PathoTOP,Identification rapide de pathogènes bactériens par protéomique top-down en contexte clinique(2015), European Project: 773830, H2020-SFS-2017-1 ,One Health EJP(2018), Fundação Oswaldo Cruz (FIOCRUZ), Institut Pasteur [Paris]-Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS), Institut National de la Santé et de la Recherche Médicale (INSERM)-Université de Nantes - UFR de Médecine et des Techniques Médicales (UFR MEDECINE), and Université de Nantes (UN)-Université de Nantes (UN)-Centre hospitalier universitaire de Nantes (CHU Nantes)-Centre National de la Recherche Scientifique (CNRS)-Université d'Angers (UA)

Subjects

Proteomics, 0301 basic medicine, MESH: Databases, Protein, Process (engineering), Computer science, media_common.quotation_subject, [SDV]Life Sciences [q-bio], Biophysics, Context (language use), MESH: Algorithms, computer.software_genre, Biochemistry, Measure (mathematics), Clustering, 03 medical and health sciences, MESH: Selection Bias, MESH: Software, Tandem Mass Spectrometry, Tandem mass spectra, [SDV.BBM.GTP]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Genomics [q-bio.GN], Cluster Analysis, Databases, Protein, Cluster analysis, Selection Bias, media_common, Selection bias, 030102 biochemistry & molecular biology, Partition assessment tool, MESH: Proteomics, MESH: Tandem Mass Spectrometry, Partition (database), MESH: Cluster Analysis, Identification (information), 030104 developmental biology, ComputingMethodologies_PATTERNRECOGNITION, Noise (video), Data mining, [INFO.INFO-BI]Computer Science [cs]/Bioinformatics [q-bio.QM], computer, Algorithms, Software

Abstract

International audience; In proteomics, the identification of peptides from mass spectral data can be mathematically described as the partitioning of mass spectra into clusters (i.e., groups of spectra derived from the same peptide). The way partitions are validated is just as important, having evolved side by side with the clustering algorithms themselves and given rise to many partition assessment measures. An assessment measure is said to have a selection bias if, and only if, the probability that a randomly chosen partition scoring a high value depends on the number of clusters in the partition. In the context of clustering mass spectra, this might mislead the validation process to favor clustering algorithms that generate too many (or few) spectral clusters, regardless of the underlying peptide sequence. A selection bias toward the number of peptides is desirable for proteomics as it estimates the number of peptides in a complex protein mixture. Here, we introduce an assessment measure that is purposely biased toward the number of peptide ion species. We also introduce a partition assessment framework for proteomics, called the Partition Assessment Tool, and demonstrate its importance by evaluating the performance of eight clustering algorithms on seven proteomics datasets while discussing the trade-offs involved. SIGNIFICANCE: Clustering algorithms are widely adopted in proteomics for undertaking several tasks such as speeding up search engines, generating consensus mass spectra, and to aid in the classification of proteomic profiles. Choosing which algorithm is most fit for the task at hand is not simple as each algorithm has advantages and disadvantages; furthermore, specifying clustering parameters is also a necessary and fundamental step. For example, deciding on whether to generate "pure clusters" or fewer clusters but accepting noise. With this as motivation, we verify the performance of several widely adopted algorithms on proteomic datasets and introduce a theoretical framework for drawing conclusions on which approach is suitable for the task at hand.

Published

2021

15. 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

16. Trypanosoma cruzi immunoproteome: Calpain-like CAP5.5 differentially detected throughout distinct stages of human Chagas disease cardiomyopathy

Author

Rubem F. S. Menna-Barreto, Silvia Marinho Martins, Marcelle Almeida Caminha, Wilson Alves de Oliveira Junior, Virgínia Maria Barros de Lorena, Jonas Perales, Maria da Glória Aureliano de Melo Cavalcanti, Diogo B. Lima, Richard H. Valente, and Paulo C. Carvalho

Subjects

Chagas Cardiomyopathy, Male, 0301 basic medicine, Chagas disease, Trypanosoma cruzi, Protozoan Proteins, Biophysics, Cardiomyopathy, Antibodies, Protozoan, Disease, Biochemistry, Asymptomatic, Epitope, Pathogenesis, 03 medical and health sciences, medicine, Humans, 030102 biochemistry & molecular biology, biology, Calpain, business.industry, medicine.disease, biology.organism_classification, 030104 developmental biology, Immunoglobulin G, Immunology, biology.protein, Female, medicine.symptom, Antibody, business

Abstract

Chagas disease, caused by the protozoan Trypanosoma cruzi, affects millions of people worldwide, especially in Latin America. Approximately 30% of the cases evolve to the chronic symptomatic stage due to cardiac and/or digestive damage, generally accompanied by nervous system impairment. Given the higher frequency and severity of clinical manifestations related to cardiac tissue lesion, the goal of this study was the identification of proteins associated with the disease progression towards its cardiac form. Thus, T. cruzi bloodstream trypomastigotes proteins were submitted to immunoprecipitation using antibodies from patients with the asymptomatic or cardiac (stages B1 and C) forms of the disease and from healthy donors as control. Immunoreactive proteins were identified and quantified based on mass spectrometry analysis and shifts in the recognition profile were further evaluated. Compared to asymptomatic samples, IgG from stage C patients predominantly detected the I/6 autoantigen, whereas IgG from B1 patients resulted in higher yield of dihydrolipoamide acetyltransferase precursor, calpain cysteine peptidase, and two variants of CAP5.5. In this work, CAP5.5 recognition by serum immunoglobulin from patients with early cardiomyopathy generated a 23-fold abundance variation when compared to samples from asymptomatic patients, highlighting the participation of this protein in cardiac form progression of the disease. SIGNIFICANCE: While T. cruzi has become the major cause of infectious cardiomyopathy in Latin America, research groups have been struggling to find alternative treatment, vaccine candidates, and improved diagnostic tests. In addition, the absence of adequate biomarkers to assess cure and progression of disease is a major setback for clinical trials and patients monitoring. Therefore, our findings may contribute to a better understanding of T. cruzi pathogenesis and evaluation of suitable candidates for vaccine and diagnostic tests, besides the clinical applicability of the potential biomarkers for patient follow-up and prognosis. Finally, the identification of T. cruzi proteins recognized by IgG from healthy donors may contribute for the understanding and discovery of epitope conservation among a broad range of pathogens.

Published

2019

17. SARS-CoV-2 proteins bind heme and hemoglobin

Author

Thiago M De-Simone, Suelen da Silva Gomes Dias, Richard H. Valente, Guilherme Curty Lechuga, Carlos Roberto Alves, Monique Ramos de Oliveira Trugilho, Mirian Claudia de Souza Pereira, Franklin Souza-Silva, Natalia Fintelman-Rodrigues, Jairo Ramos Temerozzo, Paloma Napoleão-Pêgo, Salvatore G. De-Simone, Carolina de Queiroz Sacramento, Nicolas Carels, and David William Provance-Jr

Subjects

chemistry.chemical_compound, chemistry, Membrane protein, Viral replication, viruses, Vero cell, Shotgun proteomics, Heme, Virology, Virus, Hemin, Nucleoprotein

Abstract

The coronavirus disease 2019 (COVID-19) pandemic, caused by severe acute respiratory syndrome virus 2 (SARS-CoV-2), has led to a global crisis that included collapsing healthcare systems and shut-down communities, producing considerable economic burden. Despite the number of effective vaccines quickly implemented, the emergence of new variants is a primary concern. The scientific community undertook a rapid response to better study this new virus. However, critical questions about viral protein-protein interactions and mechanisms of its physiopathology are still unclear. Although severe COVID-19 was associated with hematological dysfunctions, scarce experimental data were produced about iron dysmetabolism and the viral proteins’ possible interaction with hemoglobin (Hb) chains. This work demonstrates the binding of SARS-CoV-2 proteins to hemin and Hb using a multimethodological approach. In silico analysis indicated binding motifs between a cavity in the viral nucleoprotein and hemoglobin’s porphyrin coordination region. Different hemin binding capacities of mock and SARS-CoV-2-infected culture extracts were noticed using gel electrophoresis and TMB staining. Hemin-binding proteins were isolated from SARS-CoV-2-infected cells by affinity chromatography and identified by shotgun proteomics, indicating that structural (nucleoprotein, spike, and membrane protein) and non-structural (Nsp3 and Nsp7) viral proteins interact with hemin. In vitro analyses of virus adsorption to host cells and viral replication studies in Vero cells demonstrated inhibitory activities - at different levels - by hemin, protoporphyrin IX (PpIX) Hb. Strikingly, free Hb at 1μM suppressed viral replication (99 %), and its interaction with SARS-CoV-2 was localized to the RBD region of the Spike protein. The findings showed clear evidence of new avenues to disrupt viral replication and understand virus physiopathology that warrants further investigation.

