Molecular characterization of fall armyworm (Spodoptera frugiperda) resistant to Vip3Aa20 protein expressed in corn / Caracterização molecular da lagarta do cartucho (Spodoptera frugiperda) resistente a proteína Vip3Aa20 expressa em milho

Fatoretto, Júlio César

27 April 2017

Transgenic plants containing genes from Bacillus thuringiensis have been used as an alternative to chemical insecticides for insect pest control. The vegetative insecticidal proteins (Vip) secreted during the vegetative growth phase of bacteria are considered a second generation of insecticidal proteins since they do not share any structural or sequence homology with previously used crystal proteins (Cry) as well as having a wide insecticidal spectrum. One of the target pests for this protein is the fall armyworm (FAW) (Spodoptera frugiperda), the most important corn pest in South America. Previously it has been controlled by insecticides and maize expressing Cry proteins, but has rapidly evolved resistance to many control practices and remains a top concern for sustainable biotechnology control efforts. Thus, resistance characterization involving mode of action and genetics of resistance can help with Insect Resistance Management strategies, and improve the durability of control. In this dissertation, using two selected FAW population resistant to Vip3Aa20 Bt protein (Vip-R1and Vip-R2) we generated comparative proteomic and transcriptomic data among resistant and susceptible colonies. In the chapter 2, we bring FAW biology/ecology and Brazilian agriculture landscape data to support the high adaptive potential of this pest to genetically modified maize expressing Bt Cry proteins in Brazil. Proteomics studies in the chapter 3 revealed that neither Vip-R1 nor Vip-R2 showed difference between resistant and susceptible colonies either for Vip3Aa20 activation through proteolysis assay nor protein binding to the receptor. Transcriptomic sequencing and RNA-seq analysis in the chapter 4 showed strong evidence of ABC transporter genes associated with resistance as well as genes related to G-protein signaling pathway as downregulated. These results will be discussed in context of providing best management practices for managing FAW resistance to Vip, and extending the durability of Vip technology. / Plantas Transgênicas expressando genes de Bacillus thuringiensis (Bt) tem sido usadas como alternativa ao controle químico para controle de insetos praga. A proteina Vip (Vegetative Insecticide Protein) cuja secreção é realizada durante fase de crescimento da bacteria é considerada como segunda geração de proteinas inseticidas em função desta não apresentar similaridade de sequencias com todas as outras proteinas cristal (Cry), apresentando ainda maior espectro de controle de pragas. Uma das pragas alvo desta proteina é a lagarta-do-cartucho do milho (Spodoptera frugiperda), considerada a mais importante na cultura do milho na América do Sul. Larvas desta espécie foram sempre controladas com inseticidas e mais recentemente, milho expressando proteínas Cry. No entanto, esta praga tem desenvolvido resistência para várias ferramentas de controle, trazendo preocupação para a sustentabilidade das taticas de controle geradas através da biotecnologia. Dessa forma, estudos de caracterização da resistencia envolvendo modo de ação e characteristicas genéticas envolvidas com resistência pode contribuir para melhorar estratégias de Manejo de Resistencia de Insetos (IRM) e aumentar a durabilidade destas tecnologias para o controle. Nesta dissertação, foi gerado dados proteômicos e de transcriptoma comparando uma população de S. frugiperda resistente a Vip3Aa20 com a susceptivel. No capítulo 2, abordamos as características de bio-ecologia da praga associado ao sistema de cultivo suportando o alto potencial adaptativo desta espécie para hibridos de milho expressando proteinas Bt no Brazil. No capitulo 3, estudos de proteômica mostrou que Vip-R1 e Vip-R2 quando comparado com SUS, não demostraram diferenças para ativação da proteina nem ausencia de ligação da proteína com receptor de membrana no intestino do inseto. Dados de transcriptoma descritos no capitulo 5 mostrou forte evidências de que a baixa expressão de genes relacionados ao sistema transportador ABC pode estar associado com resistência bem como genes da via de sinalização das proteínas G. Estes resultados serão discutidos em um contexto para suportar boas praticas de manejo de resistência para lagarta-do-cartucho e assim estender a durabilidade da tecnologia Viptera® no campo.

