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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
91

Verticillium longisporum, infection, host range, prevalence and plant defence responses /

Johansson, Anna, January 2006 (has links) (PDF)
Licentiatavhandling Uppsala : Sveriges lantbruksuniversitet, 2006. / Härtill 3 uppsatser.
92

Studies of gammaherpesvirus infection and host response /

Buckingham, Erin M. January 2007 (has links)
Thesis (Ph.D. in Microbiology & Immunology) -- University of Colorado Denver, 2007. / Typescript. Includes bibliographical references (leaves 200-212).
93

The late blight pathogen, Phytophthora infestans : interaction with the potato plant and inoculum sources /

Widmark, Anna-Karin, January 2010 (has links) (PDF)
Diss. (sammanfattning) Uppsala : Sveriges lantbruksuniversitet, 2010. / Härtill 4 uppsatser.
94

Isolamento e caraterização de Lactobacillus spp. da cavidade bucal e sua ação probiótica sob Candida albicans: formação de biofilme, infecção em modelos de invertebrados e expressão dos genes EFG1, HWP1 e ALS1 / Isolation and characterization of Lactobacillus spp. from oral cavity and their probiotic action in Candida albicans: biofilm formation, infection in invertebrate models and EFG1, HWP1 and ALS1 gene expression

Rossoni, Rodnei Dennis [UNESP] 04 December 2017 (has links)
Submitted by Rodnei Dennis Rossoni (rodnei.rossoni@fosjc.unesp.br) on 2017-12-11T11:19:52Z No. of bitstreams: 1 Tese_Pronta.pdf: 4361864 bytes, checksum: 4e8e22ae0f0744e73ce578cec2fbcce4 (MD5) / Submitted by Rodnei Dennis Rossoni (rodnei.rossoni@fosjc.unesp.br) on 2017-12-11T18:47:11Z No. of bitstreams: 1 Tese_Pronta.pdf: 4361864 bytes, checksum: 4e8e22ae0f0744e73ce578cec2fbcce4 (MD5) / Submitted by Rodnei Dennis Rossoni (rodnei.rossoni@fosjc.unesp.br) on 2017-12-14T11:25:03Z No. of bitstreams: 1 Tese_Pronta.pdf: 4361864 bytes, checksum: 4e8e22ae0f0744e73ce578cec2fbcce4 (MD5) / Submitted by Rodnei Dennis Rossoni (rodnei.rossoni@fosjc.unesp.br) on 2017-12-14T13:50:32Z No. of bitstreams: 1 Tese_Pronta.pdf: 4361864 bytes, checksum: 4e8e22ae0f0744e73ce578cec2fbcce4 (MD5) / Approved for entry into archive by Silvana Alvarez null (silvana@ict.unesp.br) on 2017-12-18T15:12:51Z (GMT) No. of bitstreams: 1 rossoni_rd_dr_sjc.pdf: 4361864 bytes, checksum: 4e8e22ae0f0744e73ce578cec2fbcce4 (MD5) / Made available in DSpace on 2017-12-18T15:12:51Z (GMT). No. of bitstreams: 1 rossoni_rd_dr_sjc.pdf: 4361864 bytes, checksum: 4e8e22ae0f0744e73ce578cec2fbcce4 (MD5) Previous issue date: 2017-12-04 / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / O estudo da atividade inibitória de Lactobacillus pode contribuir na descoberta de novas estratégias terapêuticas nas infecções por Candida. Nesse contexto, o objetivo desse estudo foi isolar e identificar Lactobacillus da cavidade bucal de indivíduos livres de cárie e avaliar seu potencial de inibição de C. albicans por meio de estudos in vitro e in vivo. Primeiramente, foram avaliados os efeitos de 30 isolados clínicos de Lactobacillus sobre o número de células viáveis (UFC) em biofilme de C. albicans e sobre a formação de hifas. Os isolados que obtiveram os maiores efeitos inibitórios sobre C. albicans foram selecionados para os testes de determinação da biomassa total dos biofilmes pela absorbância do cristal violeta, análise da arquitetura dos biofilmes por microscopia eletrônica de varredura (MEV) e quantificação da expressão de genes de C. albicans (ALS3, HWP1, EFG1 e CPH1) por qPCR. Esses isolados também foram submetidos a estudos in vivo usando os modelos de Galleria mellonella e Caenorhabditis elegans. Para o estudo em G. mellonella, a infecção experimental foi avaliada pela curva de sobrevivência, quantificação da carga fúngica na hemolinfa, densidade hemocitária, quantificação da expressão gênica de peptídeos antifúngicos (Gallerymicina e Galiomicina) e monitoramento da infecção de C. albicans por análise de bioluminescência. No modelo