Virulence et résistance aux antibiotiques du staphylocoque doré : recherche des ARNm ciblés par deux ARN régulateurs / Staphylococcal virulence and antibiotic resistance : research of mRNA targeted by two sRNAs

Ivain, Lorraine

12 July 2017

Staphylococcus aureus est une bactérie pathogène opportuniste de l’Homme et de l’animal qui représente l’une des premières causes d’infections nosocomiales. A l’heure actuelle, la sévérité de ces infections est accentuée par l’augmentation des multi-résistances aux antibiotiques qui en font un problème majeur de santé public. La découverte et l’étude des ARN régulateurs (ARNrég) exprimés par le staphylocoque doré a permis de mettre en évidence leurs rôles de régulateurs de l’étape de colonisation et d’infection (quorum sensing, virulence, résistance aux antibiotique, adaptation environnementales). Au cours de ma thèse, je me suis intéressée à l’étude de deux ARNrég, SprD impliqué dans la virulence de la bactérie sur modèle animal murin et SprX régulant la résistance aux glycopeptides. Dans le but de comprendre les bases moléculaires de leurs rôles dans la bactérie, nous avons souhaité identifier et valider l’ensemble des cibles directes à ces deux ARN. Dans un premier temps, nous nous sommes intéressés à l’étude des nouvelles cibles de SprX. Pour cela, nous avons mis en place une approche in vivo de validation des cibles des ARNrég basée sur la technique des gènes rapporteurs. Nous avons ainsi pu valider deux nouvelles cibles de SprX, les ARNm ecb et purC impliqués respectivement dans l’évasion du système immunitaire et dans le métabolisme des purines. SprX interagit au niveau du site d’initiation de la traduction de ces deux ARNm, et inhibe leurs traductions. Par la suite, nous avons souhaité rechercher de nouvelles cibles pour SprD. Nous avons pu adapter à S. aureus une technique d’identification de nouvelles cibles des ARNrég. L’ensemble des résultats obtenus permettent de préciser les rôles déjà connus des deux ARNrég et offrent de nouvelles possibilités concernant l’étude et la validation des cibles potentielles. / Staphylococcus aureus is an opportunistic pathogen that causes a wide variety of nosocomial and community-acquired infections. Its adaptive capacities, multiple antibiotic resistances and high virulence makes it a major public health issue. The discovery and study of small regulatory RNAs (sRNAs) expressed by S. aureus showed their implication in the switch colonization to host infection. During my phD, I focused on the study of two sRNAs: (i) SprD, involved in staphylococcal virulence and (ii) SprX which regulates glycopeptides resistance. To understand the molecular basis of their roles in staphylococcal physiology, we searched for their direct targets using two different techniques. For SprX, we set up an in vivo technique to validate mRNA targets previously predicted using bioinformatics tools. This method based on the use of a fluorescent reporter gene allowed us to validate two novels SprX targets, the ecb and purC mRNAs involved in immune evasion system and purine metabolism, respectively. We further showed that SprX interacts at the ribosome binding sites preventing translation initiation. In another chapter of my phD project, we adapted the MAPS technique to S. aureus and applied it to the search of SprD direct partners by affinity purification of sRNA-mRNA duplexes. Overall, the results obtained during my thesis allowed us to precise the roles of SprD and SprX and will offer novel possibilities for the staphylococcal community to identify and/or validate of sRNA targets.

ARNrég

Staphylococcus aureus

ARNm cibles

Virulence

Résistance aux glycopeptides

Srna

Staphylococcus aureus

MRNA targets

Virulence

Glycopeptides resistance

Staphylococcus aureus protein S1, an RNA chaperone involved in translation initiation and sRNA regulation / La protéine S1 chez Staphylococcus aureus, une protéine chaperonne de l’ARN impliquée dans l'initiation de la traduction et la régulation médiée par des ARN non codants