Published

2021

18. Beyond Melanin: Proteomics Reveals Virulence-Related Proteins in Paracoccidioides brasiliensis and Paracoccidioides lutzii Yeast Cells Grown in the Presence of L-Dihydroxyphenylalanine

Author

Leticia Andrade Mendes Marmello, Célia Maria de Almeida Soares, Monique R.O. Trugilho, Joshua D. Nosanchuk, Marcos de Abreu Almeida, Rodrigo Almeida-Paes, Richard H. Valente, Lilian Cristiane Baeza, and Rosely Maria Zancopé-Oliveira

Subjects

Microbiology (medical), L-dihydroxyphenylalanine, Quantitative proteomics, Virulence, Plant Science, Proteomics, Paracoccidioides, Article, Microbiology, 03 medical and health sciences, proteomics, lcsh:QH301-705.5, Pathogen, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Paracoccidioides brasiliensis, 0303 health sciences, biology, 030306 microbiology, biology.organism_classification, Yeast, melanin, Bacterial adhesin, virulence, lcsh:Biology (General), metabolism

Abstract

Species of the genus Paracoccidioides cause a systemic infection in human patients. Yeast cells of Paracoccidioides spp. produce melanin in the presence of L-dihydroxyphenylalanine and during infection, which may impact the pathogen&rsquo, s survival in the host. To better understand the metabolic changes that occur in melanized Paracoccidioides spp. cells, a proteomic approach was performed to compare melanized and non-melanized Paracoccidioides brasiliensis and Paracoccidioides lutzii yeast cells. Melanization was induced using L-dihydroxyphenylalanine as a precursor, and quantitative proteomics were performed using reversed-phase nano-chromatography coupled to high-resolution mass spectrometry. When comparing melanized versus non-melanized cells, 1006 and 582 differentially abundant/detected proteins were identified for P. brasiliensis and P. lutzii, respectively. Functional enrichment and comparative analysis revealed 30 important KEGG (Kyoto Encyclopedia of Genes and Genomes) pathways in melanized P. brasiliensis and 18 in P. lutzii, while differentially abundant proteins from non-melanized cells from these species were involved in 21 and 25 enriched pathways, respectively. Melanized cells presented an abundance of additional virulence-associated proteins, such as phospholipase, proteases, superoxide dis-mutases, heat-shock proteins, adhesins, and proteins related to vesicular transport. The results suggest that L-dihydroxyphenylalanine increases the virulence of Paracoccidioides spp. through complex mechanisms involving not only melanin but other virulence factors as well.

Published

2020

19. Immunoproteomics Reveals Pathogen’s Antigens Involved in Homo sapiens–Histoplasma capsulatum Interaction and Specific Linear B-Cell Epitopes in Histoplasmosis

Author

Marcos de Abreu Almeida, Rodrigo Almeida-Paes, Richard H. Valente, Célia Maria de Almeida Soares, Allan J. Guimarães, and Rosely Maria Zancopé-Oliveira

Subjects

0301 basic medicine, Microbiology (medical), M antigen, Antigens, Fungal, immunoproteome, Histoplasma, 030106 microbiology, Immunology, lcsh:QR1-502, Virulence, HIV Infections, Microbiology, Immunoproteomics, Histoplasmosis, Epitope, lcsh:Microbiology, Serology, 03 medical and health sciences, Cellular and Infection Microbiology, Immune system, Antigen, medicine, Humans, Original Research, mass spectrometry, YPS-3, Homo sapiens, biology, catalase P, epitopes, medicine.disease, Virology, Histoplasma capsulatum, 030104 developmental biology, Infectious Diseases, biology.protein, Epitopes, B-Lymphocyte, Antibody

Abstract

Histoplasmosis is one of the most frequent systemic mycosis in HIV patients. In these patients, histoplasmosis has high rates of morbidity/mortality if diagnosis and treatment are delayed. Despite its relevance, there is a paucity of information concerning the interaction between Histoplasma capsulatum and the human host, especially regarding the B-cell response, which has a direct impact on the diagnosis. Culture-based “gold-standard” methods have limitations, making immunodiagnostic tests an attractive option for clinical decisions. Despite the continuous development of those tests, improving serological parameters is necessary to make these methods efficient tools for definitive diagnosis of histoplasmosis. This includes the determination of more specific and immunogenic antigens to improve specificity and sensitivity of assays. In this study, we performed a co-immunoprecipitation assay between a protein extract from the yeast form of H. capsulatum and pooled sera from patients with proven histoplasmosis, followed by shotgun mass spectrometry identification of antigenic targets. Sera from patients with other pulmonary infections or from healthy individuals living in endemic areas of histoplasmosis were also assayed to determine potentially cross-reactive proteins. The primary structures of H. capsulatum immunoprecipitated proteins were evaluated using the DNAStar Protean 7.0 software. In parallel, the online epitope prediction server, BCPREDS, was used to complement the B-epitope prediction analysis. Our approach detected 132 reactive proteins to antibodies present in histoplasmosis patients’ sera. Among these antigens, 127 were recognized also by antibodies in heterologous patients’ and/or normal healthy donors’ sera. Therefore, the only three antigens specifically recognized by antibodies of histoplasmosis patients were mapped as potential antigenic targets: the M antigen, previously demonstrated in the diagnosis of histoplasmosis, and the catalase P and YPS-3 proteins, characterized as virulence factors of H. capsulatum, with antigenic properties still unclear. The other two proteins were fragments of the YPS-3 and M antigen. Overlapping results obtained from the two aforementioned bioinformatic tools, 16 regions from these three proteins are proposed as putative B-cell epitopes exclusive to H. capsulatum. These data reveal a new role for these proteins on H. capsulatum interactions with the immune system and indicate their possible use in new methods for the diagnosis of histoplasmosis.

Published

2020

20. The interaction between the natural metalloendopeptidase inhibitor BJ46a and its target toxin jararhagin analyzed by structural mass spectrometry and molecular modeling

Author

Viviane A. Bastos, Jonas Perales, Richard H. Valente, Surza Lucia Gonçalves da Rocha, Ana G.C. Neves-Ferreira, Francisco Gomes-Neto, and André Teixeira-Ferreira

Subjects

0301 basic medicine, Bothrops jararaca, 030102 biochemistry & molecular biology, biology, Chemistry, Antivenom, Biophysics, Metalloendopeptidases, Venom, Computational biology, biology.organism_classification, complex mixtures, Biochemistry, Mass Spectrometry, 03 medical and health sciences, 030104 developmental biology, Docking (molecular), Snake venom, Jararhagin, Crotalid Venoms, Metalloendopeptidase, Animals, Bothrops, Envenomation

Abstract

Snakebite envenoming affects millions of people worldwide, being officially considered a neglected tropical disease by the World Health Organization. The antivenom is effective in neutralizing the systemic effects of envenomation, but local effects are poorly neutralized, often leading to permanent disability. The natural resistance of the South American pit viper Bothrops jararaca to its venom is partly attributed to BJ46a, a natural snake venom metalloendopeptidase inhibitor. Upon complex formation, BJ46a binds non-covalently to the metalloendopeptidase, rendering it unable to exert its proteolytic activity. However, the structural features that govern this interaction are largely unknown. In this work, we applied structural mass spectrometry techniques (cross-linking-MS and hydrogen-deuterium exchange MS) and in silico analyses (molecular modeling, docking, and dynamics simulations) to understand the interaction between BJ46a and jararhagin, a metalloendopeptidase from B. jararaca venom. We explored the distance restraints generated from XL-MS experiments to guide the modeling of BJ46a and jararhagin, as well as the protein-protein docking simulations. HDX-MS data pinpointed regions of protection/deprotection at the interface of the BJ46a-jararhagin complex which, in addition to the molecular dynamics simulation data, reinforced our proposed interaction model. Ultimately, the structural understanding of snake venom metalloendopeptidases inhibition by BJ46a could lead to the rational design of drugs to improve anti-snake venom therapeutics, alleviating the high morbidity rates currently observed.

Published

2020

21. Bothrops jararaca accessory venom gland is an ancillary source of toxins to the snake

Author

Inácio de L. Junqueira-de-Azevedo, Leonardo Sanches, José Antonio Portes-Junior, Ana Maria Moura-da-Silva, Luciana Godoy Viana, Ursula Castro de Oliveira, Milton Yutaka Nishiyama-Junior, Richard H. Valente, Milene Schmidt Luna, Norma Yamanouye, Jonas Perales, and Patricia Bianca Clissa

Subjects

0301 basic medicine, Proteome, Phospholipase A2 Inhibitors, Biophysics, Venom, Phospholipase, complex mixtures, Biochemistry, 03 medical and health sciences, Exocrine Glands, Phospholipase A2, stomatognathic system, Cysteine-rich secretory protein, Viperidae, biology.animal, Crotalid Venoms, Animals, Bothrops, Secretion, Metalloproteinase, 030102 biochemistry & molecular biology, biology, Gene Expression Profiling, Lectin, Phospholipases A2, 030104 developmental biology, Metalloproteases, biology.protein

Abstract

In Viperidae snakes, it has been attributed to the main venom gland, a component of the venom gland apparatus, the function of synthesizing all venom toxins and storing them inside a basal-central lumen. However, the role of the accessory gland is still unknown. Here, we analyzed the proteome and the transcriptome of the accessory gland during venom production and secretion cycle. We showed that the accessory gland expresses and synthesizes toxins that are similar to those produced by the main venom gland such as C-type lectin/C-type lectin-like proteins, metalloproteinase, phospholipase A2, cysteine rich secretory protein, nerve growth factor, vascular endothelial growth factor, serine proteinase, and l -amino acid oxidase. Our data have shown that toxin synthesis in the accessory gland is asynchronous when compared to the same process in the venom gland. Moreover, this gland also expresses inhibitors of venom phospholipases A2 and metalloproteinases. Transcriptome analysis showed that the transcripts that correspond to toxins in the accessory gland have a good correlation to the main venom gland transcripts. Therefore, it is proposed that the accessory gland is an ancillary source of toxins to the snake, and provides inhibitors that could control venom toxicity (and integrity) during storage. Significance In this study, we propose that the accessory venom gland acts as an important ancillary source of toxins to the snake, in lieu of a depleted main venom gland, and provides inhibiting agents that control venom toxicity (and integrity) during its storage.