de C. elegans, a infecção foi avaliada por meio dos ensaios de curva de sobrevivência e estudo da filamentação de C. albicans. Os resultados dos ensaios in vitro demonstraram que L. paracasei 28.4, L. rhamnosus 5.2 e L. fermentum 20.4 foram as cepas com maior atividade antimicrobiana sobre os biofilmes de C. albicans. Nessas cepas, todos os genes analisados foram regulados negativamente na associação com Lactobacillus quando comparados com o grupo controle. No estudo in vivo, a injeção de L. paracasei 28.4 em G. mellonella infectadas com C. albicans aumentou a sobrevida das larvas, o número de hemócitos e a expressão de peptídeos antifúngicos, reduzindo assim a UFC de C. albicans. Em C. elegans, L. paracasei 28.4 também foi capaz de aumentar a sobrevida dos vermes infectados com C. albicans e reduzir a filamentação. Conclui-se que L. fermentum 20.4, L. paracasei 28.4 e L. rhamnosus 5.2 tem potencial para serem usados como probióticos na cavidade bucal devido sua ação anti-biofilme e sua regulação negativa dos genes de virulência de C. albicans. L. paracasei 28.4 foi capaz de prolongar a sobrevida nos dois modelos experimentais infectados com C. albicans por apresentarem ação antifúngica e imunomodulatória. / The study of the antifungal activity of Lactobacillus may contribute to the discovery of new therapeutic strategies for Candida infections. In this context, the objective of this study was to isolate and identify Lactobacillus from the oral cavity of caries-free subjects and to evaluate its effects through in vitro and in vivo studies. First, the effects of 30 clinical isolates of Lactobacillus on the number of viable cells (CFU) in biofilms of C. albicans and on hyphae formation were evaluated. The isolates that obtained the highest inhibitory effects on C. albicans were selected for biofilm biomass determination by violet crystal absorbance, analysis of biofilm architecture by scanning electron microscopy (SEM) and quantification of the expression of C. albicans (ALS3, HWP1, EFG1 and CPH1) by real time PCR. These isolates were also submitted to in vivo studies using the Galleria mellonella and Caenorhabditis elegans models. For the study in the model of Galleria mellonella, the experimental infection was evaluated by the survival curve, quantification of the fungal load in the hemolymph, hemocitary density, the gene expression of antifungal peptides (Gallerymicin and Galiomicin) and monitoring of C. albicans infection by bioluminescence analysis. In the Caenorhabditis elegans model, the infection was evaluated by the survival curve assays and the study of C. albicans filamentation. The results of in vitro tests demonstrated that L. paracasei 28.4, L. rhamnosus 5.2 and L. fermentum 20.4 were the strains with the highest antimicrobial activity on the biofilms of C. albicans. In these strains, all analyzed genes were negatively regulated in association with Lactobacillus when compared to the control group. In the in vivo study, the injection of L. paracasei 28.4 into the G. mellonella increased survival of the larvae, the number of hemocytes and the expression of antifungal peptides, thus reducing the CFU of C. albicans. In C. elegans, L. paracasei 28.4 was also able to increase the survival of worms infected with C. albicans and reduce the filamentation. We conclude that L. fermentum 20.4, L. paracasei 28.4 and L. rhamnosus 5.2 have potential to be used as probiotics in the oral cavity due to their anti-biofilm action and their negative regulation of virulence genes of C. albicans. L. paracasei 28.4 was able to prolong survival of both experimental models infected with C. albicans for having antifungal and immunomodulatory action. / 13/25181-8 / 14/12458-4
95

Réseau régulatoire de HDAC3 pour comprendre les mécanismes de différenciation et de pathogenèse de Toxoplasma gondii / Characterization of histone modifications inside nucleosome H4K31ac and H4K31me1 in Apicomplexan parasites