Spodoptera frugiperda

ABC transportador

ABC transporter

Fall armyworm

Insect resistance management

ligação proteina-receptor

Manejo de resistência de insetos

Protein-receptor binding

RNA-seq

RNA-seq

Transcriptoma

Transcriptome

Vip3A

Vip3A

Développement de nouveaux tests fonctionnels d'aide à l'interpretation des variants de signification biologique inconnue dans le cadre de prédispositions génétiques au cancer. / Development of new functional assays for the interpretation of variants of unknown biological significance in the context of genetic predispositions to cancer

Raad, Sabine

06 December 2018

L’identification des mutations constitutionnelles à l’origine d’une prédisposition génétique au cancer est essentielle à la prise en charge médicale des patients et de leurs familles. Depuis l’implémentation des technologies de séquençage à haut-débit dans les laboratoires diagnostiques, le principal défi n’est plus la détection des variations génétiques mais leur interprétation et leur classification. La question de l’interprétation de la variation est particulièrement cruciale lorsqu’elle conditionne la stratégie thérapeutique. Ainsi, il est essentiel de disposer de tests simples adaptables en routine diagnostique pour faciliter l’interprétation des variations génétiques. Dans ce contexte, nous avons utilisé un test fonctionnel développé par notre équipe pour classer des variations dans le gène TP53 à l’origine du syndrome de Li-Fraumeni et pour appréhender la corrélation génotype - phénotype chez les patients LFS. Dans un deuxième temps, nous avons évalué la pertinence d’une approche multi-omique (RNA-Seq et métabolomique) pour discriminer les cellules sauvages des cellules avec mutation hétérozygote du gène TP53 ou des gènes BRCA impliqués dans la prédisposition génétique aux cancers du sein et de l’ovaire. Sur la base des données de transcriptome, un modèle mathématique a été développé pour détecter les variants correspondant à des mutations délétères. Nous avons ensuite sélectionné les biomarqueurs les plus discriminants pour les intégrer dans un test fonctionnel de RT-MLPA dédié à la voie p53. Nous avons enfin adapté cet essai pour qu’il soit réalisable sur une simple prise de sang, sans immortalisation des lymphocytes du patient. / The identification of the constitutional mutation responsible for a genetic predisposition to cancer is essential to the clinical management of the patient and its relatives. With the implementation of high-throughput sequencing to the diagnostic routine of these pathologies, the challenge no longer lies within the detection of alterations but in their biological and clinical interpretation. While specific treatments are emerging, simple functional assays to help with the interpretation of the detected variants are needed. In this context, we used a functional test developed by our team to classify variations in the TP53 gene responsible for Li-Fraumeni syndrome and to understand the genotype-phenotype correlation in LFS patients. On the other hand, we assessed the relevance of a multi-omic approach (RNA-Seq and metabolomics) to discriminate wild-type cells from cells with a deleterious heterozygous mutation in TP53 or in the BRCA genes implicated in genetic predisposition to breast and ovarian cancers. Based on the transcriptomic data, a mathematical model has been developed to detect variants corresponding to deleterious mutations. Then we selected the most discriminating biomarkers and integrated them into a RT-MLPA functional assay dedicated to the p53 pathway. We finally adapted this test to be feasible on a simple blood test, without immortalization of the patient's lymphocytes.

Prédispositions génétiques au cancer

Approche multi-omique

Métabolomique

RNA-seq

Tests fonctionnels

TP53

BRCA

Genetic cancer predispositions

Multi-omic approach

RNA-seq

Metabolomics

Functional assays

TP53

BRCA

616.99

Dinâmica do perfil transcricional de duas cultivares de cana-de-açúcar contrastantes à seca e submetidas ao déficit hídrico prolongado /