Published

2018

22. SARS-CoV-2 Proteins Bind to Hemoglobin and Its Metabolites

Author

Carolina de Queiroz Sacramento, Mirian Claudia de Souza Pereira, Thiago Moreno L. Souza, David W. Provance, Guilherme Curty Lechuga, Paloma Napoleão-Pêgo, Jairo R. Temerozo, Franklin Souza-Silva, Richard H. Valente, Monique Ramos de Oliveira Trugilho, Salvatore G. De-Simone, Suelen da Silva Gomes Dias, Natalia Fintelman-Rodrigues, Carlos R Alves, and Nicolas Carels

Subjects

Proteomics, Nsp7, QH301-705.5, viruses, Nsp3, Protein domain, Protoporphyrins, Virus Attachment, Plasma protein binding, Viral Nonstructural Proteins, Virus Replication, Article, Catalysis, RBD, Inorganic Chemistry, Hemoglobins, chemistry.chemical_compound, Protein Domains, Affinity chromatography, Humans, Biology (General), Physical and Theoretical Chemistry, Shotgun proteomics, QD1-999, Molecular Biology, Heme, Spectroscopy, Viral Structural Proteins, protein–protein binding, SARS-CoV-2, Chemistry, Organic Chemistry, COVID-19, General Medicine, hemoglobin, Computer Science Applications, Nucleoprotein, Molecular Docking Simulation, Biochemistry, Hemin, Hemoglobin, Protein Binding

Abstract

(1) Background: coronavirus disease 2019 (COVID-19), caused by severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), has been linked to hematological dysfunctions, but there are little experimental data that explain this. Spike (S) and Nucleoprotein (N) proteins have been putatively associated with these dysfunctions. In this work, we analyzed the recruitment of hemoglobin (Hb) and other metabolites (hemin and protoporphyrin IX-PpIX) by SARS-Cov2 proteins using different approaches. (2) Methods: shotgun proteomics (LC–MS/MS) after affinity column adsorption identified hemin-binding SARS-CoV-2 proteins. The parallel synthesis of the peptides technique was used to study the interaction of the receptor bind domain (RBD) and N-terminal domain (NTD) of the S protein with Hb and in silico analysis to identify the binding motifs of the N protein. The plaque assay was used to investigate the inhibitory effect of Hb and the metabolites hemin and PpIX on virus adsorption and replication in Vero cells. (3) Results: the proteomic analysis by LC–MS/MS identified the S, N, M, Nsp3, and Nsp7 as putative hemin-binding proteins. Six short sequences in the RBD and 11 in the NTD of the spike were identified by microarray of peptides to interact with Hb and tree motifs in the N protein by in silico analysis to bind with heme. An inhibitory effect in vitro of Hb, hemin, and PpIX at different levels was observed. Strikingly, free Hb at 1mM suppressed viral replication (99%), and its interaction with SARS-CoV-2 was localized into the RBD region of the spike protein. (4) Conclusions: in this study, we identified that (at least) five proteins (S, N, M, Nsp3, and Nsp7) of SARS-CoV-2 recruit Hb/metabolites. The motifs of the RDB of SARS-CoV-2 spike, which binds Hb, and the sites of the heme bind-N protein were disclosed. In addition, these compounds and PpIX block the virus’s adsorption and replication. Furthermore, we also identified heme-binding motifs and interaction with hemin in N protein and other structural (S and M) and non-structural (Nsp3 and Nsp7) proteins.

Published

2021

23. Functional proteomic analyses of Bothrops atrox venom reveals phenotypes associated with habitat variation in the Amazon

Author

Ana Maria Moura-da-Silva, Milton Y. Nishiyama, Carolina A. Nicolau, José Antonio Portes-Junior, Richard H. Valente, Hipócrates de Menezes Chalkidis, Leijiane F. Sousa, Juliana L. Bernardoni, Diana R. Amazonas, Rosa Helena Veras Mourão, and Luciana A. Freitas-de-Sousa

Subjects

Proteomics, 0301 basic medicine, Gene isoform, In silico, Antivenom, Biophysics, Zoology, Venom, Biology, complex mixtures, Biochemistry, Intraspecific competition, Transcriptome, 03 medical and health sciences, Exocrine Glands, Crotalid Venoms, Animals, Bothrops, Ecosystem, 030102 biochemistry & molecular biology, Ecology, biology.organism_classification, Phenotype, 030104 developmental biology, Brazil

Abstract

Venom variability is commonly reported for venomous snakes including Bothrops atrox. Here, we compared the composition of venoms from B. atrox snakes collected at Amazonian conserved habitats (terra-firme upland forest and varzea) and human modified areas (pasture and degraded areas). Venom samples were submitted to shotgun proteomic analysis as a whole or compared after fractionation by reversed-phase chromatography. Whole venom proteomes revealed a similar composition among the venoms with predominance of SVMPs, CTLs, and SVSPs and intermediate amounts of PLA2s and LAAOs. However, when distribution of particular isoforms was analyzed by either method, the venom from varzea snakes showed a decrease in hemorrhagic SVMPs and an increase in SVSPs, and procoagulant SVMPs and PLA2s. These differences were validated by experimental approaches including both enzymatic and in vivo assays, and indicated restrictions in respect to antivenom efficacy to variable components. Thus, proteomic analysis at the isoform level combined to in silico prediction of functional properties may indicate venom biological activity. These results also suggest that the prevalence of functionally distinct isoforms contributes to the variability of the venoms and could reflect the adaptation of B. atrox to distinct prey communities in different Amazon habitats. Biological significance In this report, we compared isoforms present in venoms from snakes collected at different Amazonian habitats. By means of a species venom gland transcriptome and the in silico functional prediction of each isoform, we were able to predict the principal venom activities in vitro and in animal models. We also showed remarkable differences in the venom pools from snakes collected at the floodplain (varzea habitat) compared to other habitats. Not only was this venom less hemorrhagic and more procoagulant, when compared to the venom pools from the other three habitats studied, but also this enhanced procoagulant activity was not efficiently neutralized by Bothrops antivenom. Thus, using a functional proteomic approach, we highlighted intraspecific differences in B. atrox venom that could impact both in the ecology of snakes but also in the treatment of snake bite patients in the region.

Published

2017

24. Screening for target toxins of the antiophidic protein DM64 through a gel-based interactomics approach

Author

Jonas Perales, Yamileth Angulo, Surza Lucia Gonçalves da Rocha, Bruno Lomonte, Gilberto B. Domont, Monique R.O. Trugilho, Ana G.C. Neves-Ferreira, and Richard H. Valente

Subjects

Proteomics, 0301 basic medicine, Snake venom, Myotoxin, Antivenom, Biophysics, Venom, Bioinformatics, complex mixtures, Biochemistry, Chromatography, Affinity, Phospholipases A, 03 medical and health sciences, Species Specificity, Affinity chromatography, Tandem Mass Spectrometry, Crotalid Venoms, Animals, Electrophoresis, Gel, Two-Dimensional, Interactomics, Toxins, Biological, Gel electrophoresis, biology, Chemistry, Myotoxin inhibitor, Crotalus, Blood Proteins, biology.organism_classification, 030104 developmental biology, Didelphis aurita, Bothrops, Protein Binding

Abstract

DM64 is a glycosylated protein with antivenomactivity isolated fromthe serum of the opossumDidelphis aurita. It binds non-covalently to myotoxins I (Asp49) and II (Lys49) from Bothrops asper venom and inhibits their myotoxic effect. In this study, an affinity columnwith immobilizedDM64 as baitwas used to fish potential target toxins. All ten isolated myotoxins tested were able to effectively bind to the DM64 column. To better access the specificity of the inhibitor, crude venoms from Bothrops (8 species), Crotalus (2 species) and Naja naja atra were submitted to the affinity purification. Venom fractions bound and nonbound to the DM64 columnwere analyzed by two-dimensional gel electrophoresis andMALDI-TOF/TOFMS. Although venomfractions bound to the column were mainly composed of basic PLA2, a few spots corresponding to acidic PLA2 were also observed. Some unexpected protein spotswere also identified: C-type lectins and CRISPmay represent putative new targets forDM64, whereas the presence of serine peptidases in the venom bound fraction is likely a consequence of nonspecific binding to the column matrix. The present results contribute to better delineate the inhibitory potential of DM64, providing a framework for the development of more specific antivenom therapies. Biological significance: Local tissue damage induced bymyotoxic PLA2 remains a serious consequence of snake envenomation, since it is only partially neutralized by traditional antivenom serotherapy. Myotoxin inhibition by highly specific molecules offers great promise in the treatment of snakebites, a health problemlargely neglected by governments and pharmaceutical industries. Bioactive compounds such as DM64 can represent a valuable source of scaffolds for drug development in this area. The present study has systematically profiled the binding specificity of DM64 toward a variety of snake venom toxin classes and therefore can lead to a better understanding of the structure-function relationship of this important antivenom protein. Fundação Oswaldo Cruz:uma instituição a serviço da visto/[RPT02A]/FIOCRUZ/Brasil Fundação Oswaldo Cruz:uma instituição a serviço da visto/[RPT02B]/FIOCRUZ/Brasil Conselho Nacional de Desenvolvimento Científico e Tecnológico/[400147 / 2014-4]/CNPq/Brasil Fundação de Amparo à Pesquisa do Estado do Rio de Janeiro/[E-26 / 102.807 / 2012-BBP]/FAPERJ/Brasil Coordenação de Aperfeiçoamento de Pessoal de Nível Superior/[23038.006270 / 2011-63]/CAPES/Brasil UCR::Vicerrectoría de Investigación::Unidades de Investigación::Ciencias de la Salud::Instituto Clodomiro Picado (ICP)