Sindikubwabo, Fabien 12 October 2017 (has links)
Apicomplexan parasites are leading causes of human and livestock diseases such as toxoplasmosis and malaria caused by Toxoplasma gondii and Plasmodium falciparum respectively. These organisms are varied in their morphologies and astoundingly complex on their life cycles that include infections of more than one host organism, differentiation through several morphologically distinct forms, and both sexual and asexual replication. What we and others have initially proposed was that the control of gene expression and cellular differentiation are particularly interesting in these organisms, as the apparent lack of large families of recognizable transcription factors typically found in other eukaryotic organisms suggests that they may be unusually reliant on epigenetic mechanisms. The initial hypothesis had to be re-assessed in light of the discovery in Apicomplexa of an expanded family of plant-like transcription factors (TFs) harbouring APETALA2 (AP2)-like domains. Yet, a growing body of evidence tends to favor epigenetic as one of the main contributor to parasite developmental programs and adjustments to fluctuant environment. One way to examine dynamic changes in post-translations modifications (PTMs) patterns is to alter the histone code writing. We therefore took advantage of HDAC inhibitors and showed that specific inhibition of TgHDAC3 by the cyclopeptide FR235222 disrupts the genome wide steady-state level of histone H4 acetylation inducing derepression of stage-specific genes. Yet, many questions about TgHDAC3 modus operandi remain unanswered. During my thesis, I uncovered the TgHDAC3-regulated proteome-wide acetylome typified by the presence of non-histone proteins including AP2 TFs and novel PTMs, e.g. the acetylation at Lys31 within the globular domain of histone H4. H4K31ac promotes a relaxed chromatin state at the promoter of active genes through nucleosome disassembly in both parasites. We identified TgGCN5B and TgHDAC3 as two antagonist enzymes regulating H4K31 acetylation in T. gondii. In contrast, H4K31monomethylation is enriched throughout the gene body of T. gondii active genes and contributes to transcription, whereas it is enriched at transcriptionally inactive pericentromeric heterochromatin regions in P. falciparum, a region that is lacking H3K9me3 and heterochromatin protein 1 in this parasite. We also showed that treating T. gondii cystogenic strains with a low dose of FR235222 induces the levels of proteins known to be expressed exclusively in cat (sporozoite and merozoite) or in murine chronic stage (bradyzoite). Lastly, we determined the specific interactome of TgHDAC3 and found as partners a MORC protein (CR230), several AP2 TFs, and ELM2 domain-containing scaffolding proteins. Collectively, these data established TgHDAC3 family as a central regulator of gene expression and stage conversion in T. gondii and, likely, other Apicomplexa. / Apicomplexan genome architecture is typified by a binary chromatin structure, with a major fraction of the bulk genome packaged as transcriptionally permissive euchromatin while few loci are embedded in silenced heterochromatin. There is evidence that histone modifications occurring at the lateral surface of the nucleosome play a substantial role in shaping chromatin structure, yet our understanding of the exact mechanism of action is poor. Here, we address how versatile modifications at Lys31 within the globular domain of histone H4 contribute to genome organization and expression in Apicomplexa. H4K31 acetylation was found at the promoter of active genes. The residue lies where the DNA wraps around the histone and its acetylation may enhance nucleosome disassembly, thereby favoring a more relaxed, open chromatin state. This residue tends also to be monomethylated and depending of the parasite examined different patterns were found. H4K31me1 was enriched in the core body of Toxoplasma active genes, yet its occupancy was inversely correlated with transcripts levels likely because the mark by reducing histone turnover impedes RNA polymerase progression across transcribed units. In contrast to the methylation of H3, it is the first time that a methylated residue of H4 has been clearly associated with transcriptional regulation. In Plasmodium, H4K31me1 was exclusively enriched at transcriptionally inactive genomic regions and peculiarly at pericentromeric heterochromatin, likely to replace the missing H3K9me3 that commonly decorated pericentric nucleosomes in other species.
96

Estudo da utilização de heme por Paracoccidioides lutzii: análise do proteoma de parede celular após exposição à hemoglobina e expressão heteróloga de Pga7, um provável receptor de hemoglobina / Study of the use of heme by Paracoccidioides lutzii: analysis of the cell wall proteome after exposure to hemoglobin and heterologous expression of Pga7, a probable hemoglobin receptor

