Vacina multicomponente recombinante baseada em antígenos secretados por Rhipicephalus microplus induz imunidade protetora contra carrapatos em bovinos e cães / Recombinant multicomponent vaccine based on antigens secreted by Rhipicephalus microplus induces protective immunity against ticks in cattle and dogs

Fisch, Andressa

17 October 2018

Carrapatos são parasitas hematófagos transmissores de doenças para humanos e animais, e responsáveis por prejuízos econômicos de bilhões de dólares para os sistemas pecuários mundiais. A emergência de carrapatos multirresistentes a acaricidas torna urgente o desenvolvimento de vacinas efetivas contra este parasita. Neste trabalho, nós utilizamos dados de sialotranscriptomas de carrapatos R. microplus para selecionar antígenos secretados pelo parasita para serem testados como uma vacina multicomponente. Os antígenos produzidos de forma recombinante em E. coli foram utilizados como imunógenos em animais suscetíveis à carrapatos para testes de proteção vacinal contra infestações por R. microplus em bovinos e por R. sanguineus em cães. No primeiro ensaio, bovinos imunizados com oito antígenos recombinantes adjuvantados com um polímero sintético apresentaram indução de IgG sérica específica para cinco antígenos, e redução de 22% na infestação por carrapatos R. microplus. No segundo ensaio, a imunização de bovinos com nove antígenos adjuvantados com sais de alumínio gerou IgG específica para todos os antígenos inoculados, e proteção vacinal crescente de 70% e 75% em duas infestações sucessivas com carrapatos R. microplus, sem revacinação, indicando boost natural pela infestação. No terceiro ensaio, a imunização de cães com nove antígenos recombinantes associados à hidróxido de alumínio induziu a soroconversão de IgG dos animais para todos os antígenos, e proteção vacinal de 36% contra a infestação por carrapatos R. sanguineus. Todas as formulações afetaram principalmente o número de fêmeas ingurgitadas após a infestação. O efeito protetor de antígenos derivados de carrapatos R. microplus sobre carrapatos R. sanguineus (proteção cruzada) indica ser possível o desenvolvimento de uma vacina multicomponente efetiva contra os dois parasitas. / Ticks are hematophagous parasites which transmit diseases to humans and animals, and are responsible for billions of dollars of damage to the world\'s livestock systems. The emergence of ticks resistant to multiple acaricides makes urgent the development of effective vaccines against this parasite. In this work, we used data from the R. microplus tick sialotranscriptome to select antigens secreted by the parasite to be tested as a multicomponent vaccine. Recombinant antigens expressed in E. coli were used as antigens in tick\'s susceptible hosts to evaluate it efficacy in protect animals against R. microplus and R. sanguineus infestations. In the first assay, bovines immunized with eight recombinant antigens adjuvanted with a synthetic polymer presented the induction of serum IgG reactive for five antigens, and reduction of R. microplus infestation in 22%. In the second trial, immunization of cattle with nine antigens adjuvanted with aluminum salts generated serum IgG against all antigens, and vaccine protection against R. microplus parasitism was calculated in 70% and 75% for each infestation. In the third trial, the immunization of dogs with recombinant antigens adjuvanted with aluminum hydroxide induced IgG seroconversion against all antigens, and a 36% of protection against infestation by R. sanguineus ticks in immunized animals. All formulations reduced mainly the number of engorged females recovered from infestation. The cross reactive protection induced by R. microplus derived antigens R. sanguineus tick infestation indicate that it is possible to develop a unique multicomponent vaccine against the two parasites.

Secretoma da bactéria fitopatogênica Xanthomonas citri subsp. citri /

Ferreira, Rafael Marini.