Published

2017

25. Quantitative Proteomic Map of the Trypanosomatid Strigomonas culicis: The Biological Contribution of its Endosymbiotic Bacterium

Author

Marcos Catanho, Claudia M. d’Avila-Levy, Rubem F. S. Menna-Barreto, Paulo C. Carvalho, Veit Schwämmle, Giselle Villa Flor Brunoro, Maria Cristina M. Motta, Ana Tereza Ribeiro de Vasconcelos, Jonas Perales, Carolina Boucinha, Diogo B. Lima, Richard H. Valente, Aline dos Santos Garcia-Gomes, Monique R.O. Trugilho, and André Teixeira-Ferreira

Subjects

0301 basic medicine, Symbiogenesis, Proteome, Biology, medicine.disease_cause, Proteomics, Bacterial Physiological Phenomena, Microbiology, amino acid and protein syntheses, 03 medical and health sciences, Aposymbiotic, Strigomonas culicis, proteomics, protein folding, Organelle, energy metabolism, medicine, Protein biosynthesis, Shotgun proteomics, Symbiosis, Amino acid synthesis, Genetics, chemistry.chemical_classification, fungi, Protist, 030108 mycology & parasitology, endosymbiont-bearing trypanosomatid, 030104 developmental biology, chemistry, Trypanosomatina

Abstract

Strigomonas culicis is a kinetoplastid parasite of insects that maintains a mutualistic association with an intracellular symbiotic bacterium, which is highly integrated into the protist metabolism: it furnishes essential compounds and divides in synchrony with the eukaryotic nucleus. The protist, conversely, can be cured of the endosymbiont, producing an aposymbiotic cell line, which presents a diminished ability to colonize the insect host. This obligatory association can represent an intermediate step of the evolution towards the formation of an organelle, therefore representing an interesting model to understand the symbiogenesis theory. Here, we used shotgun proteomics to compare the S. culicis endosymbiont-containing and aposymbiotic strains, revealing a total of 11,305 peptides, and up to 2,213 proteins (2,029 and 1,452 for wild type and aposymbiotic, respectively). Gene ontology associated to comparative analysis between both strains revealed that the biological processes most affected by the elimination of the symbiont were the amino acid synthesis, as well as protein synthesis and folding. This large-scale comparison of the protein expression in S. culicis marks a step forward in the comprehension of the role of endosymbiotic bacteria in monoxenous trypanosomatid biology, particularly because trypanosomatids expression is mostly post-transcriptionally regulated.

Published

2019

26. Differential proteomic comparison of breast cancer secretome using a quantitative paired analysis workflow

Author

Jonas Perales, Claudia Vitoria de Moura Gallo, Dante Pagnoncelli, Richard H. Valente, Paulo C. Carvalho, Giselle Villa Flor Brunoro, Valmir C. Barbosa, René P. Zahedi, and Ana G.C. Neves-Ferreira

Subjects

Proteomics, 0301 basic medicine, Cancer Research, Proteome, Breast Neoplasms, Biology, lcsh:RC254-282, Workflow, 03 medical and health sciences, Breast cancer, 0302 clinical medicine, Platelet degranulation, Paired analysis, Biomarkers, Tumor, Tumor Microenvironment, Genetics, medicine, Humans, Liquid biopsy, Aged, Aged, 80 and over, Nipple aspirate fluid, Tumor microenvironment, Cancer, Middle Aged, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, Prognosis, medicine.disease, Warburg effect, 030104 developmental biology, Oncology, Case-Control Studies, 030220 oncology & carcinogenesis, Cancer research, Female, Breast secretion, Research Article, Follow-Up Studies

Abstract

Background Worldwide, breast cancer is the main cause of cancer mortality in women. Most cases originate in mammary ductal cells that produce the nipple aspirate fluid (NAF). In cancer patients, this secretome contains proteins associated with the tumor microenvironment. NAF studies are challenging because of inter-individual variability. We introduced a paired-proteomic shotgun strategy that relies on NAF analysis from both breasts of patients with unilateral breast cancer and extended PatternLab for Proteomics software to take advantage of this setup. Methods The software is based on a peptide-centric approach and uses the binomial distribution to attribute a probability for each peptide as being linked to the disease; these probabilities are propagated to a final protein p-value according to the Stouffer’s Z-score method. Results A total of 1227 proteins were identified and quantified, of which 87 were differentially abundant, being mainly involved in glycolysis (Warburg effect) and immune system activation (activated stroma). Additionally, in the estrogen receptor-positive subgroup, proteins related to the regulation of insulin-like growth factor transport and platelet degranulation displayed higher abundance, confirming the presence of a proliferative microenvironment. Conclusions We debuted a differential bioinformatics workflow for the proteomic analysis of NAF, validating this secretome as a treasure-trove for studying a paired-organ cancer type. Electronic supplementary material The online version of this article (10.1186/s12885-019-5547-y) contains supplementary material, which is available to authorized users.

Published

2019

27. Molecular effects of Microcystin-LA in tilapia (Oreochromis niloticus)

Author

Daniel A. Moreira, Mauro de Freitas Rebelo, Raquel M. Soares, Maria João Bebianno, and Richard H. Valente

Subjects

0106 biological sciences, food.ingredient, Microcystins, Glutathione transferase, Phosphatase, Biology, Toxicology, 01 natural sciences, Injections, 03 medical and health sciences, Nile tilapia, food, Protein phosphatase 1, Protein Phosphatase 1, Gene expression, Animals, Intraperitoneal, Protein Phosphatase 2, Protein phosphatase 2, Glutathione Transferase, chemistry.chemical_classification, Gene expression regulation, Glutathione Peroxidase, 0303 health sciences, 010604 marine biology & hydrobiology, Glutathione peroxidase, 030302 biochemistry & molecular biology, Tilapia, Cichlids, biology.organism_classification, Molecular biology, Actins, Oreochromis, Real-time polymerase chain reaction, Gene Expression Regulation, chemistry, Injections, Intraperitoneal

Abstract

Nile tilapia (Oreochromis niloticus) is a freshwater phytoplanktivorous fish species reported to accumulate and tolerate large amounts of cyanotoxins such as microcystins (MCs). The present study aimed to investigate molecular responses to the acute exposure of Nile tilapia to the Microcystin-LA analogue (MC-LA). Thus, the specimens were sublethally exposed to 1000 μg kg-1 of MC-LA for 12, 24, 48, and 96 h. Gene expression of PP1, PP2A, GST, GPX and actin was analyzed by quantitative PCR. The protein abundance profile of PP2A was determined by immunoblotting, while the integrity of its biological function was assessed by a phosphatase enzymatic assay. PP2A activity was significantly and strongly reduced by MC-LA. A resulting feedback mechanism significantly increased PP2A gene expression and protein abundance in all assessed times. However, a recovery of that phosphatase activity was not observed. In this study, the observed increase in GPX gene expression was the only response that could be directly related to the unknown factors associated to the fish survival to such high dose exposure. E-26/111.540/2008 info:eu-repo/semantics/publishedVersion

Published

2019

28. Mixed-Data Acquisition: Next-Generation Quantitative Proteomics Data Acquisition

Author

Giselle Villa Flor Brunoro, Michel Batista, Valmir C. Barbosa, Eduardo S B Lyra, Fabio C. Gozzo, Paulo C. Carvalho, Louise U. Kurt, Amanda Caroline Camillo-Andrade, Marlon D.M. Santos, Richard H. Valente, Milan A. Clasen, and Juliana de Saldanha da Gama Fischer

Subjects

Proteomics, 0301 basic medicine, Proteome, 030102 biochemistry & molecular biology, Computer science, business.industry, Test data generation, Quantitative proteomics, Biophysics, Yeast proteome, Computational biology, Biochemistry, Mass Spectrometry, Bottleneck, 03 medical and health sciences, 030104 developmental biology, Software, Data acquisition, skin and connective tissue diseases, business

Abstract

We present the Mixed-Data Acquisition (MDA) strategy for mass spectrometry data acquisition. MDA combines Data-Dependent Acquisition (DDA) and Data-Independent Acquisition (DIA) in the same run, thus doing away with the requirements for separate DDA spectral libraries. MDA is a natural result from advances in mass spectrometry, such as high scan rates and multiple analyzers, and is tailored toward exploiting these features. We demonstrate MDA's effectiveness on a yeast proteome analysis by overcoming a common bottleneck for XIC-based label-free quantitation; namely, the coelution of precursors when m/z values cannot be distinguished. We anticipate that MDA will become the next mainstream data generation approach for proteomics. MDA can also serve as an orthogonal validation approach for DDA experiments. Specialized software for MDA data analysis is made available on the project's website.