Souza, Aparecido Ferreira de 21 February 2017 (has links)
Submitted by Erika Demachki (erikademachki@gmail.com) on 2017-03-07T13:37:49Z No. of bitstreams: 4 Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 01.pdf: 17508857 bytes, checksum: 1d04cb16c6e33e54fe0304cecb5e491b (MD5) Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 02.pdf: 14162361 bytes, checksum: b19921eb48893ef7a1aa4ddc2a2e1553 (MD5) Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 03.pdf: 17178000 bytes, checksum: aaf5cfd215078190a7900eafd1e47790 (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) / Approved for entry into archive by Luciana Ferreira (lucgeral@gmail.com) on 2017-03-07T15:14:15Z (GMT) No. of bitstreams: 4 Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 01.pdf: 17508857 bytes, checksum: 1d04cb16c6e33e54fe0304cecb5e491b (MD5) Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 02.pdf: 14162361 bytes, checksum: b19921eb48893ef7a1aa4ddc2a2e1553 (MD5) Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 03.pdf: 17178000 bytes, checksum: aaf5cfd215078190a7900eafd1e47790 (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) / Made available in DSpace on 2017-03-07T15:14:15Z (GMT). No. of bitstreams: 4 Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 01.pdf: 17508857 bytes, checksum: 1d04cb16c6e33e54fe0304cecb5e491b (MD5) Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 02.pdf: 14162361 bytes, checksum: b19921eb48893ef7a1aa4ddc2a2e1553 (MD5) Dissertação - Aparecido Ferreira de Souza - 2017 - Parte 03.pdf: 17178000 bytes, checksum: aaf5cfd215078190a7900eafd1e47790 (MD5) license_rdf: 0 bytes, checksum: d41d8cd98f00b204e9800998ecf8427e (MD5) Previous issue date: 2017-02-21 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPES / Conselho Nacional de Pesquisa e Desenvolvimento Científico e Tecnológico - CNPq / Fundação de Amparo à Pesquisa do Estado de Goiás - FAPEG / Iron (Fe) is an indispensable metal for most biological systems and is a target of competition in host-pathogen interactions. In humans, most Fe is complexed to the cofactor heme, present in hemoglobin, a molecule that is exploited by pathogens as an iron source. Paracoccidioides spp., a complex of thermodymorphic pathogenic fungi, are the etiological agents of paracoccidioidomycosis (PCM), a systemic mycosis endemic in Latin America. Paracoccidioides spp. are able to use hemoglobin in a receptor(PbRbt5)-mediated process. However experimental evidence points to the existence of a complex system with the presence of other proteins. In the present work, we demonstrated the similarity between PAAG_02225 (PbPga7), from Paracoccidioides lutzii, and the sequence of the heme/hemoglobin receptor Pga7 from Candida albicans, and expressed PbPga7 in Escherichia coli. Due to the presence of rare codons in P. lutzii sequence, compared to the codons preferably used by Escherichia coli, chemical synthesis of the gene was employed. The expression of PbPga7 protein opens perspectives for PbPga7 characterization. In addition, nanoUPLC-MSE was employed to analyze P. lutzii cell wall proteome. We observed that the treatment of fungus with hemoglobin promotes induction of potential adhesins and defense-related enzymes against reactive oxygen species. These data indicate that these proteins may be important for the pathogen to access hemoglobin by adhering and lysing erythrocytes, besides counteracting the toxicity generated by heme/hemoglobin released from erythrocytes, allowing the uptake and use of these molecules. The results obtained in the present work reinforce the complexity of the interaction event between pathogen and host and, in addition, contribute to broaden the understanding of the biology of Paracoccidioides spp. / O Ferro (Fe) é um metal indispensável para a maioria dos sistemas biológicos e é alvo de competição em interações patógeno-hospedeiro. Em humanos, a maioria do Fe encontra-se complexada ao cofator heme, presente na hemoglobina, uma molécula que é explorada por patógenos como uma fonte de Fe. Paracoccidioides spp., um complexo de fungos patogênicos termodimórifocos, são agentes etiológicos da paracoccidioidomicose (PCM), uma micose sistêmica endêmica na América Latina. Paracoccidioides spp. é hábil em utilizar hemoglobina por um processo mediado por receptor (PbRbt5). Contudo, evidências experimentais apontam para a existência de um sistema complexo com a presença de outras proteínas. No presente trabalho, foi demonstrada a similaridade de PAAG_02225 (PbPga7), de Paracoccidioides lutzii, com a sequência do receptor de heme/hemoglobina Pga7 de Candida albicans. A expressão heteróloga de PbPga7 foi realizada em Escherichia coli. Devido a presença de códons raros na sequência de P. lutzii, comparados aos códons utilizados preferencialmente por E. coli, a síntese química do gene foi empregada. A expressão da proteína PbPga7 abre perspectivas para estudos de caracterização da mesma. Adicionalmente, nanoUPLC-MSE foi utilizada para analisar o proteoma de parede celular de P. lutzii. Observou-se que o tratamento do fungo com hemoglobina promove a regulação positiva de potenciais adesinas e enzimas relacionadas com a defesa contra espécies reativas de oxigênio. Estes dados indicam que estas proteínas podem ser importantes para que o patógeno possa acessar a hemoglobina, aderindo e lisando eritrócitos, além de contrapor a toxicidade gerada pelo heme/hemoglobina liberados, permitindo a captação e utilização dessas moléculas. Os resultados obtidos no presente trabalho reiteram a complexidade do evento de interação entre patógeno e hospedeiro e, adicionalmente, contribuem para a ampliação do entendimento da biologia de Paracoccidioides spp.
97

