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Molecular Quest for Avirulence Factors in Venturia inaequalisWin, Joe January 2004 (has links)
The molecular basis for the gene-for-gene relationship of Vm-resistance in apple to Venturia inaequalis was investigated. Incompatible reactions involved a hypersensitive response (HR), which was accompanied by the accumulation of dark brown pigments and autofluorescent materials in epidermal and mesophyll cells at the site of invasion. Cell-free culture filtrates of the avirulent isolate elicited an HR in the Vm host (h5) leaves, but not in the susceptible host (h1). The elicitor activity was resistant to boiling but was abolished by proteinase K digestion. Elicitation of HR was used to monitor purification of the avirulence factor, AVRVm, from liquid cultures of the avirulent isolate following ultrafiltration, acetone precipitation and ion-exchange chromatography. The purest fraction contained three major proteins all with low isoelectric points (pI 3.0-4.5). The fraction also elicited HR on the differential host h4, but not on other resistant hosts (h2, h3 and h6) tested. Three candidate AVRVm proteins were identified and amino acid sequences were obtained using Edman degradation and mass spectrometry. Nucleotide sequences corresponding to these proteins were found in databases of V. inaequalis expressed sequence tags. There were no polymorphisms evident between avirulent and virulent isolates (representing races 1 and 5 respectively) either at genomic DNA or cDNA level of the full open reading frames. RT-PCR revealed that all genes were expressed in both avirulent and virulent isolates during in vitro and in planta growth. All three genes showed similar levels of expression between avirulent and virulent isolates during their in vitro growth. However, preliminary RT-PCR experiments showed that two of these genes were likely to be expressed at lower levels in the virulent compared with the avirulent isolate during compatible infection. Implications of this difference in expression and the future experiments to identify the genuine AvrVm gene were discussed.
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Bacterial Endophytes from Pioneer Desert Plants for Sustainable AgricultureEida, Abdul Aziz 06 1900 (has links)
One of the major challenges for agricultural research in the 21st century is to increase crop productivity to meet the growing demand for food and feed. Biotic (e.g. plant pathogens) and abiotic stresses (e.g. soil salinity) have detrimental effects on agricultural productivity, with yield losses being as high as 60% for major crops such as barley, corn, potatoes, sorghum, soybean and wheat, especially in semi-arid regions such as Saudi Arabia. Plant growth promoting bacteria isolated from pioneer desert plants could serve as an eco-friendly, sustainable solution for improving plant growth, stress tolerance and health. In this dissertation, culture-independent amplicon sequencing of bacterial communities revealed how native desert plants influence their surrounding bacterial communities in a phylogeny-dependent manner. By culture-dependent isolation of the plant endosphere compartments and a number of bioassays, more than a hundred bacterial isolates with various biochemical properties, such as nutrient acquisition, hormone production and growth under stress conditions were obtained. From this collection, five phylogenetically diverse bacterial strains were able to promote the growth of the model plant Arabidopsis thaliana under salinity stress conditions in a common mechanism of inducing transcriptional changes of tissue-specific ion transporters and lowering Na+/K+ ratios in the shoots. By combining a number of in vitro bioassays, plant phenotyping and volatile-mediated inhibition assays with next-generation sequencing technology, gas chromatography–mass spectrometry and bioinformatics tools, a candidate strain was presented as a multi-stress tolerance promoting bacterium with potential use in agriculture. Since recent research showed the importance of microbial partners for enhancing the growth and health of plants, a review of the different factors influencing plant-associated microbial communities is presented and a framework for the successful application of microbial inoculants in agriculture is proposed. The presented work demonstrates a holistic approach for tackling agricultural challenges using microbial inoculants from desert plants by combining culturomics, phenomics, genomics and transcriptomics. Microbial inoculants are promising tools for studying abiotic stress tolerance mechanisms in plants, and they provide an eco-friendly solution for increasing crop yield in arid and semi-arid regions, especially in light of a dramatically growing human population and detrimental effects of global warming and climate change.