Published

2020

29. Inferring venom peptidomics biological activities with connectivity mapping

Author

Richard H. Valente

Subjects

Venom, Computational biology, Biology, Toxicology

Published

2020

30. Data on antigen recognition hindrance by antibodies covalently immobilized to Protein G magnetic beads by dimethyl pimelimidate (DMP) cross-linking

Author

Wilson Alves de Oliveira Junior, Rubem F. S. Menna-Barreto, Silvia Marinho Martins, Jonas Perales, Virgínia Maria Barros de Lorena, Maria da Glória Aureliano de Melo Cavalcanti, Paulo C. Carvalho, Marcelle Almeida Caminha, Diogo B. Lima, and Richard H. Valente

Subjects

Immunoprecipitation, lcsh:Computer applications to medicine. Medical informatics, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Antigen, parasitic diseases, Trypanosoma cruzi, lcsh:Science (General), 030304 developmental biology, Immunology and Microbiology, 0303 health sciences, Multidisciplinary, biology, Chemistry, biology.organism_classification, 3. Good health, Electrophoresis, Dimethyl pimelimidate, Biochemistry, Covalent bond, biology.protein, lcsh:R858-859.7, Protein G, Antibody, 030217 neurology & neurosurgery, lcsh:Q1-390

Abstract

The data presented herein is related to the article entitled ''Trypanosoma cruzi immunoproteome: calpain-like CAP5.5 differentially detected throughout distinct stages of human Chagas disease cardiomyopathy'' [1]. Electrophoretic analyses under denaturing and reducing conditions indicate that covalent immobilization of human IgG to Protein G magnetic beads by cross-linking with 50 mM dimethyl pimelimidate hinders the recognition of T. cruzi antigens in immunoprecipitation assays.

Published

2018

31. Penicillium citrinum UFV1 β-glucosidases: purification, characterization, and application for biomass saccharification

Author

Olinto Liparini Pereira, Richard H. Valente, Fernando A. Genta, Valéria Monteze Guimarães, Samara G. da Costa, Sebastião Tavares de Rezende, and André Teixeira-Ferreira

Subjects

0106 biological sciences, 0301 basic medicine, lcsh:Biotechnology, Cellobiose, Cellulase, Management, Monitoring, Policy and Law, 01 natural sciences, Applied Microbiology and Biotechnology, lcsh:Fuel, 03 medical and health sciences, chemistry.chemical_compound, Hydrolysis, lcsh:TP315-360, lcsh:TP248.13-248.65, 010608 biotechnology, Gentiobiose, Penicillium citrinum, Food science, Laminaribiose, Trichoderma reesei, Inhibition, Subsite analysis, biology, Renewable Energy, Sustainability and the Environment, Beta-glucosidase, Research, Synergism, biology.organism_classification, β-Glucosidase, 030104 developmental biology, General Energy, chemistry, biology.protein, Biomass hydrolysis, Biotechnology

Abstract

Background β-Glucosidases are components of the cellulase system, a family of enzymes that hydrolyze the β-1,4 linkages of cellulose. These proteins have been extensively studied due to the possibility of their use in various biotechnological processes. They have different affinities for substrates (depending on their source) and their activities can be used for saccharification of different types of biomass. In this context, the properties and the synergistic capacity of β-glucosidases from different organisms, to supplement the available commercial cellulase cocktails, need a comprehensive evaluation. Results Two β-glucosidases belonging to GH3 family were secreted by Penicillium citrinum UFV. PcβGlu1 (241 kDa) and PcβGlu2 (95 kDa) presented acidic and thermo-tolerant characteristics. PcβGlu1 showed Michaelis–Menten kinetics for all substrates tested with Km values ranging from 0.09 ± 0.01 (laminarin) to 1.7 ± 0.1 mM (cellobiose, C2) and kcat values ranging from 0.143 ± 0.005 (laminarin) to 8.0 ± 0.2 s−1 (laminaribiose, Lb). PcβGlu2 showed substrate inhibition for 4-methylumbelliferyl-β-d-glucopyranoside (MUβGlu), p-nitrophenyl-β-d-glucopyranoside (pNPβGlu), cellodextrins (C3, C4, and C5), N-octil-β-d-glucopyranoside, and laminaribiose, with Km values ranging from 0.014 ± 0.001 (MUβGlu) to 0.64 ± 0.06 mM (C2) and kcat values ranging from 0.49 ± 0.01 (gentiobiose) to 1.5 ± 0.2 s−1 (C4). Inhibition constants (Ki) for PcβGlu2 substrate inhibition ranged from 0.69 ± 0.07 (MUβGlu) to 10 ± 1 mM (Lb). Glucose and cellobiose are competitive inhibitors of PcβGlu1 and PcβGlu2 when pNPβGlu is used as a substrate. For PcβGlu1 inhibition, Ki = 1.89 ± 0.08 mM (glucose) and Ki = 3.8 ± 0.1 mM (cellobiose); for PcβGlu2, Ki = 0.83 ± 0.05 mM (glucose) and Ki = 0.95 ± 0.07 mM (cellobiose). The enzymes were tested for saccharification of different biomasses, individually or supplementing a Trichoderma reesei commercial cellulose preparation. PcβGlu2 was able to hydrolyze banana pseudostem and coconut fiber with the same efficiency as the T. reesei cocktail, showing significant synergistic properties with T. reesei enzymes in the hydrolysis of these alternative biomasses. Conclusions The β-glucosidases from P. citrinum UFV1 present different enzymatic properties from each other and might have potential application in several biotechnological processes, such as hydrolysis of different types of biomass. Electronic supplementary material The online version of this article (10.1186/s13068-018-1226-5) contains supplementary material, which is available to authorized users.

Published

2018

32. The Primary Duct of Bothrops jararaca Glandular Apparatus Secretes Toxins

Author

Jonas Perales, Luciana Godoy Viana, Richard H. Valente, Norma Yamanouye, Sylvia Mendes Carneiro, Fernanda Sakai, and José Antonio Portes-Junior

Subjects

0301 basic medicine, Bothrops jararaca, primary duct, Health, Toxicology and Mutagenesis, lcsh:Medicine, Venom, Reptilian Proteins, Toxicology, complex mixtures, Article, 03 medical and health sciences, Exocrine Glands, proteomics, Microscopy, Electron, Transmission, venom glandular apparatus, morphology, secretory cycle, venom production, Viperidae, biology.animal, Crotalid Venoms, medicine, Animals, Bothrops, Secretion, Salivary gland, biology, lcsh:R, biology.organism_classification, Secretory Vesicle, Molecular biology, Epithelium, 030104 developmental biology, medicine.anatomical_structure, Female, Duct (anatomy)

Abstract

Despite numerous studies concerning morphology and venom production and secretion in the main venom gland (and some data on the accessory gland) of the venom glandular apparatus of Viperidae snakes, the primary duct has been overlooked. We characterized the primary duct of the Bothrops jararaca snake by morphological analysis, immunohistochemistry and proteomics. The duct has a pseudostratified epithelium with secretory columnar cells with vesicles of various electrondensities, as well as mitochondria-rich, dark, basal, and horizontal cells. Morphological analysis, at different periods after venom extraction, showed that the primary duct has a long cycle of synthesis and secretion, as do the main venom and accessory glands; however, the duct has a mixed mode venom storage, both in the lumen and in secretory vesicles. Mouse anti-B. jararaca venom serum strongly stained the primary duct’s epithelium. Subsequent proteomic analysis revealed the synthesis of venom toxins—mainly C-type lectin/C-type lectin-like proteins. We propose that the primary duct’s toxin synthesis products complement the final venom bolus. Finally, we hypothesize that the primary duct and the accessory gland (components of the venom glandular apparatus) are part of the evolutionary path from a salivary gland towards the main venom gland.

Published

2018

33. Revisiting the Therapeutic Potential of Bothrops jararaca Venom: Screening for Novel Activities Using Connectivity Mapping

Author

Yongde Bao, Ana G.C. Neves-Ferreira, Alyson Prorock, Jay W. Fox, Richard H. Valente, and Carolina A. Nicolau

Subjects

0301 basic medicine, Drug, Bothrops jararaca, Antiparasitic, medicine.drug_class, Health, Toxicology and Mutagenesis, media_common.quotation_subject, lcsh:Medicine, biosimilar drugs, Venom, Pharmacology, Toxicology, complex mixtures, Article, 03 medical and health sciences, Crotalid Venoms, Drug Discovery, medicine, Animals, Humans, Bothrops, media_common, biology, Drug discovery, therapeutic potential, connectivity map, drug discovery, lcsh:R, Biological activity, biology.organism_classification, 030104 developmental biology, Snake venom, MCF-7 Cells, Transcriptome, Functional genomics

Abstract

Snake venoms are sources of molecules with proven and potential therapeutic applications. However, most activities assayed in venoms (or their components) are of hemorrhagic, hypotensive, edematogenic, neurotoxic or myotoxic natures. Thus, other relevant activities might remain unknown. Using functional genomics coupled to the connectivity map (C-map) approach, we undertook a wide range indirect search for biological activities within the venom of the South American pit viper Bothrops jararaca. For that effect, venom was incubated with human breast adenocarcinoma cell line (MCF7) followed by RNA extraction and gene expression analysis. A list of 90 differentially expressed genes was submitted to biosimilar drug discovery based on pattern recognition. Among the 100 highest-ranked positively correlated drugs, only the antihypertensive, antimicrobial (both antibiotic and antiparasitic), and antitumor classes had been previously reported for B. jararaca venom. The majority of drug classes identified were related to (1) antimicrobial activity; (2) treatment of neuropsychiatric illnesses (Parkinson’s disease, schizophrenia, depression, and epilepsy); (3) treatment of cardiovascular diseases, and (4) anti-inflammatory action. The C-map results also indicated that B. jararaca venom may have components that target G-protein-coupled receptors (muscarinic, serotonergic, histaminergic, dopaminergic, GABA, and adrenergic) and ion channels. Although validation experiments are still necessary, the C-map correlation to drugs with activities previously linked to snake venoms supports the efficacy of this strategy as a broad-spectrum approach for biological activity screening, and rekindles the snake venom-based search for new therapeutic agents.