Epidemiologia da vassoura-de-bruxa (Crinipellis perniciosa (STAHEL) Singer) em cacaueiros enxertados em Uruçuca, BA. / Epidemiology of witches' broom (Crinipellis perniciosa (STAHEL) Singer) on grafted cocoa in Uruçuca, BA.

Silvio André Meirelles Alves 22 January 2003 (has links)
A vassoura-de-bruxa é a doença mais importante da cultura do cacaueiro, nos países onde ela ocorre. Em 1989 foi constatada pela primeira vez a presença do patógeno causador dessa doença na principal região produtora do Brasil. A falta de medidas de controle eficientes resultou, nos últimos anos, em menor produção, mudanças no uso da terra, venda de propriedades, diminuição do nível de emprego e danos ao meio ambiente. Em vista do pouco conhecimento sobre aspectos epidemiológicos da doença nas condições do sudeste da Bahia, elaborou-se o presente trabalho com os seguintes objetivos: estudar o gradiente de infecção da vassoura-de-bruxa em ramos e frutos em cacaueiros enxertados; comparar o efeito de genótipos e três tratamentos (poda fitossanitária semestral, poda fitossanitária mensal e poda fitossanitária aliada a aplicação de fungicida mensais) no controle da doença; estudar o progresso da vassoura-de-bruxa no tempo, quantificado em ramos e frutos doentes. O experimento foi conduzido em Uruçuca, BA, em área contendo 16 genótipos diferentes, adjacente a uma área com cacaueiros abandonados com alta incidência da doença. A área experimental foi dividida em três partes, as quais receberam os seguintes tratamentos: poda fitossanitária semestral, poda fitossanitária mensal e poda fitossanitária aliada a aplicação de fungicida mensal. Pelo menos uma vez por mês foram contados os ramos e frutos com vassoura. Os resultados mostraram a ausência de evidência clara da existência de gradiente de doença. Os níveis de resistência genética à vassoura-de-bruxa de ramos e frutos não foram correlacionados entre si. Houve bom ajuste do progresso da doença ao modelo monomolecular. As menores taxas de crescimento foram obtidas no tratamento com poda e aplicação de fungicida mensal. O tratamento que combinou poda e pulverização com fungicida apresentou diferença significativa na redução do percentual de frutos com vassoura. Os genótipos NO-34, NO-17 e NO-02 foram os que apresentaram menores percentagens de frutos com vassoura, sendo significativamente diferentes dos genótipos NO-24 e NO-13. / Witches' broom is the most important disease of cocoa, in the countries where it occurs. In 1989, it was verified for the first time the presence of the pathogen in the main producing area of Brazil. The lack of efficient control measures resulted, in the last years, in losses in the production, changes in the use of the soil, sale of properties, decrease of the employment level and damages to the environment. In view of the little knowledge on epidemic aspects of the disease in the conditions of the southeast of Bahia, the present work was elaborated with the following objectives: to study the gradient of the witches' broom infection in flushes and pods in grafted cocoa; to compare the effect of genotypes and three treatments (half-yearly phytosanitation, monthly phytosanitation and monthly phytosanitation allied to fungicide application) in the control of the disease; to study the witches' broom temporal progress, quantified in flushes and pods. Trials were carried out in Uruçuca, BA, in area contends 16 different genotypes, adjacent an area with abandoned cocoa with high incidence of the disease. The experimental area was divided in three parts, which received the following treatments: half-yearly phytosanitation, monthly phytosanitation and monthly phytosanitation allied to fungicide application. At least once a month, flushes and pods with broom were counted. Results showed the absence of clear evidence of the existence of disease gradient. The levels of genetic resistance to the witches' broom of flushes and pods were not correlated to each other. There was good adjustment of progress of the disease to the monomolecular model. The smallest growth rates were obtained in the treatment with monthly phytosanitation and fungicide application. The treatment that allied phytosanitation and fungicide application presented significant difference in the reduction of the percentage of witches' broom infected pods. The genotypes NO-34, NO-17 and NO-02 presented smaller percentages of diseased pods, being significantly different from the genotypes NO-24 and NO-13.
98

