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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.
31

Investigating the regulation of host tissue colonisation by the rice blast fungus Magnaporthe oryzae

Sakulkoo, Wasin January 2016 (has links)
The filamentous fungus Magnaporthe oryzae is a devastating pathogen of cultivated rice. M. oryzae elaborates a pressurized dome-shaped infection structure, called the appressorium, which physically ruptures the cuticle and gains entry into host tissue. Intracellular invasive hyphae invade neighbouring host cells through plasmodesmata. The Pmk1 MAPK cascade is well known for its roles in regulating the formation and function of the appressorium. Interestingly, ∆pmk1 mutants cannot infect host plant tissue through wounds, suggesting a role in invasive growth. Here, I define biological functions of the Pmk1 MAPK at various stages of the life cycle, by using a controllable version of Pmk1 that is specifically inhibited by a cell-permeable compound without disturbing other wild-type kinases. The Pmk1 MAPK signalling regulates morphogenesis of narrow invasive hyphae traversing the host cell wall, and modulates production of several putative secreted effectors, providing a direct link between the signalling cascade and effector-driven host immune suppression. These results indicate that the Pmk1 pathway is a central regulator of infection-related development necessary for many stages of plant infection including appressorium development, plant penetration, and importantly tissue colonisation. I also report the role of cell cycle progression in the development of plant infection structure. By using two novel conditional mutants that arrest in S and G2 phases, I defined that S-phase progression is crucial for appressorium-mediated plant penetration.
32

Unraveling the mechanisms of Sr35-based resistance in the wheat-Puccinia graminis f.sp. tritici pathosystem

Salcedo, Andrés Felipe January 1900 (has links)
Doctor of Philosophy / Department of Plant Pathology / Eduard Akhunov / The fungus Puccinia graminis f. sp. tritici (Pgt) is the causal agent of the wheat stem rust disease. Wheat stem rust has attracted a lot of attention after the emergence of the Ug99 race group, which at the time of its origin was virulent on most of the wheat varieties cultivated around the world. The evolution and spread of the Pgt isolates from the Ug99 race group posed a serious threat to worldwide wheat production. To mitigate the potential impact of new rust epidemics in major wheat production areas, it remains critical to identify new strategies for breeding durable resistance traits. A detailed understanding of the plant-pathogen interaction mechanisms in the wheat-Pgt pathosystem should be the foundation of these strategies. The interaction between the matching pair of resistance (R) and avirulence (Avr) genes, an important element of the plant-pathogen interactions, is described by the broadly documented gene-for-gene model. The cloning of the Sr35 gene, which confers near immunity against all isolates from the Ug99 race group provided a unique opportunity to investigate the molecular mechanisms of resistance to stem rust in wheat. The goals of the present study were: (1) to determine whether the Sr35 gene alone is sufficient for conferring resistance against Ug99, (2) to assess the Sr35 transcript levels during the time course of infection, and (3) to identify and validate the corresponding Avr gene interacting with Sr35. The cloning of Avr genes from the biotrophic fungi represents a substantial challenge due to the variability, redundant nature, the lack of similarity to known proteins, and lack of adequate functional tools to validate them. To overcome these limitations, we performed a comparative genomic analysis using multiple Sr35-avirulent and Sr35-virulent races, including 15 chemically mutagenized Pgt strains that acquired virulence on the Sr35 gene. Whole genome shotgun sequencing of the Pgt mutants identified a single candidate gene, which carried strong effect mutations in each mutant strain. The Avr gene candidate (AvrSr35) was expressed at early stages of infection and had a signal peptide indicating that the gene product is secreted. Comparative microscopic analysis of the infected tissues at different time points after infection indicated that AvrSr35 secretion occurs before haustoria formation. The re-sequencing of the AvrSr35 candidate gene in a panel of Sr35-virulent and Sr35-avirulent isolates including isolates from the Ug99 race group, revealed the presence of a mobile DNA element inserted into the coding sequence of virulent isolates. This insertion resulted in a premature termination codon and explains the origin of Pgt field isolates virulent in the presence of the Sr35 gene. Co-expression of AvrSr35 with the Sr35 in N. benthamiana leaves induced a specific hypersensitive response confirming the avirulence function of the candidate effector gene. Subcellular localization, bi-molecular fluorescence complementation, and co-immunoprecipitation assays in N. benthamiana leaves revealed that the AvrSr35 and Sr35 proteins interact and are likely associated with the endoplasmic reticulum and plasma membrane. Thus, this study identified and functionally characterized the first matching pair of Avr/R genes for cereal rusts.
33