Marenna, Alessandra

29 September 2017

Bien que l'initiation de la traduction soit un processus conservé entre les bactéries, nous avons montré que le mécanisme par lequel les ARNm structurés sont reconnus et adaptés sur le ribosome diffère chez Staphylococcus aureus, un micro-organisme avec un bas taux de G+C et chez Escherichia coli. Une particularité du ribosome de S. aureus est l'absence de la protéine ribosomale S1, qui non seulement est plus courte que celle de E. coli mais qui possède également une organisation distincte des domaines. Mes expériences suggèrent que la protéine S1 (SauS1) favorise spécifiquement l'initiation de la traduction de l'opéron α-psm 1-4 en liant son ARNm hautement structuré. En outre, il influence aussi l'expression et la production de facteurs de virulence comme les exotoxines (α-haemolysine, δ-hémolysine et γ- hémolysine) et les exoenzymes (protéases et lipases). En plus de son rôle dans la traduction, SauS1 pourrait être impliquée dans d'autres processus cellulaires tels que le métabolisme de l'ARN et la régulation par des ARN non-codants (ARNnc). Elle forme des complexes in vivo avec plusieurs ARNnc dont la stabilité serait affectée dans la souche délétée du gène rpsA codant S1. SauS1 a donc une activité chaperonne favorisant la cinétique d’appariement entre deux molécules d'ARN et au moins dans un cas, elle stimule la reconnaissance entre un ARNnc et son ARN cible. Ainsi, SauS1 appartient à une nouvelle classe de chaperons d'ARN qui jouent un rôle clé dans la régulation du virulon de S. aureus. / Even if translation initiation is a conserved process among bacteria, we have recently shown that low G+C content Gram-positive, such as Staphylococcus aureus, differ from E. coli on the mechanism by which structured mRNAs are recognized and adapted on the ribosome. One peculiarity of the S. aureus ribosome is the absence of ribosomal protein S1, which is shorter than E. coli S1 and has different domains organization. My work could demonstrate that S. aureus S1 (SauS1) specifically promotes translation initiation of the α-psm 1-4 operon by binding its highly structured mRNA. Moreover, it influences the expression and production of other exotoxins (α-haemolysin, δ-haemolysin and γ-haemolysins) and exoenzymes (proteases and lipases). Besides its role in translation, SauS1 could be implicated in other cellular processes such as RNA maturation/degradation and sRNA-mediated regulation. It forms in vivo complexes with several sRNAs whose level is affected in a strain deleted of rpsA gene, coding for S1. Preliminary results show that SauS1 has a chaperone activity promoting the kinetic of annealing of two model RNA molecules and at least in one case, we could demonstrate that it stimulates the recognition between a sRNA and its target RNA. Taken together, SauS1 belongs to a new class of RNA chaperones that play key roles in the regulation of S.aureus virulon.

S. aureus S1

Traduction

ARNnc

Régulation du virulon

S. aureus S1

Translation

SRNA

Regulation of S. aureus virulon

572.8

579.3

Non-coding small RNAs regulate multiple mRNA targets to control the Vibrio cholerae quorum sensing response

Zhao, Xiaonan

09 April 2013

The waterborne bacterial pathogen Vibrio cholerae uses a process of cell-to-cell communication called quorum sensing (QS) to coordinate transcription of four sRNAs (Qrr1-4; quorum regulatory RNAs) in response to changes in extracellular QS signals that accumulate with cell density. The Qrr sRNAs are predicted to negatively control translation of several mRNAs, including hapR, which encodes the master QS transcription factor that controls genes for virulence factors, biofilm formation, protease production, and DNA uptake. The Qrr sRNAs are also predicted to positively control vca0939, which encodes a GGDEF family protein that promote biofilm formation by elevating intracellular levels of the second messenger molecule c-di-GMP. Using complementary in vivo, in vitro, and bioinformatic approaches, I showed that Qrr sRNAs base-pair with and repress translation of the mRNA encoding HapR. A single nucleotide mutation in Qrr RNA abolishes hapR pairing and thus prevents cholera toxin production and biofilm formation that are important in disease, and also alters expression of competence genes required for uptake of DNA in marine settings. I also demonstrated that base-pairing of the Qrr sRNAs with vca0939 disrupts an inhibitory structure in the 5' UTR of the mRNA. Qrr-activated translation of vca0939 was sufficient to promote synthesis of c-di-GMP and early biofilm formation in a HapR-independent manner. Thus, these studies define the non-coding Qrr sRNAs as a critical component allowing V. cholerae to sense and respond to environmental cues to regulate important developmental processes such as biofilm formation.