Konrad, Daniela

January 2019

Orientador: Maria Ines Tiraboschi Ferro / Resumo: Períodos prolongados de seca têm se tornado mais frequentes em algumas regiões do Brasil. Além disso, a expansão da cultura de cana-de-açúcar para regiões com deficiência hídrica prolongada torna a produção sucroenergética limitada nestes locais. A melhor forma de contornar esse problema é utilizar cultivares tolerantes a este estresse. Neste trabalho, o perfil de expressão gênica da cana-de-açúcar foi avaliado, a partir de duas cultivares com respostas contrastantes ao déficit hídrico: uma delas com comportamento considerado tolerante (SP81-3250), e a outra altamente exigente em água (RB855453), considerada sensível. Ambas foram submetidas a três potenciais hídricos do solo (controle (sem estresse hídrico), déficit hídrico moderado e déficit hídrico severo) a partir de 60 dias após o plantio. Essas plantas foram avaliadas molecular e fisiologicamente em três épocas distintas: 30, 60 e 90 dias após a aplicação dos tratamentos, sendo este um dos poucos estudos realizados até o momento sobre a resposta de plantas de cana-de-açúcar sob déficit hídrico prolongado, estresse esse que foi realizado no período conhecido como fase de formação da cana-de-açúcar, compreendendo o período mais crítico por demanda de água. A análise global da expressão gênica através da tecnologia de RNA-Seq mostrou alterações significativas em resposta ao déficit hídrico entre as duas cultivares. Os transcritos do genótipo tolerante apresentaram uma maior capacidade de reação das plantas frente ao déficit... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: Extended periods of drought have become more frequent in some regions of Brazil. In addition, the expansion of sugarcane cultivation to regions with prolonged water deficiency makes sugarcane production limited at these locations. The best way around this problem is to use stress-tolerant cultivars. In this work, the sugarcane gene expression profile was evaluated from two cultivars with contrasting responses to water deficit: one of them with tolerant behavior (SP81-3250), and the other highly demanding in water (RB855453 ), considered sensitive. Both were submitted to three soil water potentials (control (without water stress), moderate water deficit and severe water deficit) from 60 days after planting. These plants were evaluated molecularly and physiologically at three different times: 30, 60 and 90 days after the application of the treatments. This is one of the few studies carried out so far on the response of sugarcane plants under prolonged water deficit. This stress was realized during the period known as sugarcane formation phase, comprising the most critical period by water demand. The overall analysis of gene expression through RNA-Seq technology showed significant changes in response to water deficit between the two cultivars. The transcripts of the tolerant genotype showed a higher reaction capacity of the plants to prolonged water deficit, while in the sensitive genotype, several plant survival mechanisms were repressed. The tolerant cultivar presented inducti... (Complete abstract click electronic access below) / Mestre

Cana-de-açúcar.

Déficit hídrico prolongado

Montagem "de novo"

RNA-Seq

RT-qPCR

"de novo" assembly

Cana-de-açúcar.

Prolonged water deficit

RNA-Seq

RT-qPCR

An RNA comparison study between the Amazonian, Centro-American and Orinocan semispecies of Drosophila paulistorum

Hedman, Erik

January 2020

Differential expression analysis can be a powerful method to investigate expressed differences between closely related species. Our ambition is to highlight differentially expressed nuclear genes to explain the hybrid incompatibilities among the Amazonian, Centro-American and Orinocan semispecies of Drosophila paulistorum. RNA sequencing (RNA-seq) establishes the foundation of the study where we first evaluate the influence of two distinct alignment references. We discover the benefits of concatenating a de novo assembly instead of using the genome reference of a close relative. The bioinformatic pipeline handles the interesting inclusion of D. melanogaster and D. willistoni, where their contribution assists in the search for previously studied speciation genes. Among the down- and upregulated subsets we can see a diverse mix of general biological processes such as regulatory functions and transcriptional factors. In the end we uncover potential indications to why the Amazonian seems to be the least compatible semispecie to produce hybrids. This study provides a competitive working frame for comparative RNA-seq studies between closely related species.

Drosophila paulistorum

D. paulistorum

RNA-seq

RNA-seq comparison study

Differential expression analysis

Amazonian semispecie

Centro-American semispecie

Orinocan semispecie

Bioinformatics (Computational Biology)

Bioinformatik (beräkningsbiologi)

Classification et inférence de réseaux pour les données RNA-seq / Clustering and network inference for RNA-seq data