Functional characterization of a subset (RipAX2, RipH2, RipHS and RipG7) of type III effectors from Ralstonia solanacearum / Analyse fonctionnelle des effecteurs de type III (RipAX2, RipH2, RipH3 et RipG7) de la bactérie phytopathogène Ralstonia solanacearum

Wang, Keke 05 October 2015 (has links)
La bactérie phytopathogène du sol, Ralstonia solanacearum cause la maladie du flétrissement bactérien sur un grand nombre de plante hôtes. Un des déterminants clefs de son pouvoir pathogène est le système de sécrétion de type III. Celui-ci permet à la bactérie d'injecter des protéines directement dans les cellules de l'hôte. Dans ma thèse je me suis attaché à décrire et analyser finement la contribution au pouvoir pathogène de la bactérie de certains de ces substrats de l'appareil de sécrétion de type III (RipAX2, RipH2, RipH3 et RipG). Des expériences de double-hybride nous ont permis d'identifier des protéines des plantes hôtes pouvant être ciblées par ces effecteurs de type III. Dans une autre partie de mon travail j'ai contribué à l'étude de RipAX2 qui est induit spécifiquement la résistance dans des lignées d'aubergines porteur d'un locus de résistance. J'ai également travaillé sur l'identification des cellules de plantes soumises à l'injection de type III dans une interaction compatible. Pour cela j'ai utilisé la plante hôte Medicago truncatula, en exprimant dans certaines lignées cellulaires un effecteurs (RipG7) pour lequel nous avions démontré que son expression constitutive das M. truncatula pouvait restaurer l'infection de ces plantes par un mutant bactérien dans ce même effecteur. Enfin, j'ai aussi contribué à l'analyse structure-fonction fine de l'effecteur RipG7 dans sa fonction de contribution au pouvoir pathogène de R. solanacearum sur la plante hôte M. truncatula. Ce travail nous a permis d'identifier les acides aminés de RipG7 qui sont sous sélection positive, et parmi ceux-là, ceux qui contribuent directement à la fonction de RipG7 sur M. truncatula. / The soil-borne pathogen Ralstonia solanacearum causes bacterial wilt in a broad range of plants. The type III secretion system (T3SS) and its associated type III effectors (T3Es) are the main virulence determinants of R. solanacearum. In my PhD study, to understand the mode of action of several "core" effectors (RipH2, RipH3, RipG7, RipG6) from R. solanacearum in host cells. We performed yeast two-hybrid screening of plant cDNA library to identify their protein targets. Besides, we also collaborated on the identification and characterization of a specific type III effector RipAX2 which is an avirulence factor that triggers a hypersensitive response in specific Eggplant lines. To understand which plant root cells are actually subjected to type III injection during the compatible interaction, I have generated transiently transformed Medicago truncatula lines (hairy root), expressing a host specificity and core T3E RipG7 in different root cell layers. When the transformed plant expressing RipG7 under 35S promoter, the plant can be infected and colonized by the ripG7 single mutant strain. The study could be refined by using specific root cell layer promoter to identify the root cell layers that are key players in this interaction. We also worked on the characterization of the structure-function of RipG7 from R. solanacearum. Our work revealed the genetic and functional variation of RipG7. Furthermore, positive selection study and mutagenesis analysis enabled us to identify essential functional residues which likely to have been differentially selected during the host-pathogen co-evolution. The potential plant targets of RipG7 were also studies further in our study by differential yeast two-hybrid.
34

Diarrheagenic Escherichia coli signaling and interactions with host innate immunity and intestinal microbiota