HapR

Vca0939

Biofilm

Virulence

Qrr sRNA

V. cholerae

Virulence (Microbiology)

Pathogenic microorganisms

Vibrio cholerae

Quorum sensing (Microbiology)

GlmY and GlmZ: a hierarchically acting cascade composed of two small RNAs

Göpel, Yvonne

02 October 2013

No description available.

570

Biologie (PPN619462639)

Recent Advances in Developing Molecular Biotechnology Tools for Metabolic Engineering and Recombinant Protein Purification

Stimple, Samuel Douglas

25 May 2018

No description available.

Chemical Engineering

Développement de méthodes bioinformatiques dédiées à la prédiction et l'analyse des réseaux métaboliques et des ARN non codants / Development of bioinformatic methods dedicated to the prediction and the analysis of metabolic networks and non-coding RNA

Ghozlane, Amine

20 November 2012

L'identification des interactions survenant au niveau moléculaire joue un rôle crucial pour la compréhension du vivant. L'objectif de ce travail a consisté à développer des méthodes permettant de modéliser et de prédire ces interactions pour le métabolisme et la régulation de la transcription. Nous nous sommes basés pour cela sur la modélisation de ces systèmes sous la forme de graphes et d'automates. Nous avons dans un premier temps développé une méthode permettant de tester et de prédire la distribution du flux au sein d'un réseau métabolique en permettant la formulation d'une à plusieurs contraintes. Nous montrons que la prise en compte des données biologiques par cette méthode permet de mieux reproduire certains phénotypes observés in vivo pour notre modèle d'étude du métabolisme énergétique du parasite Trypanosoma brucei. Les résultats obtenus ont ainsi permis de fournir des éléments d'explication pour comprendre la flexibilité du flux de ce métabolisme, qui étaient cohérentes avec les données expérimentales. Dans un second temps, nous nous sommes intéressés à une catégorie particulière d'ARN non codants appelés sRNAs, qui sont impliqués dans la régulation de la réponse cellulaire aux variations environnementales. Nous avons développé une approche permettant de mieux prédire les interactions qu'ils effectuent avec d'autres ARN en nous basant sur une prédiction des interactions, une analyse par enrichissement du contexte biologique de ces cibles, et en développant un système de visualisation spécialement adapté à la manipulation de ces données. Nous avons appliqué notre méthode pour l'étude des sRNAs de la bactérie Escherichia coli. Les prédictions réalisées sont apparues être en accord avec les données expérimentales disponibles, et ont permis de proposer plusieurs nouvelles cibles candidates. / The identification of the interactions occurring at the molecular level is crucial to understand the life process. The aim of this work was to develop methods to model and to predict these interactions for the metabolism and the regulation of transcription. We modeled these systems by graphs and automata.Firstly, we developed a method to test and to predict the flux distribution in a metabolic network, which consider the formulation of several constraints. We showed that this method can better mimic the in vivo phenotype of the energy metabolism of the parasite Trypanosoma brucei. The results enabled to provide a good explanation of the metabolic flux flexibility, which were consistent with the experimental data. Secondly, we have considered a particular class of non-coding RNAs called sRNAs, which are involved in the regulation of the cellular response to environmental changes. We developed an approach to better predict their interactions with other RNAs based on the interaction prediction, an enrichment analysis, and by developing a visualization system adapted to the manipulation of these data. We applied our method to the study of the sRNAs interactions within the bacteria Escherichia coli. The predictions were in agreement with the available experimental data, and helped to propose several new target candidates.