Gallopin, Mélina

09 December 2015

Cette thèse regroupe des contributions méthodologiques à l'analyse statistique des données issues des technologies de séquençage du transcriptome (RNA-seq). Les difficultés de modélisation des données de comptage RNA-seq sont liées à leur caractère discret et au faible nombre d'échantillons disponibles, limité par le coût financier du séquençage. Une première partie de travaux de cette thèse porte sur la classification à l'aide de modèle de mélange. L'objectif de la classification est la détection de modules de gènes co-exprimés. Un choix naturel de modélisation des données RNA-seq est un modèle de mélange de lois de Poisson. Mais des transformations simples des données permettent de se ramener à un modèle de mélange de lois gaussiennes. Nous proposons de comparer, pour chaque jeu de données RNA-seq, les différentes modélisations à l'aide d'un critère objectif permettant de sélectionner la modélisation la plus adaptée aux données. Par ailleurs, nous présentons un critère de sélection de modèle prenant en compte des informations biologiques externes sur les gènes. Ce critère facilite l'obtention de classes biologiquement interprétables. Il n'est pas spécifique aux données RNA-seq. Il est utile à toute analyse de co-expression à l'aide de modèles de mélange visant à enrichir les bases de données d'annotations fonctionnelles des gènes. Une seconde partie de travaux de cette thèse porte sur l'inférence de réseau à l'aide d'un modèle graphique. L'objectif de l'inférence de réseau est la détection des relations de dépendance entre les niveaux d'expression des gènes. Nous proposons un modèle d'inférence de réseau basé sur des lois de Poisson, prenant en compte le caractère discret et la grande variabilité inter-échantillons des données RNA-seq. Cependant, les méthodes d'inférence de réseau nécessitent un nombre d'échantillons élevé.Dans le cadre du modèle graphique gaussien, modèle concurrent au précédent, nous présentons une approche non-asymptotique pour sélectionner des sous-ensembles de gènes pertinents, en décomposant la matrice variance en blocs diagonaux. Cette méthode n'est pas spécifique aux données RNA-seq et permet de réduire la dimension de tout problème d'inférence de réseau basé sur le modèle graphique gaussien. / This thesis gathers methodologicals contributions to the statistical analysis of next-generation high-throughput transcriptome sequencing data (RNA-seq). RNA-seq data are discrete and the number of samples sequenced is usually small due to the cost of the technology. These two points are the main statistical challenges for modelling RNA-seq data.The first part of the thesis is dedicated to the co-expression analysis of RNA-seq data using model-based clustering. A natural model for discrete RNA-seq data is a Poisson mixture model. However, a Gaussian mixture model in conjunction with a simple transformation applied to the data is a reasonable alternative. We propose to compare the two alternatives using a data-driven criterion to select the model that best fits each dataset. In addition, we present a model selection criterion to take into account external gene annotations. This model selection criterion is not specific to RNA-seq data. It is useful in any co-expression analysis using model-based clustering designed to enrich functional annotation databases.The second part of the thesis is dedicated to network inference using graphical models. The aim of network inference is to detect relationships among genes based on their expression. We propose a network inference model based on a Poisson distribution taking into account the discrete nature and high inter sample variability of RNA-seq data. However, network inference methods require a large number of samples. For Gaussian graphical models, we propose a non-asymptotic approach to detect relevant subsets of genes based on a block-diagonale decomposition of the covariance matrix. This method is not specific to RNA-seq data and reduces the dimension of any network inference problem based on the Gaussian graphical model.

Modèle de mélange

Modèle graphique

RNA-Seq data

Classification

Inférence de réseau

Sélection de modèle

Mixture model

Graphical model selection

RNA-Seq data

Clustering

Network inference

Model selection

Analyses génomiques comparatives de souches de Brevibacterium et étude de leurs interactions biotiques avec Hafnia alvei dans un fromage modèle / Comparative genomic analysis of Brevibacterium strains and study of their biotic interactions with Hafnia alvei in a model cheese