Etude comparative des interactions Vibrio - phagocytes dans l'environnement marin / Comparative study of Vibrio - phagocytes interactions in marine environment

Poirier, Aurore 15 December 2015 (has links)
Des souches de Vibrio appartenant au clade Splendidus sont retrouvées de manière récurrente lors des mortalités estivales d’huîtres juvéniles. La souche V. tasmaniensis LGP32 est un pathogène intracellulaire facultatif des hémocytes d’huître, dont elle altère les fonctions de défense. Nous nous intéressons ici aux interactions entre les phagocytes et V. tasmaniensis LGP32, à diverses échelles (moléculaire, cellulaire et environnementale). Dans une première partie, nous avons découvert un mécanisme antimicrobien, encore inconnu chez C. gigas : la formation de pièges d'ADN extracellulaire (ETs). Ces ETs sont associés à des histones antimicrobiennes et sont capables de piéger des bactéries. Comme chez les vertébrés, la formation de ces ETs est dépendante de la production d'espèces réactives de l'oxygène. De plus, la présence de ces ETs a été confirmée in vivo et a été associée à une accumulation d'histones antimicrobiennes dans les tissus, suite à une blessure ou à une infection. Dans une seconde partie,nous avons étudié les interactions entre V. tasmaniensis LGP32 et des protistes hétérotrophes présents dans l’environnement des huîtres, tels que les amibes et les ciliés, qui se nourrissent de micro-organismes par phagocytose. Un résultat important de cette thèse a été de montrer que V. tasmaniensis LGP32 résiste également à la phagocytose des protistes hétérotrophes environnementaux, de manière intracellulaire. C'est à notre connaissance la première fois que les mécanismes d’interaction entre des bactéries pathogènes d'origine marine et des amibes marines sont décrits. Les amibes que nous avons isolées étant présentes dans l'environnement direct des huîtres, nous pouvons donc supposer que la pression de sélection exercée par les phagocytes environnementaux pourrait favoriser l’émergence de traits de virulence et/ou de résistance à la phagocytose parmi les bactéries marines, comme c’est le cas pour V. tasmaniensis LGP32. / Vibrio strains belonging to the Splendidus clade have been repeatedly found in juvenile diseased oysters affected by summer mortalities. V. tasmaniensis LGP32 is an intracellular pathogen of oyster hemocytes which has been reported to alter the oxidative burst and inhibit phagosome maturation.We here focus on the interactions between phagocytes and V. tasmaniensis LGP32, at molecular, cellular and environmental scales. In the first part of this work, we uncover anunknown antimicrobial mechanism of C. gigas hemocytes: the formation of DNA extracellular traps (ETs). These ETs are associated with antimicrobial histones and are able to entrap bacteria. As in vertebrates, ETs formation depends on reactive oxygen species production. In addition, the presence of ETs was confirmed in vivo and has been associated with antimicrobial histones accumulation in tissues, in response to injury or infection. In the second part of this work, we studied the interactions between V. tasmaniensis LGP32 and heterotrophic protists found in the oyster’s environment, such as amoebae and ciliates, which feed on microorganisms by phagocytosis. An important result of this workwas that V. tasmaniensis LGP32 resists to phagocytosis by environmental heterotrophic protists, as well as to oyster hemocytes. To our knowledge, this is the first mechanical description of an interaction between marine amoebae and marine pathogenic bacteria. As the amoebae were isolated from the direct environment of oysters, we can presume that the selective pressure exerted by environmental phagocytes could select for virulence and/or phagocytosis resistance traits in marine bacteria as in the case of V. tasmaniensis LGP32.
99

A computational framework for transcriptome assembly and annotation in non-model organisms: the case of venturia inaequalis