January 2009

Resumo: O cancro cítrico está entre as principais doenças que afetam a produção de laranjas no Brasil e é causado pela bactéria fitopatogênica gram-negativa Xanthomonas citri subsp. citri (Xac). O presente trabalho teve por objetivo analisar a expressão diferencial de proteínas secretadas pela bactéria selvagem e por um mutante (02H02) assintomático, que teve a proteína HrpB4, que participa de seu sistema de secreção tipo III (SSTT) inativada, em condição de cultivo em meio rico CN e em meio XAM1 indutor de hipersensibilidade e patogenicidade (genes hrp). As proteínas secretadas em meio de cultura foram extraídas pela ação do ácido tricloroacético (TCA) e identificadas através de espectrometria de massas. Tais análises identificaram 55 proteínas diferentes secretadas em ambos os meios de cultura, tanto para Xac quanto para 02H02, de modo que 13 destas proteínas são comuns entre a Xac e seu mutante cultivados em XAM1 e 14 são exclusivas para Xac cultivada em XAM1, as quais deixaram de ser secretadas no 02H02. Proteínas relacionadas aos genes reguladores do SSTT foram detectadas em condição infectante para ambas as bactérias, demonstrando a eficácia do meio de cultura XAM1 em induzir Hrp. Foi observado que diversas proteínas secretadas pelo sistema de secreção tipo II (SSTD) em condição infectante para Xac e seu mutante possuem um papel ativo na degradação das paredes celulares do hospedeiro e podem ser reguladas por proteínas controladoras do SSTT. Fatores de sinalização difusíveis produzidos por Xac aparentemente sofreram alteração em sua secreção no mutante devido à inativação do pilus do SSTT, demonstrando a relação dessa molécula com o SSTT. A não detecção de proteínas secretadas diretamente pelo SSTT denota que as mesmas podem estar sendo secretadas no interior de vesículas lipídicas de membrana externa, assim como ocorre em Xanthomonas campestris / Abstract: Citrus canker is among the major diseases which affect citrus production in Brazil and is caused by the gram-negative phytopathogenic bacterium Xanthomonas citri subsp. citri (Xac). This work aimed to analyze the differential expression of secreted proteins by the wild bacterium and by an asymptomatic mutant (02H02), lacking the type III secretion system (TTSS) protein HrpB4, in rich cultivation medium NB and in the hrp inducing medium XAM1. The proteins secreted in all culture media have been extracted by trichloroacetic acid based protocols (TCA) and identified using mass spectrometry. The analysis identified 55 different proteins secreted in both culture medium for Xac and 02H02, of which 13 are common among Xac and its mutant cultivated in XAM1 and 14 proteins are exclusively secreted by Xac cultivated in XAM1. Proteins related to the TTSS regulatory genes have been detected in infecting condition in both bacteria, showing the effectiveness of XAM1 hrp inducing medium. It has been observed that several type II secretion system's secreted proteins showed an active role in host cell wall degradation and may be regulated by type III secretion system's proteins in Xac and 02H02 in infecting condition. Diffusible signal factors produced by wild Xac apparently suffered an altered secretion in the mutant due the inactivation of the type three secretion system's pilus, showing the relationship of this molecule with this secretion system. The lack of detection of proteins secreted by the TTSS denote that these proteins may be secreted in the interior of outer membrane lipid vesicles, just like it was verified in Xanthomonas campestris / Orientador: Jesus Aparecido Ferro / Coorientador: Julio Cezar Franco de Oliveira / Banca: Maria Teresa Marques Novo / Banca: Leandro Márcio Moreira / Mestre

Cancro citrico.

Xanthomonas campestris.

Plant pathogen interactions. eng

Pathogenicity inducing medium. eng

Secreted proteins. eng

Citrus canker proteome. eng

Type III secretion systems (TTSS) eng

Caractérisation fonctionnelle de petites protéines sécrétées chez les champignons lignolytiques / Characterization of small proteins by lignolytic fungi

