Identification de marqueurs de susceptibilité dans les formes chroniques de la maladie de Chagas / Identification of genetic markers in chronic chagas cardiomyopathy

Laugier, Laurie

02 October 2017

La maladie de Chagas est une maladie parasitaire causée par le protozoaire Trypanosoma cruzi et transmise par des insectes hématophages . Elle est composée de 2 phases : la phase aiguë et la phase chronique. Parmi les individus infectés, 30 % développent la forme chronique de la maladie. Les patients présentent des atteintes cardiaques, digestives (œsophage, côlon) et cardiodigestives. Notre étude a été focalisée sur les patients atteints de cardiomyopathie chagasique (CCC). Notre objectif est d’identifier des gènes de susceptibilité pouvant être impliqués dans le développement des formes chroniques. Notre étude a permis de mettre en évidence une variation d’expression de certains gènes entre les CCC et les contrôles. Nous nous sommes également intéressés aux processus épigénétiques pouvant réguler l’expression des gènes. Une étude de la méthylation de l’ADN croisée avec l’étude du transcriptome nous ont permis d’identifier des gènes présentant à la fois des variations d’expression et de méthylation. Pour certains de ces gènes, nous avons démontré que la méthylation est responsable de la variation d’expression observée. Enfin, nous avons étudié un ARN long non-codant, MIAT. Nous avons démontré qu’il est surexprimé chez les CCC par rapport aux contrôles et dans un modèle murin infecté par T. cruzi. De plus, l’analyse de l’expression de micro-ARNs couplée à une analyse de transcriptome nous a permis d'identifier plusieurs micro-ARNs indispensables à la régulation de l’expression des gènes. Enfin, une étude protéomique nous a permis de mettre en évidence une augmentation de la production de protéine pour certains gènes, en lien avec l’augmentation de l’expression observée. / Chagas disease is a parasitic disease caused by the protozoan Trypanosoma cruzi and transmitted by the hematophagous insects. The disease is composed by acute and chronic phases. Among the infected individuals, 30 % develop chronic form. They suffer from heart, digestive (esophagus, colon) and cardiodigestives injury. Our study was focused on patients with dilated chagasic cardiomyopathy (CCC). Our goal is to identify susceptibility genes that may be involved in the development of chronic forms. Our study revealed a variation in the expression of certain genes between CCC group and controls. We are also interested in epigenetic processes that can regulate the expression of genes. A study of the DNA methylation crossed with the transcriptome allowed us to identify genes presenting both variations in expression and methylation. For some of these genes we demonstrated that methylation is responsible for the expression variation observed. Finally, we studied a long non-coding RNA called MIAT. Our study demonstrated that it is overexpressed in CCC compared to controls and in a murine model infected by T. cruzi. Furthermore, the analysis of the expression of micro-RNAs crossed with transcriptome analysis allowed us to identify several micro-RNAs whose functions are essential in the regulation of gene expression. Finally, a proteomic study allowed us to demonstrate an increase in the production of protein for certain genes, correlated with the increase in expression levels observed.

Maladie de Chagas

Trypanosoma cruzi

Cardiomyopathie dilatée

Transcriptome

Méthylation de l’ADN

Micro-ARNs

ARNs longs non-Codants

Protéine.

Chagas disease

Trypanosoma cruzi

Dilated cardiomyopathy

Transcriptome

DNA methylation

Micro-RNAs

Long non-Coding RNAs

Protein.

Réponse des agents non codants du génome – éléments transposables et petits ARN – à un événement d'allopolyploïdie : le génome du colza (Brassica napus) comme modèle d'étude / Response of non-coding components of the genome – transposable elements and small non-coding RNAs – to a new allopolyploidisation event : the genome of oilseed rape (Brassica napus) as a model of study