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The Environmental Microbiome In A Changing World: Microbial Processes And BiogeochemistryJuice, Stephanie 01 January 2020 (has links)
Climate change can alter ecosystem processes and organismal phenology through both long-term, gradual changes and alteration of disturbance regimes. Because microbes mediate decomposition, and therefore the initial stages of nutrient cycling, soil biogeochemical responses to climate change will be driven by microbial responses to changes in temperature, precipitation, and pulsed climatic events. Improving projections of soil ecological and biogeochemical responses to climate change effects therefore requires greater knowledge of microbial contributions to decomposition. This dissertation examines soil microbial and biogeochemical responses to the long-term and punctuated effects of climate change, as well as improvement to decomposition models following addition of microbial parameters.
First, through a climate change mesocosm experiment on two soils, I determined that biogeochemical losses due to warming and snow reduction vary across soil types. Additionally, the length of time with soil microbial activity during plant dormancy increased under warming, and in some cases decreased following snow reduction. Asynchrony length was positively related to carbon and nitrogen loss. Next, I examined soil enzyme activity, carbon and nitrogen biodegradability, and fungal abundance in response to ice storms, an extreme event projected to occur more frequently under climate change in the northeastern United States. Enzyme activity response to ice storm treatments varied by both target nutrient and, for nitrogen, soil horizon. Soil horizons often experienced opposite response of enzyme activity to ice storm treatments, and increasing ice storm frequency also altered the direction of the microbial response. Mid-levels of ice storm treatment additionally increased fungal hyphal abundance. Finally, I added explicit microbial parameters to a global decomposition model that previously incorporated climate and litter quality. The best mass loss model simply added microbial flows between litter quality pools, and addition of a microbial biomass and products pool also improved model performance compared to the traditional implicit microbial model.
Collectively, these results illustrate the importance of soil characteristics to the biogeochemical and microbial response to both gradual climate change effects and extreme events. Furthermore, they show that large-scale decomposition models can be improved by adding microbial parameters. This information is relevant to the effects of climate change and microbial activity on biogeochemical cycles.
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Elucidating three novel mechanisms of Pseudomonas syringae pathogenicityClarke, Christopher R. 12 March 2012 (has links)
Pseudomonas syringae is an important bacterial plant pathogen that, as a species, is known to cause disease on hundreds of different plant species. However, any individual pathovar of P. syringae typically only causes disease on one or a few plant species, which constitute the host range of the pathovar. Plants are generally resistant to most pathogens primarily because the plant innate immune system is capable of recognizing conserved microbial-associated molecular patterns (MAMPs). Adapted pathovars of P. syringae secrete effector proteins through a Type Three Secretion System (T3SS) to suppress the immune response elicited by their MAMPs. However, secretion of effectors can also trigger a strong plant immune response if the plant harbors resistance proteins capable of recognizing the secreted effectors. Successful pathovars, therefore, must secrete a combination of effectors capable of suppressing MAMP/Pattern-Triggered Immunity (PTI) without eliciting Effector-Triggered Immunity. Here we identify several novel strategies employed by P. syringae to overcome the plant immune system and cause disease. First, we demonstrate that, in place of the canonical T3SS used by all known pathogens of P. syringae, several apparently nonpathogenic isolates of P. syringae employ a novel T3SS that is functional but not necessary for colonization of plants. Despite being closely related to pathogenic isolates of P. syringae, the isolates employing the noncanonical T3SS do not cause disease on any tested plants and instead appear to act more as commensal organisms. Second, we advance the understanding of PTI by identifying a second region of bacterial flagellin that triggers PTI in addition to the archetypical MAMP flg22, which is recognized by the archetypical plant receptor FLS2. This new elicitor, termed flgII-28, is also detected by FLS2 and appears to be under selection in very closely related lineages of P. syringae. Alleles of flagellin present in one recently expanded and agriculturally problematic lineage of P. syringae appear to trigger less PTI on their host plant, tomato, than the ancestral allele suggesting that avoidance of PTI through allelic diversity in MAMPs is an effective alternative strategy to suppression of PTI through delivery of effectors. Finally, we start to elucidate a role for chemotaxis (chemical-directed movement) in P. syringae pathogenicity. Not only is chemotaxis required for pathogenicity of P. syringae on plants, but it also appears to contribute to delimiting the host range of several P. syringae pathovars. These results highlight that additional aspects of P. syringae pathogenicity, such as chemotaxis, can directly contribute to defining the host range of individual P. syringae pathovars. The current paradigm of P. syringae pathogenicity posits that MAMPS and the repertoire of effector proteins are the primary determinant of the host range of any P. syringae pathovar; in contrast these results inspire a more nuanced view of pathogenicity that considers multiple aspects of the infection process. / Ph. D.