Published

2018

34. Molecular mechanisms underlying intraspecific variation in snake venom

Author

Carolina A. Nicolau, José Antonio Portes-Junior, Milton Yutaka Nishiyama-Jr, Felipe G. Grazziotin, Darin R. Rokyta, Inácio L.M. Junqueira-de-Azevedo, Richard H. Valente, Hipócrates de Menezes Chalkidis, Diana R. Amazonas, Ana Maria Moura-da-Silva, H. Lisle Gibbs, and Rosa Helena Veras Mourão

Subjects

0301 basic medicine, Genetics, Proteome, Structural gene, Biophysics, Venom, Venom Protein, Biology, Proteomics, complex mixtures, Biochemistry, people.cause_of_death, Phenotype, 03 medical and health sciences, 030104 developmental biology, Species Specificity, Snake venom, Venomous snake, Crotalid Venoms, Animals, Bothrops, people, Gene

Abstract

Elucidating the molecular mechanisms underlying snake venom variability provides important clues for understanding how the biological functions of this powerful toxic arsenal evolve. We analyzed in detail individual transcripts and venom protein isoforms produced by five specimens of a venomous snake (Bothrops atrox) from two nearby but genetically distinct populations from the Brazilian Amazon rainforest which show functional similarities in venom properties. Individual variation was observed among the venoms of these specimens, but the overall abundance of each general toxin family was conserved both in transcript and in venom protein levels. However, when expression of independent paralogues was analyzed, remarkable differences were observed within and among each toxin group, both between individuals and between populations. Transcripts for functionally essential venom proteins (“core function” proteins) were highly expressed in all specimens and showed similar transcription/translation rates. In contrast, other paralogues (“adaptive” proteins) showed lower expression levels and the toxins they coded for varied among different individuals. These results provide support for the inferences that (a) expression and translational differences play a greater role in defining adaptive variation in venom phenotypes than does sequence variation in protein coding genes and (b) convergent adaptive venom phenotypes can be generated through different molecular mechanisms. Significance Analysis of individual transcripts and venom protein isoforms produced by specimens of a venomous snake (Bothrops atrox), from the Brazilian Amazon rainforest, revealed that transcriptional and translational mechanisms contribute to venom phenotypic variation. Our finding of evidence for high expression of toxin proteins with conserved function supports the hypothesis that the venom phenotype consists of two kinds of proteins: conserved “core function” proteins that provide essential functional activities with broader relevance and less conserved “adaptive” proteins that vary in expression and may permit customization of protein function. These observations allowed us to suggest that genetic mechanisms controlling venom variability are not restricted to selection of gene copies or mutations in structural genes but also to selection of the mechanisms controlling gene expression, contributing to the plasticity of this important phenotype for venomous snakes.

Published

2018

35. Structural analysis of the natural snake venom metalloendopeptidase inhibitor BJ46a and its target toxin, jararhagin, based on XL-MS and HDX-MS

Author

Richard H. Valente

Subjects

Biochemistry, Chemistry, Toxin, Snake venom, Jararhagin, medicine, Metalloendopeptidase, Toxicology, medicine.disease_cause

Published

2019

36. Integrative structural analysis of the antihemorrhagic protein DM43 and its target toxins BaP1 and jararhagin

Author

Teresa Escalante, Jonas Perales, Surza Lucia Gonçalves da Rocha, Fabio C. Gozzo, Francisco Gomes-Neto, Alexandra Rucavado, Mariana Fioramonte, Diogo B. Lima, Richard H. Valente, Ana G.C. Neves-Ferreira, and Barbara Da Silva Soares

Subjects

Chemistry, Jararhagin, Antihemorrhagic, Pharmacology, Toxicology

Published

2019

37. Structural analysis of a myotoxin-antimyotoxin complex by cross-linking, mass spectrometry, and bioinformatics

Author

Barbara Da Silva Soares, Jonas Perales, Surza Lucia Gonçalves da Rocha, Ana Gisele Da Costa Neves Ferreira, Mariana Fioramonte, Francisco Gomes-Neto, Fabio C. Gozzo, Bruno Lomonte, Diogo B. Lima, and Richard H. Valente

Subjects

Chromatography, Chemistry, Myotoxin, Toxicology, Mass spectrometry

Published

2019

38. Proteomic profiling of nipple aspirate fluid (NAF): Exploring the complementarity of different peptide fractionation strategies

Author

Giselle Villa Flor Brunoro, André Teixeira da Silva Ferreira, Richard H. Valente, Paulo C. Carvalho, Claudia Vitoria de Moura Gallo, Ana G.C. Neves-Ferreira, Jonas Perales, and Dante Pagnoncelli

Subjects

Adult, Proteomics, Carbohydrate biosynthesis, Chromatography, Chemistry, Peptide fractionation, Proteomic Profiling, Nipple Aspirate Fluid, Biophysics, Fractionation, Mass spectrometry, Biochemistry, Mass Spectrometry, Neoplasm Proteins, Fibroadenoma, Tumor Microenvironment, Humans, Female, Protein identification, Peptides, Breast fluid

Abstract

NAF is a breast fluid that is closely related to the tumor microenvironment and a valuable sample for studying breast cancer. To perform an in-depth proteomic analysis of this sample, aliquots of a single NAF digest were analyzed by the following peptide-centric fractionation strategies: a) 30-cm reversed-phase (RP) column on-line with an LTQ-Orbitrap XL; b) off-line strong cation-exchange (SCX) column; and c) pI-based OFFGEL fractionation. All fractions from approaches (b) and (c) were further analyzed on a 10-cm RP column hyphenated to the same mass spectrometer. The RP-30cm, SCX/RP-10cm, and OFFGEL/RP-10cm approaches identified 1676, 2930, and 3240 peptides, which corresponded to 193, 390 and 528 proteins, respectively. In our cumulative dataset, 4466 distinct NAF peptides corresponded to a total of 557 proteins, of which only 34% were identified by all three approaches. No exclusive protein identification was associated to the RP-30cm approach, while SCX/RP-10cm and OFFGEL/RP-10cm contributed to 28 and 166 exclusive identifications, respectively. Each approach provided additional information related to energy metabolism (fermentation process/carbohydrate biosynthesis). In conclusion, the pre-fractionation platforms used were complementary for the comprehensive characterization of NAF and our work provides methodological information for future quantitative cancer-related NAF sample studies.High-resolution peptide separation is a sine qua non condition for achieving extensive proteome coverage. Various techniques have been employed to improve peptide fractionation prior to LC-MS/MS, thus allowing a comprehensive characterization of complex biological samples. Although fractionation efficiency is very sample-dependent, this issue is commonly overlooked, and a "cookbook" approach is routinely used during this critical step. The present study provides a systematic comparison of analytical information needed for the successful large-scale differential proteomic analysis of NAF samples from breast cancer patients, a precious and volume-limited biological sample. It reinforces the importance of optimizing sample-specific fractionation protocols for information retrieval from mass spectrometric analysis.

Published

2015

39. Reevaluating the Trypanosoma cruzi proteomic map: The shotgun description of bloodstream trypomastigotes

Author

Paulo C. Carvalho, André Teixeira da Silva Ferreira, Giselle Villa Flor Brunoro, Felipe da Veiga Leprevost, Marcelle Almeida Caminha, Rubem Figueiredo Sadok Menna-Barreto, Richard H. Valente, and Jonas Perales

Subjects

Proteomics, Chagas disease, Cell signaling, Proteome, DNA repair, Trypanosoma cruzi, Protozoan Proteins, Biophysics, Cell cycle, Biology, medicine.disease, biology.organism_classification, Biochemistry, Microbiology, Cell biology, Mice, parasitic diseases, medicine, Animals, Chagas Disease, Secretion

Abstract

Chagas disease is a neglected disease, caused by the protozoan Trypanosoma cruzi. This kinetoplastid presents a cycle involving different forms and hosts, being trypomastigotes the main infective form. Despite various T. cruzi proteomic studies, the assessment of bloodstream trypomastigote profile remains unexplored. The aim of this work is T. cruzi bloodstream form proteomic description. Employing shotgun approach, 17,394 peptides were identified, corresponding to 7514 proteins of which 5901 belong to T. cruzi. Cytoskeletal proteins, chaperones, bioenergetics-related enzymes, and trans-sialidases are among the top-scoring. GO analysis revealed that all T. cruzi compartments were assessed; and majority of proteins are involved in metabolic processes and/or presented catalytic activity. The comparative analysis between the bloodstream trypomastigotes and cultured-derived or metacyclic trypomastigote proteomic profiles pointed to 2202 proteins exclusively detected in the bloodstream form. These exclusive proteins are related to: (a) surface proteins; (b) non-classical secretion pathway; (c) cytoskeletal dynamics; (d) cell cycle and transcription; (e) proteolysis; (f) redox metabolism; (g) biosynthetic pathways; (h) bioenergetics; (i) protein folding; (j) cell signaling; (k) vesicular traffic; (l) DNA repair; and (m) cell death. This large-scale evaluation of bloodstream trypomastigotes, responsible for the parasite dissemination in the patient, marks a step forward in the comprehension of Chagas disease pathogenesis.The hemoflagellate protozoan T. cruzi is the etiological agent of Chagas disease and affects people by the millions in Latin America and other non-endemic countries. The absence of efficient drugs, especially for treatment during the chronic phase of the disease, stimulates the continuous search for novel molecular targets. The identification of essential molecules, particularly those found in clinically relevant forms of the parasite, could be crucial. Inside the vertebrate host, trypomastigotes circulate in the bloodstream before infecting various tissues. The exposure of bloodstream forms of the parasite to the host immune system likely leads to differential protein expression in the parasite. In this context, an extensive characterization of the proteomic profile of bloodstream trypomastigotes could help to find not only promising drug targets but also antigens for vaccines or diagnostics. This work is a large-scale proteomic assessment of bloodstream trypomastigotes that show a considerable number of proteins belonging to different metabolic pathways and functions exclusive to this parasitic form, and provides a valuable dataset for the biological understanding of this clinically relevant form of T. cruzi.