Wang, Gaochan January 1900 (has links)
Doctor of Philosophy / Department of Diagnostic Medicine/Pathobiology / Philip R. Hardwidge / Diarrheagenic Escherichia coli (E. coli) strains are common etiological agents of diarrhea. Diarrheagenic E. coli are classified into enterotoxigenic E. coli (ETEC), Shiga toxin-producing E. coli (STEC or enterohemorrhagic E. coli [EHEC]), enteropathogenic E. coli (EPEC), enteroinvasive E. coli (EIEC), enteroaggregative E. coli (EAEC), diffuse-adherent E. coli (DAEC), and adherent invasive E. coli (AIEC). In addition to encoding toxins that cause diarrhea, diarrheagenic E. coli have evolved numerous strategies to interfere with host defenses. In the first project, we identified an ETEC-secreted factor (ESF) that blocked TNF-induced NF-[kappa]B activation. One of the consequences of TNF-induced NF-[kappa]B activation is the production of pro-inflammatory cytokines that help to eliminate pathogens. Modulation of NF-[kappa]B signaling may promote ETEC colonization of the host small intestine. In this study, we fractionated ETEC supernatants and identified flagellin as necessary and sufficient for blocking the degradation of the NF-[kappa]B inhibitor I[kappa]B[alpha] in response to TNF[alpha]. In the second project, we attempted to identify an ETEC cAMP importer. ETEC diarrhea leads to cAMP release into the lumen of the small intestine. cAMP is a key secondary messenger that regulates ETEC adhesin expression. We hypothesized that a cAMP importer is present in ETEC, accounting for its hypersensitivity to extracellular cAMP. We used Tn5 transposome-mediated mutagenesis to construct a mutant library and screen for cAMP-hyporesponsive mutants. However, none of the 17,956 mutants we screened were cAMP-hyporesponsive. In the third project, we focused on gut microbiota and the T3SS effector NleH. We used the mouse-specific pathogen C. rodentium and transplanted performed microbiota between different mouse strains. We evaluated microbiota populations as a function of infection with WT and [Delta]nleH C. rodentium strains before and after microbiota transplantation. Microbiota transfer altered the resistance to WT C. rodentium infection in C57BL/10ScNJ mice and the NleH effector promoted host resistance to C. rodentium.
35

Effector identification from the susceptible Exserohilum turcicum – Zea mays interaction

Human, Maria Petronella January 2019 (has links)
Exserohilum turcicum is the hemibiotrophic causal agent of Northern leaf blight of maize and sorghum. Despite the global importance of this yield-limiting pathogen, knowledge regarding genes contributing to disease development and race-specificity is limited. Therefore, this study aimed to identify genes involved in host colonization during biotrophic and necrotrophic phases of infection, as well as race-specific differences in gene expression. RNAseq of maize seedlings inoculated with a race 13N or 23N E. turcicum isolate was conducted to identify genes contributing to fungal pathogenicity, and expression was validated for four effector candidates. A population genetic study was undertaken of isolates from maize and sorghum to select isolates for sequencing of three putative effectors. Fungal biomass positively correlated with the percentages of E. turcicum reads mapped and indicated a lifestyle switch from biotrophy to necrotrophy between 7 and 13 dpi. Transcriptome sequencing enabled identification of cell wall degrading enzymes, peptidase-encoding genes, secondary metabolite biosynthesis genes and candidate effectors likely contributing to the pathogenicity of E. turcicum. Profiling of Ecp6 and candidate effector SIX13-like revealed increased expression at 5 and 7 dpi compared to 2 and 13 dpi. Evidence of host specificity was obtained from microsatellite haplotypes and sequencing of SIX13-like. Identification of candidate effector SIX13-like is consistent with the colonization of E. turcicum through the xylem of susceptible hosts and possibly indicates specificity of E. turcicum to either maize or sorghum. This study identified E. turcicum genes putatively involved in pathogenicity and describes a hypothetical model of the E. turcicum – maize interaction. / Thesis (PhD)--University of Pretoria, 2019. / The financial assistance of the National Research Foundation (NRF South Africa, grant unique numbers 85847, 88785, 92762 and 93671) toward this research is hereby acknowledged. Opinions expressed and conclusions arrived at, are those of the authors and are not necessarily to be attributed to the NRF. / Plant Science / PhD / Unrestricted
36