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Genome-enabled discovery and characterization of type III effector-encoding genes of plant symbiotic bacteriaKimbrel, Jeffrey A. 13 March 2012 (has links)
Symbiosis is the close and protracted interaction between organisms. The molecular interactions that occur during symbiosis are complex with multiple barriers that must be overcome. Many Gram-negative, host-associated bacteria use a type III secretion system to mediate associations with their eukaryotic hosts. This secretion system is a specialized apparatus for the injection of type III effector proteins directly into host cells, which in the case of plant pathogens, are collectively necessary to modulate host defense. The type III secretion system is not a mechanism exclusive to pathogens, however, as many strains of commensal Pseudomonas fluorescens and mutualistic rhizobia demonstrably require a type III secretion system to interact with their host plants. The work presented in this thesis describes genome-enabled approaches for characterizing type III effector genes across the range of plant symbiosis. Using high-throughput sequencing technology, draft genome sequences were generated for the plant pathogen, Xanthomonas hortorum pv. carotae M081, the plant commensal, Pseudomonas fluorescens WH6, and six strains from the plant mutualists Sinorhizobium fredii and Bradyrhizobium japonicum. Analyses of the draft genome sequences and publicly available finished sequences contributed insights into mechanisms of host-association and to increasing the inventory of type III effector sequences as well as developing methods directly applicable for agriculture. Finally, characterization of the genetic diversity of type III effectors from rhizobia shows that collections of type III effectors of mutualists are static, with little diversity in content and sequence variation. This represents the first comprehensive cataloging of type III effector from species of mutualistic bacteria and the first to provide evidence for purifying selection of this important class of genes. / Graduation date: 2012
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Vliv rostlin na strukturu, funkci a diverzitu společenstev bakterií / Effects of plants on the structure, function and diversity of bacterial communitiesHavlíčková, Petra January 2018 (has links)
Vegetation is known to influence the composition of microbial communities. Bacteria can act as roots symbionts or be involved in the decomposition of plant biomass. They can be influenced by soil chemistry but also by plant exudates. Some plants produce targeted exudates to attract specific bacteria to their roots. Bacteria associate with plants frequently but the effect of plant diversity on bacterial communities on their roots and in the surrounding soil remains unclear. The aim of this work was to describe the relationship between the diversity and community composition of bacteria and the diversity of vegetation in forest and grassland ecosystems. The study areas were selected to represent a gradient of vegetation in Bohemian Forest NP and in White Carpathian flowery grasslands. I hypothesized that the diversity and evenness of bacterial community increase with increasing plant diversity. The composition of bacterial community was characterized by 16S rRNA sequencing. The composition of vegetation was determined by phytocenological relevées and by molecular markers trnL. In grassland ecosystem, there was a positive relationship between plant and bacterial diversity only in shoots. The space and vegetation were identified as an important drivers of bacterial community composition in shoots. The...