Pham, Nguyen Phuong

20 December 2018

L’objectif de ce travail était de mieux comprendre les mécanismes moléculaires de l’adaptation microbienne à l’environnement fromager par des approches de génomique fonctionnelle via le modèle de Brevibacterium, un genre bactérien largement utilisé en technologie fromagère, mais dont l’implantation est parfois difficile à maîtriser.L’analyse génomique comparative de 23 souches de Brevibacterium, dont 12 issues de fromages, a révélé des différences en déterminants génétiques impliqués dans la capacité à croître à la surface du fromage. Parmi ces différences, plusieurs sont corrélées à la phylogénie des souches, et d’autres résultent de transferts horizontaux, notamment dans le cas des gènes liés à l’acquisition du fer et à la biosynthèse de bactériocines. Nous avons identifié des îlots génomiques correspondant à des transferts de gènes d’acquisition du fer entre des souches fromagères de Brevibacterium et des bactéries d’affinage appartenant à d’autres genres. Nous avons également mis en évidence un transposon conjugatif codant pour la synthèse de bactériocines présent chez des souches de Brevibacterium d'origine fromagère mais aussi chez une souche fromagère du genre Corynebacterium.L’étude fonctionnelle des interactions biotiques entre Brevibacterium et Hafnia alvei, une autre bactérie d’affinage du fromage, a été menée dans un modèle fromager développé au cours de ce travail. En couplant des analyses microbiologiques, biochimiques et transcriptomiques (RNA-seq), nous avons mis en évidence l’existence de différents mécanismes d’interaction entre ces bactéries. Ceux-ci concernent notamment l’acquisition du fer, la protéolyse, la lipolyse, le métabolisme soufré et le catabolisme du D-galactonate. Nos résultats suggèrent que dans la relation mutualiste observée entre certaines souches de Brevibacterium et H. alvei, cette dernière sécrète des sidérophores qui sont utilisés par Brevibacterium pour capter le fer plus efficacement, stimulant ainsi sa croissance. En contrepartie, Brevibacterium sécrète des lipases et des protéases qui dégradent les caséines et triglycérides du fromage en constituants énergétiques favorisant la croissance de H. alvei. Ce type d’interaction est intéressant à considérer pour la formulation des ferments d'affinage car il en résulte une meilleure capacité de tous les partenaires à coloniser le fromage, et ainsi à générer les propriétés technologiques recherchées. / The objective of this study was to better understand the molecular mechanisms of microbial adaptation to the cheese habitat by functional genomic approaches using Brevibacterium as a model microorganism. This bacterium is widely used for the manufacturing of cheese but its growth on the cheese surface is sometimes difficult to control.Comparative genomic analysis of 23 Brevibacterium strains, including 12 strains isolated from cheeses, revealed differences in genetic determinants involved in the growth on the cheese surface. Some of them are correlated to strain phylogeny and others are the result of gene transfers, especially those involved in iron acquisition and bacteriocin biosynthesis. We identified genomic islands corresponding to transfers of genes involved in iron acquisition between cheese-associated Brevibacterium strains and cheese-associated strains belonging to other genera. We also detected a conjugative transposon encoding bacteriocin production, which is present in cheese-associated Brevibacterium strains as well as in a cheese-associated Corynebacterium strain.Functional study of biotic interactions between Brevibacterium and Hafnia alvei, another cheese-ripening bacterium, was performed in a model cheese developed in this study. By coupling microbial, biochemical and transcriptomic (RNA-seq) analyses, we revealed several interaction mechanisms between these bacteria. These concern, in particular, iron acquisition, proteolysis, lipolysis, sulfur metabolism and D-galactonate catabolism. Our findings suggest that in the mutualistic relationship between some Brevibacterium strains and H. alvei, the latter stimulates Brevibacterium growth by the secretion of siderophores, which can be used by Brevibacterium to capture iron more efficiently. In return, Brevibacterium secretes lipases and proteases, which degrade cheese caseins and triglycerides into energetic substrates that stimulate H. alvei growth. This type of interaction is interesting to consider in the formulation of ripening cultures because it results in a better ability of all partners to colonize the cheese, and thus to generate the desired technological properties.

Brevibacterium

Hafnia alvei

Fromage

Génomique fonctionnelle

Interactions biotiques

RNA-Seq

Brevibacterium

Hafnia alvei

Cheese

Functional genomic

Biotic interactions

RNA-Seq

664.024

Computational Analysis of Gene Expression Regulation from Cross Species Comparison to Single Cell Resolution