Published

2015

40. Bothrops jararaca venom gland secretory cells in culture: Effects of noradrenaline on toxin production and secretion

Author

Cíntia Scucuglia Heluany, Luciana Godoy Viana, Richard H. Valente, Norma Yamanouye, Jonas Perales, Milene Schmidt Luna, and Andreia Souza-Imberg

Subjects

0301 basic medicine, Proteomics, medicine.medical_specialty, Venom, Biology, Matrix metalloproteinase, Toxicology, medicine.disease_cause, complex mixtures, Salivary Glands, 03 medical and health sciences, chemistry.chemical_compound, Norepinephrine, Internal medicine, Zymogen, Crotalid Venoms, medicine, Animals, Secretion, Bothrops, Neurotransmitter, Cells, Cultured, 030102 biochemistry & molecular biology, Toxin, Cell biology, 030104 developmental biology, Endocrinology, chemistry, Snake venom, Metalloproteases, Female, medicine.drug

Abstract

Primary culture of snake venom gland secretory cells could be a good model to study the mechanism(s) of toxin(s) production. These cells can produce and secrete venom to the medium with a hemorrhagic activity comparable to that induced by venom collected from snakes. Production of new venom is triggered by the sympathetic outflow, through the release of noradrenaline, but the importance of this neurotransmitter on toxin synthesis has not been addressed. This work led to the identification and comparison of the toxin panel produced by cultured secretory cells, during a 12-day time-course analysis, as well as to the effects of noradrenaline on the process. The results showed that in our culture model the synthesis of new toxins is asynchronous, mimicking data previously published from proteomic analyses of venom glands harvested from animal experimentation. Furthermore, noradrenaline did regulate the synthesis and/or secretion of venom toxins over the analyzed period. Finally, we demonstrated that snake venom metalloproteinases present in these cultured cells secretome were mostly in their zymogen forms; consequently, processing occurs after secretion to the gland lumen. Overall, the data support the use of venom gland secretory cells as a reliable model to investigate the mechanism(s) of toxin(s) synthesis and secretion.

Published

2017

41. Natural Inhibitors of Snake Venom Metallopeptidases

Author

Ana G.C. Neves-Ferreira, Richard H. Valente, Gilberto B. Domont, and Jonas Perales

Subjects

Snake venom, Chemistry, Pharmacology

Published

2017

42. Alterations of the Kidney Cortex Proteome in Response to Exercise Training in Normoglycemic and Hyperglycemic Conditions

Author

Ileana R. León, Antonio G. Pacheco, Eduardo Tibiriçá, Marília B. Gomes, Roger de Moraes, Antonio Claudio Lucas da Nóbrega, Richard H. Valente, Monique R.O. Trugilho, and Jonas Perales

Subjects

Blood Glucose, Male, medicine.medical_specialty, Kidney Cortex, Proteome, Renal cortex, Biology, medicine.disease_cause, Physical Conditioning, Animal, Internal medicine, Heat shock protein, Drug Discovery, medicine, Animals, Aerobic exercise, Endothelial dysfunction, Protein disulfide-isomerase, Kidney, Albumin, General Medicine, medicine.disease, medicine.anatomical_structure, Endocrinology, Hyperglycemia, Female, Rabbits, Reactive Oxygen Species, Oxidative stress

Abstract

Hyperglycemia induces systemic vascular endothelial dysfunction and renal damage through the overproduction of reactive oxygen species (ROS). Regular aerobic exercise decreases the incidence of ROS-associated diseases and is involved in protection against systemic and renal vascular alterations. To investigate the impact of exercise training on renal protein expression in hyperglycemic conditions, we performed gel-based proteomic analyses of the rabbit kidney cortex from sedentary and exercised rabbits after exposure to normal or high glucose concentrations. Abundance of proteins in the renal cortex was determined by two-dimensional polyacrylamide gel electrophoresis followed by protein identification with mass spectrometry, using peptide mass and fragment fingerprintings. We identified the differential abundance of twenty seven proteins in exercise trained animals among the total of 324 spots, from which five proteins are related to the down-regulation of cellular oxidative stress (albumin, protein disulfide isomerase, heat shock protein 60-like chaperonin, DJ-1 and ubiquinol-cytochrome-c reductase), and three proteins are involved in energy metabolism (shortchain acyl-coenzyme A dehydrogenase, malate dehydrogenase and L-arginine-glycine amidinotransferase). We concluded that exercise training induces an increase in the abundance of five antioxidant proteins in the renal cortex, which could explain the well-known increase in endothelial-dependent vasodilation that results from exercise and the consequential protective effect against increased oxidative stress of the hyperglycemic milieu. Moreover, this protective effect could be important in the prevention of kidney vascular damage associated with diabetes pathophysiology.

Published

2014

43. Modeling Protein-Protein Interactions: a structural insight of myotoxin-antimyotoxin complex based on cross-linking data, resolved by mass spectrometry

Author

Barbara Da Silva Soares, Diogo B. Lima, Fabio C. Gozzo, Bruno Lomonte, Richard H. Valente, Jonas Perales, Surza Lucia Gonçalves da Rocha, Ana G.C. Neves-Ferreira, and Francisco Gomes Neto

Subjects

Chemistry, Myotoxin, Biophysics, Toxicology, Mass spectrometry, Protein–protein interaction

Published

2019

44. Molecular mapping of BJ46a / jararhagin complex by mass spectrometry

Author

André Teixeira da Silva Ferreira, Surza Lucia Gonçalves da Rocha, Viviane A. Bastos, Ana Gisele Da Costa Neves Ferreira, Richard H. Valente, Francisco Gomes Neto, and Jonas Enrique Perales Aguilar

Subjects

Chromatography, Chemistry, Jararhagin, Toxicology, Mass spectrometry, Molecular mapping

Published

2019

45. Natural Inhibitors of Snake Venom Metalloendopeptidases: History and Current Challenges

Author

Richard H. Valente, Jonas Perales, Viviane A. Bastos, Francisco Gomes-Neto, and Ana G.C. Neves-Ferreira

Subjects

0301 basic medicine, therapeutic application, Protein family, Protein Conformation, hydrogen/deuterium exchange, Health, Toxicology and Mutagenesis, Antidotes, Snake Bites, Poison control, lcsh:Medicine, Venom, Review, Reptilian Proteins, Biology, History, 18th Century, Toxicology, Metalloendopeptidase Inhibitors, History, 21st Century, complex mixtures, Structure-Activity Relationship, 03 medical and health sciences, Animals, Humans, Protease Inhibitors, structure, mass spectrometry, snake venom, chemistry.chemical_classification, lcsh:R, Metalloendopeptidases, History, 19th Century, modeling, History, 20th Century, Natural resistance, natural immunity, 030104 developmental biology, Biochemistry, chemistry, Snake venom, Immunology, natural resistance, Glycoprotein, Ficolin, metalloendopeptidase inhibitor, Snake Venoms, cross-linking

Abstract

The research on natural snake venom metalloendopeptidase inhibitors (SVMPIs) began in the 18th century with the pioneering work of Fontana on the resistance that vipers exhibited to their own venom. During the past 40 years, SVMPIs have been isolated mainly from the sera of resistant animals, and characterized to different extents. They are acidic oligomeric glycoproteins that remain biologically active over a wide range of pH and temperature values. Based on primary structure determination, mammalian plasmatic SVMPIs are classified as members of the immunoglobulin (Ig) supergene protein family, while the one isolated from muscle belongs to the ficolin/opsonin P35 family. On the other hand, SVMPIs from snake plasma have been placed in the cystatin superfamily. These natural antitoxins constitute the first line of defense against snake venoms, inhibiting the catalytic activities of snake venom metalloendopeptidases through the establishment of high-affinity, non-covalent interactions. This review presents a historical account of the field of natural resistance, summarizing its main discoveries and current challenges, which are mostly related to the limitations that preclude three-dimensional structural determinations of these inhibitors using "gold-standard" methods; perspectives on how to circumvent such limitations are presented. Potential applications of these SVMPIs in medicine are also highlighted.

Published

2016

46. Molecular effects of microcystin-LA toxicity in Tilapia (Oreochromis niloticus)

Author

Richard H. Valente, Maria João Bebianno, Raquel M. Soares, Mauro de Freitas Rebelo, and Daniel A. Moreira

Subjects

Fishery, Oreochromis, food.ingredient, food, biology, Toxicity, Tilapia, Microcystin-LA, Food science, biology.organism_classification

Abstract

A comprehensive understanding of microcystin (MC) effects and mode(s) of action(s) on aquatic biota has not been achieved yet. In the present study, Nile tilapia (Oreochromis niloticus) were sub-lethally exposed to the microcystin analogue MC-LA for 12, 24, 48 and 96 hours, and gene expression of PP1, PP2A, GST and actin were analyzed by quantitative PCR. Moreover, PP2A protein abundance profile was established by immunoblotting, while its biological function integrity was checked by a phosphatase enzymatic assay. PP2A activity was significantly reduced by MC-LA, indicating that MC acts as a PP2A inhibitor, similarly to what occurs in mammals. However, the positive (9.1-fold after 12h) feedback mechanism induced by PP2A gene, after exposure to sub-lethal MC-LA dose (1,000 µg.kg-1), did not counteract the complete PP2A catalytic activity inhibition that occurred concomitantly. A weaker inflammatory response in fish compared to mammals may be the reason why O. niloticus is able to tolerate such high concentrations of MC-LA when compared to mice.