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Comprendre l’implication des effecteurs fongiques dans l’infection d’une plante hôte : caractérisation fonctionnelle d’effecteurs de Leptosphaeria maculans, un champignon pathogène du colza / Understanding the Involment of Fungal Effectors during Infection : Functional Characterization of Leptosphaeria Maculans Effectors, a Fungal Pathogen of Oilseed RapePetit, Yohann 18 December 2017 (has links)
Pendant l’infection, les agents phytopathogènes sécrètent un arsenal de molécules, appelées effecteurs, éléments clés de la pathogénie qui modulent l’immunité innée de la plante et facilitent l’infection. Leptosphaeria maculans est le champignon responsable de la nécrose du collet du colza. Plus de 650 gènes codant des effecteurs potentiels ont été identifiés dans son génome, dont 7 ont un rôle reconnu dans l’avirulence du champignon. Les effecteurs fongiques correspondent principalement à de petites protéines potentiellement sécrétées (PPS), n’ayant pas d’homologues dans les bases de données et pas de motifs connus. Par conséquent, leur fonction biologique est difficile à prédire, et très peu de choses sont connues sur le mode d’action des effecteurs de L. maculans au cours de l’infection.L’objectif de ma thèse était de caractériser fonctionnellement des effecteurs de L. maculans afin de mieux comprendre leur rôle au cours du processus infectieux. Cette caractérisation fonctionnelle a consisté en : i) la détermination de la localisation subcellulaire de ces effecteurs dans Nicotiana benthamiana et Arabidopsis thaliana ; ii) la recherche de cibles végétales ciblées par ces effecteurs ; et iii) la détermination des processus cellulaires impactés par ces effecteurs par expression stable dans A. thaliana et tests de suppression de mort cellulaire dans N. benthamiana. Quatre effecteurs ont été choisis pour cette étude : AvrLm10-1, AvrLm10-2, AvrLm4-7 et AvrLm3.AvrLm10-1 et AvrLm10-2 sont tous les deux nécessaires pour induire une reconnaissance par le gène de résistance Rlm10. Des orthologues d’AvrLm10-1 et AvrLm10-2 ont été identifiés chez des Dothidéomycètes et des Sordariomycètes phytopathogènes ainsi que plusieurs paralogues exprimés spécifiquement pendant l’infection chez L. maculans. AvrLm10-1 et AvrLm10-2 présentent toutes les deux une localisation nucléo-cytoplasmique. Une interaction physique entre AvrLm10-1 et AvrLm10-2 a été mise en évidence, ainsi qu’une interaction potentielle de ces deux protéines avec une protéine PR1 (Pathogenesis-related 1) et une cystéine-protéase végétale.AvrLm4-7 est reconnu par deux gènes de résistance, Rlm4 et Rlm7, et sa présence empêche la reconnaissance d’AvrLm3 par Rlm3. AvrLm4-7 est capable de supprimer la mort cellulaire provoquée aussi bien par des inducteurs généraux de la mort cellulaire que par des inducteurs de la PAMP-Triggered Immunity (PTI) et de l’Effector-Triggered Immunity (ETI). AvrLm4-7 présente une localisation nucléo-cytoplasmique, qu’il soit exprimé avec ou sans son peptide signal, ce qui suggère un mode d’action intracellulaire. AvrLm4-7 interagit potentiellement avec une protéine ribosomale végétale, de la même manière qu’un effecteur de Blumeria graminis avec lequel il partage des analogies structurales. Cependant, des lignées d’A. thaliana exprimant AvrLm4-7 de façon constitutive ne présentent aucune différence morphologique ou de sensibilité aux maladies comparativement à l’écotype sauvage Col0.AvrLm3 est un gène d’avirulence très conservé dans les populations de L. maculans dont la reconnaissance par le gène de résistance Rlm3 est supprimée en présence d’AvrLm4-7. AvrLm3 est capable de supprimer la mort cellulaire associée à la PTI et à l’ETI. Cet effecteur est localisé dans l’apoplasme des cellules foliaires lorsqu’il est exprimé avec son peptide-signal, suggérant un mode d’action extracellulaire. AvrLm3 interagit potentiellement avec une myrosinase-associated proteine sécrétée impliquée dans le système myrosinase-glucosinolate, suggérant qu’AvrLm3 perturberait la synthèse des glucosinolates, ce qui est un mode d’action inédit pour un effecteur d’agent phytopathogène.Cette thèse a permis de mieux comprendre le mode d’action des effecteurs de L. maculans et de proposer de nouvelles stratégies de contrôle des maladies fongiques. / During infection, plant pathogens secrete an arsenal of molecules collectively known as effectors that circumvent plant innate immunity and trigger infection. The phytopathogenic fungus Leptosphaeria maculans is the causal agent of stem canker of oilseed rape. More than 650 putative effector-encoding genes have been identified in its genome, 7 of them