Bioinformatique

Graphe

Réseau de Petri

Métabolisme

Flux Balance Analysis

ARN non codant

Prédiction des cibles des sRNAs

Bioinformatic

Graph

Petri nets

Metabolism

Flux Balance Analysis

Non-coding RNA

SRNA target prediction

Macromolecular Matchmaking : Mechanisms and Biology of Bacterial Small RNAs

Holmqvist, Erik

January 2012

Cells sense the properties of the surrounding environment and convert this information into changes in gene expression. Bacteria are, in contrast to many multi-cellular eukaryotes, remarkable in their ability to cope with rapid environmental changes and to endure harsh and extreme milieus. Previously, control of gene expression was thought to be carried out exclusively by proteins. However, it is now clear that small regulatory RNAs (sRNA) also carry out gene regulatory functions. Bacteria such as E. coli harbor a large class of sRNAs that bind to mRNAs to alter translation and/or mRNA stability. By identifying mRNAs that are targeted by sRNAs, my studies have broadened the understanding of the mechanisms that underlie sRNA-dependent gene regulation, and have shed light on the impact that this type of regulation has on bacterial physiology. Control of gene expression often relies on the interplay of many regulators. This interplay is exemplified by our discovery of mutual regulation between the sRNA MicF and the globally acting transcription factor Lrp. Through double negative feedback, these two regulators respond to nutrient availability in the environment which results in reprogramming of downstream gene expression. We have also shown that both the transcription factor CsgD, and the anti-sigma factor FlgM, are repressed by the two sRNAs OmrA and OmrB, suggesting that these sRNAs are important players in the complex regulation that allow bacteria to switch between motility and sessility. Bacterial populations of genetically identical individuals show phenotypic variations when switching to the sessile state due to bistability in gene expression. While bistability has previously been demonstrated to arise from stochastic fluctuations in transcription, our results suggest that bistability possibly may arise from sRNA-dependent regulatory events also on the post-transcriptional level.

Small RNA

sRNA

non-coding RNA

antisense

gene regulation

post-transcriptional regulation

translational control

outer membrane protein

OmpA

MicA

biofilm

flagella

curli

bistability

Lrp

MicF

CsgD

FlgM

OmrA

OmrB

Regulace exprese Ms1, sRNA z Mycobacterium smegmatis / Regulation of expression of Ms1, a sRNA from Mycobacterium smegmatis

Páleníková, Petra

January 2016

Bacteria are exposed to various environmental conditions during their growth. They have to cope with rapid changes in temperature, lack of nutrition, etc. To survive, bacteria alter their gene expression. One type of regulation of gene expression is regulation by small RNAs (sRNAs). In bacteria, a well-studied sRNA is 6S RNA that binds to the RNA polymerase holoenzyme. However, 6S RNA has not been identified in several bacterial species. Mycobacteria are a genus that probably does not have 6S RNA. Instead, Mycobacterium smegmatis possess another sRNA - Ms1. Ms1 structurally resembles 6S RNA and indeed it was first identified as a 6S RNA structural homologue. However, Ms1 binds to RNAP devoid of any sigma factor, and, therefore, is significantly distinct from 6S RNA. This work describes regulation of expression of Ms1. DNA fragments of different length from the region upstream of the Ms1 gene were prepared. These fragments were fused to the lacZ reporter gene and their activity was tested in different growth phases and under stress. This allowed identification and characterization of the core promoter sequence and regulatory sequences that might interact with transcription factor(s). Promoter activity increased with increased length of the promoter fragment and after transition into stationary...

RNA-Seq and proteomics based analysis of regulatory RNA features and gene expression in Bacillus licheniformis

Wiegand, Sandra

25 September 2013

No description available.

570

dRNA-Seq

RNA-based regulation

proteomics

industrial production

stress response

sporulation

lichenicidin

RNA-Seq

Subtilisin Carlsberg

transcriptomics

reannotation

operon prediction

differential gene expression

antisense RNA

transcription start site

ncRNA

UTR

sRNA

Geobacillus sp. GHH01

Biologie (PPN619462639)