Valette, Nicolas

06 December 2017

Durant ces dernières décennies, les systèmes enzymatiques de dégradation du bois sécrétés par les champignons ont fait l’objet de nombreuses études aboutissant à la caractérisation fonctionnelle et biochimique des enzymes extracellulaires majeures agissant directement sur le polymère. Cependant, les systèmes annexes associés au processus de dégradation n’ont à l’heure actuelle été que peu étudiés. En particulier, les systèmes de détoxication et de réponses des champignons au stress généré par le processus de dégradation ainsi que les mécanismes lui permettant de croître dans cet environnement hostile sont encore peu connus. Ce stress est majoritairement dû à la présence de radicaux et d’extractibles. Les extractibles sont des molécules issues du métabolisme secondaire de l’arbre qui sont synthétisés pour augmenter la durabilité du bois face aux attaques biotiques et abiotiques. Une analyse transcriptomique réalisée au laboratoire a mis en évidence la surexpression de gènes codant des petites protéines sécrétées (SSP) chez Phanerochaete chrysosporium lors d’une culture en présence d’extractibles de chêne. La fonction de ce type de protéines chez les champignons lignolytiques est inconnue. Mon projet de thèse a porté sur la caractérisation d’une de ces SSP (SSP1). Les résultats obtenus ont révélé des propriétés biochimiques atypiques pour cette protéine qui est capable de former une structure fibrillaire, notamment grâce à la présence d’un domaine C-terminal riche en alanine et glycine. De plus, nous avons pu montrer que cette protéine présentait une activité β-glucuronidase in vitro, qui est dépendante de son état d’oligomérisation. Une approche physiologique a également été abordée grâce à l’obtention de mutants knock-out de SSP de Podospora anserina. La caractérisation de ces mutants a montré un défaut de croissance en condition de stress oxydant et en présence de molécules perturbant l’intégrité de la paroi cellulaire. Enfin, une analyse in silico des orthologues de SSP1 a montré la présence de ce gène dans les génomes d’organismes saprophytes, ectomycorhiziens ou pathogènes suggérant un rôle indirect de cette protéine dans les processus de dégradation du bois, probablement en lien avec la gestion du stress associé / During the last decades, the enzymatic systems involved in wood degradation have been intensively studied in fungi. This has led to functional and biochemical characterization of the main extracellular enzymes that are involved in the process. However, other systems associated to the degradation mechanisms have been poorly studied. In particular, the detoxification and stress response pathways allowing the fungus to grow in and resist the toxic conditions that are associated to the degradative process are still unknown. This stress is mostly due to the presence of radicals and extractives. Extractives are putative toxic compounds produced as secondary metabolites in tree to enhance wood durability against biotic and abiotic attacks. A transcriptomic analysis performed in the laboratory highlighted the up-regulation of genes coding for small secreted proteins (SSP) in Phanerochaete chrysosporium in presence of oak extractives. The functions of these SSP are unknown in lignolytic fungi. My PhD project was focused on the characterization of one of these SSP (namely SSP1) of P. chrysosporium. The biochemical data revealed atypical features for SSP1. Indeed, it is able to form fibrilar structure, thanks to an alanine-rich and glycine-rich C-terminal domain. Moreover, we have shown that this protein exhibits β-glucuronidase activity in vitro which is dependent on its oligomerization state. Physiological data were obtained thanks to the obtention of SSP knock-out mutants in Podospora anserina. These mutants have growth defect in oxidizing stress condition and in presence of cell wall-disruptive compounds. Finally, the in silico analysis of SSP1 orthologues revealed the presence of this gene in genomes of saprophytic, ectomycorrhizal or pathogenic fungi, suggesting an indirect role of this protein in wood degradation processes, probably linked to the associated stress

Phanerochaete chrysosporium

Petites protéines sécrétées (SSP)

Dégradation du bois

Extractibles

Saprophytes

Stress

Phanerochaete chrysosporium

Small secreted proteins (SSP)

Wood degradation

Extractives

Saprophytic fungi

Stress

579.17

579.5

Secretoma da bactéria fitopatogênica Xanthomonas citri subsp. citri

Ferreira, Rafael Marini [UNESP]