corresponding to avirulence genes. Fungal effectors mainly correspond to small secreted proteins (SSP) with no known homologs and no predicted functions. Their biological function is therefore difficult to predict, and very little is known about the mode of action of L. maculans effectors during infection.The objective of my thesis was to elucidate the role of L. maculans effectors during infection through their functional characterization which included: i) the determination of their subcellular localization in Nicotiana benthamiana et Arabidopsis thaliana; ii) a search for their plant targets; and iii) the determination of the cellular processes targeted by those effectors through their stable expression in A. thaliana and by testing their ability to suppress cell-death in N. benthamiana. We investigated four effectors in that study: AvrLm10-1, AvrLm10-2, AvrLm4-7 and AvrLm3.AvrLm10-1 and AvrLm10-2 are both necessary to trigger recognition by the Rlm10 resistance gene. We have identified orthologs for AvrLm10-1 and AvrLm10-2 in Dothideomycetes and Sordariomycetes phytopathogens, and several paralogs in L. maculans which are expressed specifically during oilseed rape infection. AvrLm10-1 and AvrLm10-2 both have a nucleo-cytoplasmic localization. AvrLm10-1 and AvrLm10-2 physically interact, and may also interact with a PR1 (Pathogenesis-related 1) protein and a secreted cysteine-protease. AvrLm4-7 is recognized by two resistance genes, Rlm4 and Rlm7, and suppresses recognition of AvrLm3 by Rlm3. AvrLm4-7 suppresses cell-death triggered by general inducers, PAMP-Triggered Immunity (PTI) and Effector-Triggered Immunity (ETI). AvrLm4-7 has a nucleo-cytoplasmic localization, whether expressed with or without its signal peptide, suggesting an intracellular mode of action. One of the potential plant targets for AvrLm4-7 is a ribosomal protein, just like a Blumeria graminis effector with structural analogy to AvrLm4-7. Transgenic lines of A. thaliana constitutively expressing AvrLm4-7 do not show any morphological phenotypes or any difference in their susceptibility to diverse fungal pathogens. AvrLm3 is an avirulence gene strongly conserved in L. maculans populations. Recognition of AvrLm3 by Rlm3 is suppressed by the presence of AvrLm4-7. AvrLm3 suppresses cell-death triggered by several inducers of PTI and ETI. AvrLm3 is localized in plant apoplasm when expressed with its signal peptide, suggesting an extracellular localization. AvrLm3 potentially interacts with a secreted myrosinase-associated protein implicated in the myrosinase-glucosinolate system, suggesting that AvrLm3 could disturb glucosinolate production, which is a novel mode of action never described for a plant pathogen effector.My thesis allowed us to improve our knowledge on fungal effector function during infection and to propose new strategies for plant diseases management
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Réponses des cellules de Nicotiana tabacum à des molécules microbiennes : évènements de signalisation précoce, influence de la dynamique membranaire et flux de sucres / Responses of Nicotiana tabacum cells to microbial molecule treatments : early signaling events, influence of membrane dynamics, and sugar fluxesPfister, Carole 19 January 2018 (has links)
Dans son environnement la plante est confrontée à une variété de microorganismes bénéfiques, neutres et pathogènes, qui sont fortement dépendants des ressources carbonées qu’elle libère dans le sol. Le transport de sucres, processus clé de la physiologie de la plante, est essentiel pour les interactions plantes-microorganismes et leur devenir. Au cours de l'évolution, les plantes ont acquis des mécanismes leur permettant de percevoir les signaux microbiens du milieu extérieur, et aboutissant à la transduction d’un signal spécifique puis à des réponses biologiques adaptées (défense versus mutualisme) à la stratégie du microorganisme. Ces réponses assurent la survie et le développement des plantes. Mes travaux de thèse, menés avec un système « d’interaction » simplifié, contribuent à une meilleure compréhension des mécanismes sous-jacents au déterminisme des interactions plantes-microorganismes. Ce système a permis d’étudier, sur des suspensions cellulaires de N. tabacum, les réponses cellulaires précoces déclenchées suite à la perception de molécules microbiennes provenant de microorganismes à stratégie pathogène avirulent ou à stratégie mutualiste. Nous avons mesuré des évènements de signalisation et des flux de sucres induits en réponse à ces molécules microbiennes. Nos résultats ont mis en évidence que les chitotétrasaccharides (CO4), sécrétés par