Published

2016

47. Processing of Snake Venom Metalloproteinases: Generation of Toxin Diversity and Enzyme Inactivation

Author

Richard H. Valente, José Antonio Portes-Junior, Ana Maria Moura-da-Silva, Carolina A. Nicolau, Michelle Teixeira de Almeida, and Francisco Gomes-Neto

Subjects

0301 basic medicine, post-translational processing, Health, Toxicology and Mutagenesis, Proteolysis, Adaptation, Biological, enzyme inhibitor, lcsh:Medicine, Venom, Review, Biology, Matrix metalloproteinase, Toxicology, medicine.disease_cause, complex mixtures, 03 medical and health sciences, Catalytic Domain, Enzyme Stability, medicine, Animals, Receptor, snake venom, Genetics, chemistry.chemical_classification, 030102 biochemistry & molecular biology, medicine.diagnostic_test, Toxin, lcsh:R, Snakes, 030104 developmental biology, Enzyme, chemistry, Snake venom, Metalloproteases, metalloproteinase, Adaptation, hemorrhage, Protein Processing, Post-Translational, human activities, Snake Venoms

Abstract

Snake venom metalloproteinases (SVMPs) are abundant in the venoms of vipers and rattlesnakes, playing important roles for the snake adaptation to different environments, and are related to most of the pathological effects of these venoms in human victims. The effectiveness of SVMPs is greatly due to their functional diversity, targeting important physiological proteins or receptors in different tissues and in the coagulation system. Functional diversity is often related to the genetic diversification of the snake venom. In this review, we discuss some published evidence that posit that processing and post-translational modifications are great contributors for the generation of functional diversity and for maintaining latency or inactivation of enzymes belonging to this relevant family of venom toxins.

Published

2016

48. An in-depth snake venom proteopeptidome characterization: Benchmarking Bothrops jararaca

Author

Paulo C. Carvalho, Richard H. Valente, Inácio L.M. Junqueira-de-Azevedo, Magno Junqueira, Ana G.C. Neves-Ferreira, Jonas Perales, Carolina A. Nicolau, and André Teixeira-Ferreira

Subjects

0301 basic medicine, Bothrops jararaca, Proteome, Biophysics, Venom, Nerve Tissue Proteins, Biology, Proteomics, complex mixtures, Biochemistry, 03 medical and health sciences, Crotalid Venoms, Animals, Nucleobindins, Bothrops, Envenomation, Chromatography, 030102 biochemistry & molecular biology, Calcium-Binding Proteins, Proteins, biology.organism_classification, DNA-Binding Proteins, Benchmarking, 030104 developmental biology, Snake venom, Elapidae, Trypsin Digestion, Lysosomes, Peptides

Abstract

A large-scale proteomic approach was devised to advance the understanding of venom composition. Bothrops jararaca venom was fractionated by OFFGEL followed by chromatography, generating peptidic and proteic fractions. The latter was submitted to trypsin digestion. Both fractions were separately analyzed by reversed-phase nanochromatography coupled to high resolution mass spectrometry. This strategy allowed deeper and joint characterizations of the peptidome and proteome (proteopeptidome) of this venom. Our results lead to the identification of 46 protein classes (with several uniquely assigned proteins per class) comprising eight high-abundance bona fide venom components, and 38 additional classes in smaller quantities. This last category included previously described B. jararaca venom proteins, common Elapidae venom constituents (cobra venom factor and three-finger toxin), and proteins typically encountered in lysosomes, cellular membranes and blood plasma. Furthermore, this report is the most complete snake venom peptidome described so far, both in number of peptides and in variety of unique proteins that could have originated them. It is hypothesized that such diversity could enclose cryptides, whose bioactivities would contribute to envenomation in yet undetermined ways. Finally, we propose that the broad range screening of B. jararaca peptidome will facilitate the discovery of bioactive molecules, eventually leading to valuable therapeutical agents.Our proteopeptidomic strategy yielded unprecedented insights into the remarkable diversity of B. jararaca venom composition, both at the peptide and protein levels. These results bring a substantial contribution to the actual pursuit of large-scale protein-level assignment in snake venomics. The detection of typical elapidic venom components, in a Viperidae venom, reinforces our view that the use of this approach (hand-in-hand with transcriptomic and genomic data) for venom proteomic analysis, at the specimen-level, can greatly contribute for venom toxin evolution studies. Furthermore, data were generated in support of a previous hypothesis that venom gland secretory vesicles are specialized forms of lysosomes. Two testable hypotheses also emerge from the results of this work. The first is that a nucleobindin-2-derived protein could lead to prey disorientation during envenomation, aiding in its capture by the snake. The other being that the venom's peptidome might contain a population of cryptides, whose biological activities could lead to the development of new therapeutical agents.

Published

2016

49. Differential gel electrophoresis (DIGE) evaluation of naphthoimidazoles mode of action: a study in Trypanosoma cruzi bloodstream Trypomastigotes

Author

Rubem Figueiredo Sadok Menna-Barreto, Marcelle Almeida Caminha, Richard H. Valente, Vitor M. Faça, André Teixeira da Silva Ferreira, Giselle Villa Flor Brunoro, Monique R.O. Trugilho, Jonas Perales, and Kelly C. G. de Moura

Subjects

0301 basic medicine, Proteomics, Life Cycles, Protozoan Proteins, Protozoology, ELETROFORESE EM GEL, Biochemistry, Heat Shock Response, Mice, 0302 clinical medicine, Electrophoresis, Gel, Two-Dimensional, Cellular Stress Responses, Protozoans, biology, lcsh:Public aspects of medicine, Trypanocidal Agents, Infectious Diseases, Benznidazole, Nitroimidazoles, Cell Processes, Epimastigotes, Protozoan Life Cycles, medicine.drug, Research Article, Chagas disease, Trypanosoma, lcsh:Arctic medicine. Tropical medicine, lcsh:RC955-962, Trypanosoma cruzi, 030231 tropical medicine, Microbiology, 03 medical and health sciences, Tubulins, Heat shock protein, medicine, Animals, Chagas Disease, Nifurtimox, Mode of action, Protein kinase C, Trypanocidal agent, Public Health, Environmental and Occupational Health, Organisms, Biology and Life Sciences, Proteins, lcsh:RA1-1270, Cell Biology, Trypomastigotes, medicine.disease, biology.organism_classification, Molecular biology, Parasitic Protozoans, Chaperone Proteins, Cytoskeletal Proteins, 030104 developmental biology, Naphthoquinones, Developmental Biology

Abstract

Background The obligate intracellular protozoan Trypanosoma cruzi is the causative agent of Chagas disease, a neglected illness affecting millions of people in Latin America that recently entered non-endemic countries through immigration, as a consequence of globalization. The chemotherapy for this disease is based mainly on benznidazole and nifurtimox, which are very efficient nitroderivatives against the acute stage but present limited efficacy during the chronic phase. Our group has been studying the trypanocidal effects of naturally occurring quinones and their derivatives, and naphthoimidazoles derived from β-lapachone N1, N2 and N3 were the most active. To assess the molecular mechanisms of action of these compounds, we applied proteomic techniques to analyze treated bloodstream trypomastigotes, which are the clinically relevant stage of the parasite. Methodology/Principal Findings The approach consisted of quantification by 2D-DIGE followed by MALDI-TOF/TOF protein identification. A total of 61 differentially abundant protein spots were detected when comparing the control with each N1, N2 or N3 treatment, for 34 identified spots. Among the differentially abundant proteins were activated protein kinase C receptor, tubulin isoforms, asparagine synthetase, arginine kinase, elongation factor 2, enolase, guanine deaminase, heat shock proteins, hypothetical proteins, paraflagellar rod components, RAB GDP dissociation inhibitor, succinyl-CoA ligase, ATP synthase subunit B and methionine sulfoxide reductase. Conclusion/Significance Our results point to different modes of action for N1, N2 and N3, which indicate a great variety of metabolic pathways involved and allow for novel perspectives on the development of trypanocidal agents., Author Summary Trypanosoma cruzi is the etiological agent of Chagas disease, an important illness for Latin American countries that is now afflicting other continents due to the immigration of infected people. The available chemotherapy is limited to the chronic phase of the disease, being the development of novel active compounds essential, and the search for specific molecular targets for drugs in T. cruzi is necessary. In this context, our group has synthesized and screened many compounds ranging from natural to semi-synthetic naphthoquinones and derivatives on T. cruzi, displaying naphthoimidazoles N1, N2 and N3 the highest activity. Previous studies correlated phenotypic alterations by cell biology techniques as well as investigated mode of action by proteomic approaches in insect stage epimastigotes as a model. However, T. cruzi presents three morphologically distinct life stages with their own specific biological peculiarities and requirements that could be potential targets to drug intervention. Here, we evaluated the mechanism of action of N1, N2 and N3 in clinical relevant form of the parasite, bloodstream trypomastigotes, by proteomics. Our data pointed to 61 differentially abundant protein spots, being these proteins involved with cellular trafficking, protein synthesis, transduction signaling and energetic metabolism, among others, open interesting perspectives for trypanocidal strategies.

Published

2016

50. Snake Venom Proteopeptidomics: What Lies Behind the Curtain

Author

Richard H. Valente, Jonas Perales, Ana G.C. Neves-Ferreira, and Carolina A. Nicolau

Subjects

Snake venom, Zoology, Biology

Published

2016