Martinez Palacios, Paulina

28 March 2014

Le succès évolutif de la polyploïdie, notamment de l’allopolyploïdie (où la duplication de génome complet est associée à une hybridation entre génomes différenciés) est en partie lié au fait que cet événement s’accompagne de nombreux changements dans l'organisation du génome et la régulation de l'expression des gènes. On parle du « choc génomique » de l’hybridation interspécifique et de l’allopolyploïdie. Ces sources de diversité génétique, à la fois structurale et fonctionnelle, apparaissent utiles et nécessaires à l'adaptation et l’évolution des espèces. Alors que de nombreuses études portant sur la compréhension des mécanismes moléculaires à l’origine du succès des allopolyploïdes ont concerné les modifications de l’expression des gènes, mes travaux de thèse ont porté sur les agents non codants du génome que sont les éléments transposables et les petits ARN non codants. Le modèle d'étude est le colza (Brassica napus, AACC), espèce allotétraploïde issue de l'hybridation entre les espèces diploïdes navette (B. rapa, AA) et chou (B. oleracea, CC). Nous disposions de colzas néo-synthétisés, étudiés à différentes générations d’autofécondation, permettant de caractériser les changements génomiques accompagnant la formation puis l’évolution du génome néo-allopolyploïde. Une étude a tout d’abord été menée sur un élément transposable (ET) spécifique du génome C, Bot1, en vue d’identifier de nouvelles transpositions survenant chez les colzas néo-synthétisés par rapport aux parents diploïdes, par une approche SSAP. Quelques rares événements de transposition ont été identifiés. Ces résultats, confrontés à ceux obtenus sur deux autres ET, ont permis de mettre en évidence un impact modéré de l’allopolyploïdie sur la transposition de ces différents ET. Par contre, il est apparu que des changements de méthylation auraient accompagné cette allopolyploïdisation, sans doute à l’origine de la réactivation et la transposition de quelques copies de Bot1. Les petits ARN non codants ont été suggérés comme impliqués dans les différents événements génomiques accompagnant la formation d’un génome allopolyploïde. Pour étudier la dynamique d’expression des petits ARN chez des colzas néo-synthétisés pris à deux générations d’autofécondation (S1, S5) en comparaison de leurs parents diploïdes, j’ai exploité des données de séquençage haut débit obtenues pour 11 banques construites à partir des tiges de ces différents génotypes. J’ai ainsi démontré, qu’à une échelle globale, les petits ARN présentaient une réponse immédiate mais transitoire à l’événement d’allopolyploïdie. Les fractions particulièrement affectées par l’allopolyploïdie se sont révélées correspondre (1) à des petits ARN interférents dérivés d’éléments transposables avec une baisse de leur abondance en génération précoce S1, et (2) à des populations de petits ARN de 21 nucléotides exprimées uniquement de manière très précoce, de l’hybride F1 à la génération S1. Nous avons notamment identifié des transcrits de type viral correspondant à ces petits ARN de 21-nt, et présentant les mêmes profils d’expression (de l’hybride F1 à la génération S1), suggérant une réactivation d’éléments viraux endogènes (EVE) en réponse à l’hybridation et l’allopolyploïdie. L’ensemble de mon étude a démontré la mise en place d’une succession des voies de régulation par petits ARN où ET et EVE, réactivés au niveau transcriptionnel, sont immédiatement soumis à une répression post-transcriptionnelle (PTGS), renforcée ensuite par une répression de leur transcription (TGS). L’hypothèse d’une absence de cette régulation par petits ARN lors des phénomènes de nécrose et létalité hybride, amène à envisager ces populations de petits ARN comme les clés de la réussite de la formation d’un génome hybride, où la répression immédiate et efficace des ET et autres endovirus, réactivés suite au choc