les champignons mycorhiziens à arbuscules dans les stades pré-symbiotiques de l’interaction, mobilisent les mêmes événements de signalisation précoce (H2O2 dépendant de la protéine rbohD, Ca2+ cytosolique, activation de MAPK) que la cryptogéine, un éliciteur des réactions de défense ; mais avec des réponses différentes en terme d’intensité et de cinétique. Les CO4 et la cryptogéine ont par ailleurs montré des impacts distincts sur les flux de sucres et l’expression de transporteurs impliqués. En complément nous avons montré un effet de la modification de la dynamique membranaire associée à la clathrine sur des évènements de signalisation déclenchés par la cryptogéine, ainsi que dans les flux entrants de sucres et l’expression de gènes de transporteurs de sucres. Enfin, l’analyse in silico de l’interactome de transporteurs de sucres chez la plante modèle A. thaliana, nous a permis d’apporter des connaissances supplémentaires quant aux évènements de régulations des transporteurs de sucres et l’identification de protéines régulatrices putatives en interaction avec ces derniers. L’ensemble de ces travaux ouvrent la voie à de nouvelles recherches visant à élucider les mécanismes cellulaires et moléculaires impliqués dans la mise en place des interactions entre plantes et microorganismes. / In their natural environment plants are in close interaction with beneficial, neutral, or pathogenic microbes, which are highly dependent on carbon resources exuded by plant roots. Sugar transport, which is a key process of plant physiology, is essential to support the fate of plant-microbe interactions. During evolution, plants have acquired the ability to perceive microbial molecules, initiating specific signal transduction cascades and leading to adapted response for microbe lifestyles (avirulent, virulent, or benefic). Plant survival will depend on the nature of the induced mechanisms. My PhD work, carried out on a simplified experimental system, contributes to the understanding of mechanisms underlying the determinism of plant-microbe interactions. We used Nicotiana tabacum cells in suspension exposed to microbial molecules derived from mutualistic or avirulent microbes. Using such a simplified system, we analyzed elements of the early signaling cascade and sugar fluxes. We have shown that CO4, which is originating from AMF, initiate early signaling components (rbohD-dependent H2O2, cytosolic Ca2+, MAPK activation) as cryptogein, a defense elicitor, but with distinct profile and amplitude. Those two molecules (CO4 and cryptogein) are responsible of different effects on sugar fluxes and the expression of the underlying sugar transporter genes. In addition, we presented an impact of the alteration of clathrin-mediated process on early signaling events triggered by cryptogein, as well as inward sugar fluxes and expression of sugar transporter genes. Finally, in silico analyses of sugar transporter interactome in Arabidopsis thaliana has provided some possible regulation mechanisms through the identification of new candidate proteins involved in sugar transporter regulation. These information open new perspectives towards a better understanding of the cellular and molecular mechanisms involved in plant-microbe interactions.
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Soil histories continue to structure the bacterial and oomycete communities of Brassicaceae host plants through time on the Canadian prairiesBlakney, Andrew 01 1900 (has links)
Afin d’étudier l’écologie microbienne, il est nécessaire, dans un premier temps, de déterminer quels micro-organismes sont présents dans un milieu et à quel instant. Ces informations sont requises pour pouvoir ensuite développer des outils permettant de prédire l’assemblage des communautés et les fonctions que celles-ci peuvent contenir. Cependant, la multitude des processus entrant en jeu dans la structure et la composition des communautés microbiennes, rendent leur étude complexe. Parmi les nombreux processus à étudier, il est notamment question de l’échelle temporelle à prendre en compte pour comprendre l’assemblage des communautés microbiennes. En effet, les événements historiques conditionnent la composition et la biodiversité des futures communautés microbiennes. Pourtant, dans les sols, peu d’études se sont intéressées à l’impact des événements historiques dans l’assemblage des communautés microbiennes. Par conséquent, l’objectif de cette thèse était de quantifier comment les différentes histoires du sol ont influencé la structure et biodiversité des communautés bactériennes et oomycètes associées aux plantes hôtes des Brassicaceae à travers le temps.