Integrace podtlakového koncového efektoru do robotického pracoviště / Vacuum End-Effector Integrated in robotics station

Baják, Zdeněk January 2009 (has links)
The subject of this thesis is to complete the project vacuum end effectors for handling objects plate type. The work includes the completion of a 3D model, drawing, computer simulation uchopovacího positioning system, the draft control system for stepping motors and verification functions of effectors with the industrial robot ABB IRB 4400/60
37

Thermo-effector responses to a 5-day high-intensity cold-acclimation procedure / Termoeffektorsvar på en 5-dagars högintensiv köldanpassningsprocedur

Wilkins, Frederick January 2020 (has links)
Long-term, repeated exposures to cold might lead to cold adaptation. The study examined, in a small homogeneous group of non-acclimatised men, the inter-individual response to a short-term, high-intensity cold acclimation regimen. In particular, six young (24 - 28 years), healthy men performed 5 daily, whole-body (immersed to the chest for up to 120-min) immersions in 14°C water, during which their thermo-effector responses were evaluated. The study also sought to determine whether, or to what extent, any thermoregulatory modifications induced by the repeated severe cold stress would be transferred to acute moderate cold stress immersions (i.e., “transfer” adaptation). Thus, a few days before and after the acclimation protocol, subjects’ thermoregulatory function was assessed during whole-body immersions in 21°C water. During all immersions, thermal (rectal and skin temperatures), cardiorespiratory (oxygen uptake, mean arterial pressure, heart rate) and perceptual (thermal sensation and comfort, pain, affective valence) responses were monitored. The 5-day cold acclimation regimen caused a hypothermic adaptation, which was characterised by: i) a reduction in the cold-induced elevation of endogenous heat production (i.e., oxygen uptake), which was mainly ascribed to a delay in the activation of shivering, ii) an attenuation in the cold-induced increase of arterial pressure and heart rate, and iii) the alleviation of thermal discomfort. Aside from the blunted pressor response, these thermo-adaptive modifications seemed to be transferrable during exposure to a moderate cold stimulus as well. Still, during both cold provocations, the thermoregulatory adjustments were described by a large inter-individual variability, regarding the direction and the magnitude of the response.
38

Measuring Individual Cell Cyclic Di-GMP: Identifying Population Diversity and Cyclic Di-GMP Heterogeneity

Miller, Samuel I., Petersen, Erik 05 March 2020 (has links)
Cyclic di-GMP is a second messenger used by bacteria to regulate motility, extracellular polysaccharide production, and the cell cycle. Recent advances in the measurement of real time cyclic di-GMP levels in single cells have uncovered significant dynamic heterogeneity of second messenger concentrations within bacterial populations. This heterogeneity results in a wide range of phenotypic outcomes within a single population, providing the potential for population survival and adaptability in response to rapidly changing environments. In this chapter, we discuss some of the measurement technologies available for single-cell measurement of cyclic di-GMP concentrations, the resulting discovery of heterogeneous cyclic di-GMP populations, the mechanisms bacteria use to generate this heterogeneity, and the biochemical and functional consequences of heterogeneity on cyclic di-GMP effector binding and the bacterial population.
39

Studies on virulence-related effectors and transcription factors preferentially expressed at the pre-invasion stage in Colletotrichum orbiculare / ウリ類炭疽病菌の侵入前に優先的に発現する病原性関連エフェクターおよび転写因子の研究

Zhang, Ru 26 September 2022 (has links)
京都大学 / 新制・課程博士 / 博士(農学) / 甲第24242号 / 農博第2521号 / 新制||農||1094(附属図書館) / 学位論文||R4||N5413(農学部図書室) / 京都大学大学院農学研究科応用生物科学専攻 / (主査)教授 髙野 義孝, 教授 寺内 良平, 教授 吉田 健太郎 / 学位規則第4条第1項該当 / Doctor of Agricultural Science / Kyoto University / DGAM
40

Planar Cable Direct Driven Robot: Hardware Implementation

Vadia, Jigar January 2003 (has links)
No description available.

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