génomique, se révèle être une nécessité. / The evolutionary success of polyploid species is partly due to the dynamic changes in genome organization and gene expression patterns that occur at the onset of the polyploid formation. These changes are promoted by the merging of divergent genomes into a single nucleus (i.e. allopolyploidy) that causes a “genomic shock”; they are thought to provide a rich source of new genetic material upon which selection can act to promote adaptation and evolution. Many studies have thus aimed to uncover molecular mechanisms that are responsible for the evolutionary success of allopolyploid species, most of them focusing on gene expression changes. In the present PhD thesis, my interest has been concentrated on the non-coding components of the genome: transposable elements and small non-coding RNAs. My study involves oilseed rape (Brassica napus, AACC), a relatively young allopolyploid species that originated from hybridizations between B. rapa (AA) and B. oleracea (CC). Specifically, I have used resynthesized B. napus polyploids advanced by self-pollination of single plants for several generations; I have analyzed these plants at different generations for genomic changes accompanying polyploid formation and subsequent evolution. In a first part, sequence-specific amplification polymorphism (SSAP) targeting the C genome-specific transposable element Bot1, was used to evaluate transposition rate of Bot1 in resynthesized B. napus in comparison with the diploid parents. Only a few transposition events were identified. When combined with the results obtained for two other TEs, this work suggests that allopolyploidy has only a moderate impact on TE transposition and restructuring. The changes observed in SSAP profiles led us to hypothesize that some of them resulted from changes in DNA methylation, resulting in rare but highly specific TE activation and transposition. In a second part, I have concentrated on small non-coding RNAs (sRNAs), which are thought to mediate different aspects of the response to the “genomic shock” induced by allopolyploid formation. Comprehensive analyses of sRNA expression in resynthesized B. napus allopolyploids have been carried out by deep sequencing sRNAs from 11 libraries prepared from stems of three allotetraploids (surveyed at the two generations S1 and S5) and the two diploid parents. Characterization of sRNA distributions in these plants indicates that sRNAs show an immediate but transient response to allopolyploidy. The sRNAs derived from transposable elements (down-regulated in the S1) or targeting unknown sequences (no Blast hit against any available public database) were particularly affected. The use of B. napus mRNAseq data revealed that these latest unknown candidates, which are 21-nt long and over-expressed in the earliest generations (F1, S0, S1) were derived from endogenous viral elements (EVE). We confirmed that these EVEs showed the same expression patterns as the 21-nt long sRNAs that specifically target them (over-expression in the F1, S0 and S1). These results suggest that (at least) some EVEs might be reactivated as a response to the merging of divergent genomes (in interspecific hybrids and newly formed allopolyploids). Altogether, our results have demonstrated a succession of sRNA pathways that counteract the reactivation of some specific TEs and/or EVEs at the onset of polyploid formation; reactivated TEs and/or EVEs being immediately repressed at the post-transcriptional level (PTGS), and then fully repressed by transcriptional gene silencing (TGS) in the subsequent generations. Such data lead to hypothesize that sRNAs are essential to overcome interspecific hybrid incompatibilities due to the uncontrolled and deleterious reactivation of TEs / EVEs. Therefore, sRNAs should be considered as the guardians of genome integrity even in newly-formed allopolyploids.