Lee, Jiyoung

31 August 2020

Gene expression regulation is dynamic and specific to various factors such as developmental stages, environmental conditions, and stimulation of pathogens. Nowadays, a tremendous amount of transcriptome data sets are available from diverse species. This trend enables us to perform comparative transcriptome analysis that identifies conserved or diverged gene expression responses across species using transcriptome data. The goal of this dissertation is to develop and apply approaches of comparative transcriptomics to transfer knowledge from model species to non-model species with the hope that such an approach can contribute to the improvement of crop yield and human health. First, we presented a comprehensive method to identify cross-species modules between two plant species. We adapted the unsupervised network-based module finding method to identify conserved patterns of co-expression and functional conservation between Arabidopsis, a model species, and soybean, a crop species. Second, we compared drought-responsive genes across Arabidopsis, soybean, rice, corn, and Populus in order to explore the genomic characteristics that are conserved under drought stress across species. We identified hundreds of common gene families and conserved regulatory motifs between monocots and dicots. We also presented a BLS-based clustering method which takes into account evolutionary relationships among species to identify conserved co-expression genes. Last, we analyzed single-cell RNA-seq data from monocytes to attempt to understand regulatory mechanism of innate immune system under low-grade inflammation. We identified novel subpopulations of cells treated with lipopolysaccharide (LPS), that show distinct expression patterns from pro-inflammatory genes. The data revealed that a promising therapeutic reagent, sodium 4-phenylbutyrate, masked the effect of LPS. We inferred the existence of specific cellular transitions under different treatments and prioritized important motifs that modulate the transitions using feature selection by a random forest method. There has been a transition in genomics research from bulk RNA-seq to single-cell RNA-seq, and scRNA-seq has become a widely used approach for transcriptome analysis. With the experience we gained by analyzing scRNA-seq data, we plan to conduct comparative single-cell transcriptome analysis across multiple species. / Doctor of Philosophy / All cells in an organism have the same set of genes, but there are different cell types, tissues, organs with different functions as the organism ages or under different conditions. Gene expression regulation is one mechanism that modulates complex, dynamic, and specific changes in tissues or cell types for any living organisms. Understanding gene regulation is of fundamental importance in biology. With the rapid advancement of sequencing technologies, there is a tremendous amount of gene expression data (transcriptome) from individual species in public repositories. However, major studies have been reported from several model species and research on non-model species have relied on comparison results with a few model species. Comparative transcriptome analysis across species will help us to transform knowledge from model species to non-model species and such knowledge transfer can contribute to the improvement of crop yields and human health. The focus of my dissertation is to develop and apply approaches for comparative transcriptome analysis that can help us better understand what makes each species unique or special, and what kinds of common functions across species have been passed down from ancestors (evolutionarily conserved functions). Three research chapters are presented in this dissertation. First, we developed a method to identify groups of genes that are commonly co-expressed in two species. We chose seed development data from soybean with the hope to contribute to crop improvement. Second, we compared gene expression data across five plant species including soybean, rice, and corn to provide new perspectives about crop plants. We chose drought stress to identify conserved functions and regulatory factors across species since drought stress is one of the major stresses that negatively impact agricultural production. We also proposed a method that groups genes with evolutionary relationships from an unlimited number of species. Third, we analyzed single-cell RNA-seq data from mouse monocytes to understand the regulatory mechanism of the innate immune system under low-grade inflammation. We observed how innate immune cells respond to inflammation that could cause no symptoms but persist for a long period of time. Also, we reported an effect of a promising therapeutic reagent (sodium 4-phenylbutyrate) on chronic inflammatory diseases. The third project will be extended to comparative single-cell transcriptome analysis with multiple species.

Cross-species comparison

Comparative transcriptome analysis

Next generation sequencing

Gene expression regulation

Gene regulatory network

Single-cell RNA-seq

RNA-seq

Arabidopsis

Soybean

Drought Stress

Mouse

Monocyte

Identification of common and unique stress responsive genes of Arabidopsis thaliana under different abiotic stress through RNA-Seq meta-analysis

Akter, Shamima

06 February 2018

Abiotic stress is a major constraint for crop productivity worldwide. To better understand the common biological mechanisms of abiotic stress responses in plants, we performed meta-analysis of 652 samples of RNA sequencing (RNA-Seq) data from 43 published abiotic stress experiments in Arabidopsis thaliana. These samples were categorized into eight different abiotic stresses including drought, heat, cold, salt, light and wounding. We developed a multi-step computational pipeline, which performs data downloading, preprocessing, read mapping, read counting and differential expression analyses for RNA-Seq data. We found that 5729 and 5062 genes are induced or repressed by only one type of abiotic stresses. There are only 18 and 12 genes that are induced or repressed by all stresses. The commonly induced genes are related to gene expression regulation by stress hormone abscisic acid. The commonly repressed genes are related to reduced growth and chloroplast activities. We compared stress responsive genes between any two types of stresses and found that heat and cold regulate similar set of genes. We also found that high light affects different set of genes than blue light and red light. Interestingly, ABA regulated genes are different from those regulated by other stresses. Finally, we found that membrane related genes are repressed by ABA, heat, cold and wounding but are up regulated by blue light and red light. The results from this work will be used to further characterize the gene regulatory networks underlying stress responsive genes in plants. / Master of Science / Abiotic stress is a major constraint for crop productivity worldwide. To better understand the common biological mechanisms of abiotic stress responses in plants, we performed analysis of 652 samples of RNA sequencing data from 43 published abiotic stress experiments in Arabidopsis thaliana. These samples were collected from eight different abiotic stresses including drought, heat, cold, salt, light and wounding. We identified genes that were induced or repressed by each of these stresses. We found that 5729 and 5062 genes are induced or repressed by only one type of abiotic stresses. There are only 18 and 12 genes that are induced or repressed by all stresses. The commonly induced genes are related to gene expression regulation by stress hormone. The commonly repressed genes are related to reduced growth. We compared stress responsive genes between any two types of stresses and found that heat and cold regulate similar set of genes. We also found that high light affects different set of genes than blue light and red light. Finally, we found that membrane related genes are repressed by stress hormone, heat, cold and wounding but are up regulated by blue light and red light. The results from this work will be used to further characterize the gene regulations underlying stress responsive genes in plants.