Kimbung, Stanley Mbandi January 2014 (has links)
Philosophiae Doctor - PhD / In this dissertation three computational approaches are presented that enable optimization of reference-free transcriptome reconstruction. The first addresses the selection of bona fide reconstructed transcribed fragments (transfrags) from de novo transcriptome assemblies and annotation with a multiple domain co-occurrence framework. We showed that selected transfrags are functionally relevant and represented over 94% of the information derived from annotation by transference. The second approach relates to quality score based RNA-seq sub-sampling and the description of a novel sequence similarity-derived metric for quality assessment of de novo transcriptome assemblies. A detail systematic analysis of the side effects induced by quality score based trimming and or filtering on artefact removal and transcriptome quality is describe. Aggressive trimming produced incomplete reconstructed and missing transfrags. This approach was applied in generating an optimal transcriptome assembly for a South African isolate of V. inaequalis. The third approach deals with the computational partitioning of transfrags assembled from RNA-Seq of mixed host and pathogen reads. We used this strategy to correct a publicly available transcriptome assembly for V. inaequalis (Indian isolate). We binned 50% of the latter to Apple transfrags and identified putative immunity transcript models. Comparative transcriptomic analysis between fungi transfrags from the Indian and South African isolates reveal effectors or transcripts that may be expressed in planta upon morphogenic differentiation. These studies have successfully identified V. inaequalis specific transfrags that can facilitate gene discovery. The unique access to an in-house draft genome assembly allowed us to provide preliminary description of genes that are implicated in pathogenesis. Gene prediction with bona fide transfrags produced 11,692 protein-coding genes. We identified two hydrophobin-like genes and six accessory genes of the melanin biosynthetic pathway that are implicated in the invasive action of the appressorium. The cazyome reveals an impressive repertoire of carbohydrate degrading enzymes and carbohydrate-binding modules amongst which are six polysaccharide lyases, and the largest number of carbohydrate esterases (twenty-eight) known in any fungus sequenced to date
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Identification du système de transformation naturelle de Legionella pneumophila / Identification of the DNA uptake system of Legionella pneumophila

Juan, Pierre-Alexandre 16 December 2015 (has links)
Sous des conditions de croissance particulières, certaines bactéries sont capables d'entrer en état de « compétence » pour la transformation naturelle, c'est-à-dire d'exprimer un ensemble de gènes nécessaires à la mise en place d'un système d'import d'ADN exogène dont l'intégration conduit à une transformation génétique et phénotypique. C'est le cas de Legionella pneumophila, bactérie environnementale et agent étiologique de la légionellose. La transformation naturelle a potentiellement participé à l'évolution du génôme de L. pneumophila.Ainsi, l'objectif premier de cette thèse était de décrire les composants principaux du système de transformation naturelle de L. pneumophila, ainsi que son activation et rôle potentiel dans la relation de la bactérie avec ses hôtes. Des méthodes d'analyse transcriptomique et de mutagénèse dirigée ont permis d'identifier les principaux gènes impliqués dans la mise en place du système de transformation naturelle qui, de façon cohérente avec un rôle adaptatif, ne semble pas impliqué dans la virulence bactérienne. Le système inclut un pilus de transformation, structure fréquemment observée chez les espèces naturellement transformables. Le rôle de la protéine structurale MreB dans le mécanisme de transformation naturelle a également été étudié. En proposant un premier modèle du système de transformation naturelle de L. pneumophila, ces travaux ouvrent la voie à une analyse plus détaillée de la dynamique du système et, plus généralement, à une meilleure compréhension des mécanismes de la transformation naturelle chez les bactéries Gram-négatives / Under certain growth conditions, some bacteria are able to develop a « competence » state for natural transformation, that is, to express a panel of genes involved in the assembly of a DNA uptake system that allows bacteria to take up and recombine free exogenous DNA, leading to a genetic and phenotypic transformation. Natural transformation may have played a role in the evolution of the L. pneumophila genome.Thus, the main objective of this work was to describe the main components of the L. pneumophila DNA uptake system and to investigate its role regarding the host-pathogen interaction. Transcriptomic analysis and directed mutagenesis permitted to identify the main components of the system which is not involved in bacterial virulence. The system include a transformation pilus that is a structure frequently found in transformable species. The role of the structural protein MreB has also been investigated.By describing a first model of the natural transformation system of L. pneumophila, this work paves the way to a deeper analysis of the system dynamics and, more generally, to a better understanding of natural transformation in Gram-negative species

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