05 November 2009

Made available in DSpace on 2014-06-11T19:26:09Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-11-05Bitstream added on 2014-06-13T20:33:53Z : No. of bitstreams: 1 ferreira_rm_me_jabo.pdf: 510263 bytes, checksum: 543073ee3d6f55d77bb1607889dc966f (MD5) / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) / O cancro cítrico está entre as principais doenças que afetam a produção de laranjas no Brasil e é causado pela bactéria fitopatogênica gram-negativa Xanthomonas citri subsp. citri (Xac). O presente trabalho teve por objetivo analisar a expressão diferencial de proteínas secretadas pela bactéria selvagem e por um mutante (02H02) assintomático, que teve a proteína HrpB4, que participa de seu sistema de secreção tipo III (SSTT) inativada, em condição de cultivo em meio rico CN e em meio XAM1 indutor de hipersensibilidade e patogenicidade (genes hrp). As proteínas secretadas em meio de cultura foram extraídas pela ação do ácido tricloroacético (TCA) e identificadas através de espectrometria de massas. Tais análises identificaram 55 proteínas diferentes secretadas em ambos os meios de cultura, tanto para Xac quanto para 02H02, de modo que 13 destas proteínas são comuns entre a Xac e seu mutante cultivados em XAM1 e 14 são exclusivas para Xac cultivada em XAM1, as quais deixaram de ser secretadas no 02H02. Proteínas relacionadas aos genes reguladores do SSTT foram detectadas em condição infectante para ambas as bactérias, demonstrando a eficácia do meio de cultura XAM1 em induzir Hrp. Foi observado que diversas proteínas secretadas pelo sistema de secreção tipo II (SSTD) em condição infectante para Xac e seu mutante possuem um papel ativo na degradação das paredes celulares do hospedeiro e podem ser reguladas por proteínas controladoras do SSTT. Fatores de sinalização difusíveis produzidos por Xac aparentemente sofreram alteração em sua secreção no mutante devido à inativação do pilus do SSTT, demonstrando a relação dessa molécula com o SSTT. A não detecção de proteínas secretadas diretamente pelo SSTT denota que as mesmas podem estar sendo secretadas no interior de vesículas lipídicas de membrana externa, assim como ocorre em Xanthomonas campestris / Citrus canker is among the major diseases which affect citrus production in Brazil and is caused by the gram-negative phytopathogenic bacterium Xanthomonas citri subsp. citri (Xac). This work aimed to analyze the differential expression of secreted proteins by the wild bacterium and by an asymptomatic mutant (02H02), lacking the type III secretion system (TTSS) protein HrpB4, in rich cultivation medium NB and in the hrp inducing medium XAM1. The proteins secreted in all culture media have been extracted by trichloroacetic acid based protocols (TCA) and identified using mass spectrometry. The analysis identified 55 different proteins secreted in both culture medium for Xac and 02H02, of which 13 are common among Xac and its mutant cultivated in XAM1 and 14 proteins are exclusively secreted by Xac cultivated in XAM1. Proteins related to the TTSS regulatory genes have been detected in infecting condition in both bacteria, showing the effectiveness of XAM1 hrp inducing medium. It has been observed that several type II secretion system’s secreted proteins showed an active role in host cell wall degradation and may be regulated by type III secretion system’s proteins in Xac and 02H02 in infecting condition. Diffusible signal factors produced by wild Xac apparently suffered an altered secretion in the mutant due the inactivation of the type three secretion system’s pilus, showing the relationship of this molecule with this secretion system. The lack of detection of proteins secreted by the TTSS denote that these proteins may be secreted in the interior of outer membrane lipid vesicles, just like it was verified in Xanthomonas campestris

Cancro cítrico

Xanthomonas campestris

Secretoma

Plant pathogen interactions

Pathogenicity inducing medium

Secreted proteins

Citrus canker proteome

Type III secretion systems (TTSS)

Host cell responses to Helicobacter pylori secreted factors

Garcia Lobato Tavares, Raquel

January 2017

The infection of the human gastric mucosa by the bacterium Helicobacter pylori can lead to the development of gastritis, gastroduodenal ulcers, and cancer. The factors that determine disease development in a small percentage of infected individuals are still not fully understood. In this thesis, we aimed to identify and functionally characterize novel virulence factors of H. pylori and to understand their effect on host cell responses. In Paper I, we found that JHP0290, an uncharacterized secreted protein of H. pylori, induced macrophage apoptosis concomitant to the release of pro-inflammatory cytokine TNF via the regulation of the Src family of kinases and ERK MAPK pathways. In paper II, we demonstrated that JHP0290 exhibits both proliferative and anti-apoptotic activity, together with a faster progression of the cell cycle in gastric epithelial cells. During these responses, ERK MAPK and NF-κB pathways were activated. Paper III revealed a pro-apoptotic effect of another H. pylori-secreted protein HP1286 in macrophages via the TNF-independent and ERK-dependent pathways. No apoptosis was observed in HP1286-treated T cells or HL60 neutrophil-like cells, suggesting cell-type specific effect of HP1286. In Paper IV, we observed the pro-inflammatory activity of H. pylori secreted protein HP1173 in macrophages. The protein was found to induce TNF, IL-1β, and IL-8 in macrophages through MAPKs, NF-κB, and AP-1 signaling pathways. Furthermore, differential expression and release of JHP0290, HP1286, and HP1173 homologues was observed among H. pylori strains (papers II, III, IV).  Due to their ability to regulate multiple host cell responses, proteins JHP0290, HP1286, and HP1173 could play an important role in bacterial pathogenesis.

Helicobacter pylori

Secreted proteins

Host cell responses

Macrophages

Apoptosis

Pro-inflammatory cytokines

MAPKs