Les rotations de cultures de Brassicaceae sont de plus en plus courantes dans le monde et ont démontré des avantages pour les cultures concernées, telles que la rétention de l’humidité du sol ou la suppression de certains agents pathogènes des plantes. En revanche, l’impact des rotations de cultures de Brassicaceae sur la structure et biodiversité des communautés microbiennes résidentes est peu connu. Ainsi, des terrains agricoles des prairies canadiennes ayant des expériences de rotations de cultures en cours ont été utilisés pour modéliser l’impact des histoires de sol précédemment établies sur les futures communautés microbiennes. Les communautés microbiennes des racines, de la rhizosphère, et du sol éloigné des racines des Brassicaceae ont été étudiées grâce aux métabarcodes d’ARNr 16S ou ITS. La PCR quantitative et des méthodes phylogénétiques ont été utilisées pour améliorer l’analyse des communautés microbiennes.
Cette thèse illustre comment différentes histories de sol établies par les cultures de l’année précédente ont continué à structurer les communautés microbiennes de la rhizosphère tout au long de la saison de croissance, à différents stades de croissance, jusqu’à un an après leur établissement. Cependant, le phénomène de rétroactions entre plantes et micro-organismes a permis de masquer cet héritage dans la rhizosphere de différentes espèces hôtes de Brassicacea pour lesquelles des communautés bactériennes phylogénétiquement similaires ont été retrouvées malgré diverses histoires du sol. Nos résultats montrent également que les différentes espèces hôtes de Brassicacea n’avaient pas d’impact sur la structure des communautés d’oomycètes et que le stress hydrique limitait également cette structuration pour les communautés bactériennes. Dans ces deux cas, l’effet de l’histoire du sol était donc encore visible sur la structure les communautés microbiennes durant l’année subséquente.
Les découvertes selon lesquelles différentes histoires de sol persistent jusqu'à un an, même en présence de nouvelles plantes hôtes, et qu’elles peuvent continuer à façonner les communautés microbiennes ont des implications importantes pour la gestion agricole et les recherches futures sur les composants physiques de l'histoire du sol. Comprendre comment l'histoire du sol est impliquée dans la structure et la biodiversité des communautés microbiennes à travers le temps est une limitation de l'écologie microbienne et est nécessaire pour utiliser les technologies microbiennes à l'avenir pour une agriculture durable et dans toute la société. / A fundamental task of microbial ecology is determining which organisms are present, and when, in order to improve the predictive models of community assembly and functions. However, the heterogeneity of community assembly processes that underlie how microbial communities are formed and structured are makes assembly of taxonomic and functional profiles difficult. One reason for this challenge is the compounding effect temporal scales have on microbial communities. For example, historical events have been shown to condition future microbial community composition and biodiversity. Yet, how historical events structure microbial communities in the soil has not been well tested. Therefore, the objective of this thesis was to quantify how different soil histories influenced the structure and biodiversity of bacterial and oomycete communities associated with Brassicaceae host plants through time.
Brassicaceae crop rotations are increasingly common globally, and have demonstrated benefits for the crops involved, such as retaining soil moisture, or suppressing certain plant pathogens. In contrast, there is a lack of knowledge surrounding how Brassicaceae crop rotations impact the structure and biodiversity of resident microbial communities. As such, on-going agricultural field experiments with crop rotations on the Canadian prairies were used to model how previously established soil histories impacted future microbial communities. The Brassicaceae microbial communities were inferred from the roots, rhizosphere and bulk soil using 16S rRNA or ITS metabarcodes. Quantitative PCR and phylogenetic methods were used to improve the analysis of the microbial communities.
This thesis illustrates how different soil histories established by the previous year’s crops continued to structure the microbial rhizosphere communities throughout the growing season, at various growth stages, and up to a year after being established. However, active plant-soil microbial feedback allowed different Brassicaceae host species to mask the soil history in the rhizosphere and derive phylogenetically similar bacterial communities from these diverse soil histories. Furthermore, host plants were unable to structure the oomycete communities, and lost the ability to structure the bacterial rhizosphere communities under water stress. In both circumstances, the soil history continued to structure the microbial communities.
The findings that different soil histories persist for up to a year, even in the presence of new host plants, and can continue to shape microbial communities has important implications for agricultural management and future research on the physical components of soil history. Understanding how soil history is involved in the structure and biodiversity of microbial communities through time is a limitation in microbial ecology and is required for employing microbial technologies in the future for sustainable agriculture and throughout society.
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Effects of a widely conserved AvrE-family effector and the phytotoxin coronatine on host plant defense signaling pathwaysTuro, Alexander Joshua January 2021 (has links)
No description available.
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