Abiotic stress

Reactive oxygen species

RNA-Seq

RNA-Seq pipeline

Gene Omnibus Series (GSE)

Differentially Expressed Genes (DEG)

Jaccard similarity index

Gene Ontology (GO)

Understanding the biochemical basis of temperature induced lipid pathway adjustments in plants

2014 April 1900

One of the cellular responses to temperature fluctuations in plants is the adjustment in the degree of membrane unsaturation. Glycerolipids are major constituents of cellular membranes. In higher plants, glycerolipids are synthesized via two major metabolic pathways compartmentalized in the ER and chloroplast. Adaptive responses in membrane lipids include alterations in fatty acid desaturation, proportional changes in membrane lipids as well as molecular composition of each lipid species. In this study, I systematically explored the significance of glycerolipid pathway balance in temperature induced lipid composition changes in three plant species that have distinctive modes of lipid pathway interactions through a combination of biochemical and molecular approaches including lipidomics and RNA-seq analysis. In Arabidopsis thaliana, a 16:3 plant, low temperature induces an augmented prokaryotic pathway, whereas high temperature enhances the eukaryotic pathway. Atriplex lentiformis reduces its overall lipid desaturation at high temperature and switches lipid phenotype from 16:3 to 18:3 through drastically increasing the contribution of the eukaryotic pathway as well as suppression of the prokaryotic pathway. In sync with the metabolic changes, coordinated expression of glycerolipid pathway genes, as revealed by RNA-seq also occurs. In Triticum aestivum, an 18:3 plant, low temperature leads to a reduced glycerolipid flux from ER to chloroplast. Evidence of differential trafficking of diacylglycerol (DAG) moieties from ER to chloroplast was uncovered in three plant species as another layer of metabolic adaptation under different temperatures. Taken together, this study has established a biochemical basis that highlights the predominance and prevalence of lipid pathway interactions in temperature induced lipid compositional changes.

fatty acid metabolism

glycerolipid pathways

temperature adaptation

RNA-seq

metabolic regulation.

Exploration, quantification, and mitigation of systematic error in high-throughput approaches to gene-expression profiling : implications for data reproducibility

Kitchen, Robert Raymond

January 2011

Technological and methodological advances in the fields of medical and life-sciences have, over the last 25 years, revolutionised the way in which cellular activity is measured at the molecular level. Three such advances have provided a means of accurately and rapidly quantifying mRNA, from the development of quantitative Polymerase Chain Reaction (qPCR), to DNA microarrays, and second-generation RNA-sequencing (RNA-seq). Despite consistent improvements in measurement precision and sample throughput, the data generated continue to be a ffected by high levels of variability due to the use of biologically distinct experimental subjects, practical restrictions necessitating the use of small sample sizes, and technical noise introduced during frequently complex sample preparation and analysis procedures. A series of experiments were performed during this project to pro le sources of technical noise in each of these three techniques, with the aim of using the information to produce more accurate and more reliable results. The mechanisms for the introduction of confounding noise in these experiments are highly unpredictable. The variance structure of a qPCR experiment, for example, depends on the particular tissue-type and gene under assessment while expression data obtained by microarray can be greatly influenced by the day on which each array was processed and scanned. RNA-seq, on the other hand, produces data that appear very consistent in terms of differences between technical replicates, however there exist large differences when results are compared against those reported by microarray, which require careful interpretation. It is demonstrated in this thesis that by quantifying some of the major sources of noise in an experiment and utilising compensation mechanisms, either pre- or post-hoc, researchers are better equipped to perform experiments that are more robust, more accurate, and more consistent.

572.072