Allopolyploïdie

Brassica

Éléments transposables

Éléments viraux endogènes (EVE)

Micro ARN (miRNAs)

Petits ARN interférents (siRNAs)

Petits ARN non codants

Séquençage haut débit (NGS)

Allopolyploidy

Brassica

Transposable elements

Endogenous viral elements (EVEs)

Micro RNAs (miRNAs)

Small interfering RNAs (siRNAs)

Small non-coding RNAs

Next generation sequencing (NGS)

Host-Pathogen Interactions in Hepatitis C Virus Infection : Deciphering the Role of Host Proteins and MicroRNAs

Shwetha, S

January 2015

Host-pathogen interactions in Hepatitis C Virus infection: Deciphering the role of host proteins and microRNAs Hepatitis C virus (HCV) is a positive sense single stranded RNA virus belonging to the Hepacivirus genus of the Flaviviridae family. HCV genome consists of a single open reading frame flanked by highly structured 5‟ and 3‟ untranslated regions (UTRs) at both ends. Unlike cellular mRNAs, HCV RNA translation is independent of the cap structure and is mediated by an internal ribosomal entry site (IRES) present in the 5‟UTR. HCV replication begins with the synthesis of a complementary negative-strand RNA using the positive strand RNA genome as a template catalyzed by the NS5B RNA dependent RNA polymerase (RdRp). The de novo priming of HCV RNA synthesis by NS5B occurs at the very end of the 3‟UTR. The 3‟UTR is organized into highly structured regions namely the variable region, poly U/UC region and the 3‟X region. These regions contain cis-acting elements that determine the efficiency of viral replication. In addition, the interaction of trans-acting factors with the 3‟ UTR is also important for regulation of HCV replication. HCV 3‟UTR interacts with several cellular proteins such as the human La protein, polypyrimdine tract binding protein (PTB), poly (rC)-binding protein 2 (PCBP2) and Human antigen R (HuR). However, the molecular basis of regulation of viral replication by these proteins is not well understood. Many proteins that are hijacked by HCV as well as other cytoplasmic RNA viruses, such as La, PCBP2, HuR and PTB are RNA binding proteins (RBPs). They are involved in post transcriptional regulation of cellular gene expression. Thus the subversion of these proteins by the virus can affect their normal physiological functions. In addition to proteins, recent reports also describe the involvement of non-coding RNAs including microRNAs (miRNA) and long non coding RNAs (lncRNA) in HCV infection. miRNAs can either directly bind to the HCV genome and regulate its life cycle or indirectly modulate the expression of host proteins required by the virus. miRNAs that are differentially regulated in virus infected tissues or body fluids of infected patients can also serve as biomarkers for diagnosis of various stages of the disease. Hence, it was planned to study the role of host proteins and miRNAs in the HCV life cycle and pathogenesis to have novel insights into the biology of HCV infection. Riboproteomic studies have identified several host proteins that directly interact with the 5‟ and/or 3‟UTRs of the HCV RNA. One of the RNA binding proteins that predominantly interact with the 3‟UTR of HCV RNA was found to be HuR. In the present study, we have extensively characterized the interaction between HuR and HCV 3‟UTR and studied its functional implications in HCV life cycle along with other host factors. Characterizing the HCV 3’UTR–HuR interaction and its role in HCV replication HuR is a ubiquitously expressed member of the Hu family which shuttles between the nucleus and cytoplasm in response to stress. Whole genome siRNA knockdown and other studies have suggested that HuR is essential for HCV replication. However, the molecular mechanism of its involvement in this process was not clear. We observed that siRNA mediated knockdown of HuR reduces the HCV RNA and protein levels. Immunofluorescence studies indicated that HuR relocalizes from the nucleus to the cytoplasm in HCV infected cells. Through confocal microscopy and GST pulldown assays, we have demonstrated that HuR co localizes with the viral polymerase, NS5B and directly interacts with the NS5B protein. Membrane flotation assays showed that HuR is present in the detergent resistant membrane fractions which are the active sites of HCV replication. In addition to the interaction of HuR with the viral protein NS5B, we also characterized its interaction with the viral RNA. Direct UV cross linking assays and UV cross linking immunoprecipitation assays were performed to demonstrate the interaction of HuR with the HCV 3‟UTR. The RRM3, hinge region and RRM1 of HuR were found to be important for binding. Further, we observed that HuR competes with PTB for binding to the 3‟UTR when cytoplasmic S10 extracts or recombinant proteins were used in UV cross linking assays. In contrast, the addition of HuR facilitated the binding of La protein to the HCV 3‟UTR in the above assays. Competition UV cross linking assays indicated that both HuR and PTB bind to the poly U/UC region of the 3‟UTR while La binds to the variable region. HuR and La showed higher affinities for binding to the 3‟UTR as compared to PTB in filter binding assays. Since HuR and PTB interact with the same region on the 3‟UTR and HuR showed ~4 fold higher affinity for binding, it could displace PTB from the 3‟UTR. Next, we investigated the roles of HuR, PTB and La in HCV translation and replication in cell culture using three different assay systems, HCV sub genomic replicon, HCV bicistronic SGR-JFH1/Luc replicon as well as the infectious HCV full length RNA (JFH1). Results clearly indicated that HuR and La are positive modulators of HCV replication. Interestingly, PTB facilitated HCV IRES mediated translation but appeared to have a negative effect on HCV replication. The positive effectors, HuR and La showed significant co localization with one another in the cytoplasm in immunofluorescence studies. GST pulldown and coimmunoprecipitation experiments indicated protein-protein interactions between HuR and La but not between HuR and PTB. Through quantitative IP-RT assays, we demonstrated that the overexpression of HuR in HCV RNA transfected cells increases the association of La with the HCV RNA while HuR knockdown reduces the association of La with the HCV RNA. Previous studies in our laboratory have shown that La helps in HCV genome circularization. The addition of HuR significantly increased La mediated interactions between the 5‟UTR and the 3‟UTR of HCV RNA as monitored by 5‟-3‟ co precipitation assays, suggesting a possible mechanism by which cooperative binding of HuR and La could positively regulate HCV replication. Taken together, our results suggest a possible interplay between HuR, PTB and La in the regulation of HCV replication. Studying the role of HuR- associated cellular RNAs in HCV infection HuR belongs to the category of mRNA turnover and translation regulatory proteins (TTR-RBPs), which are capable of triggering rapid and robust changes in cellular gene expression. HuR plays a role in several post transcriptional events such as mRNA splicing, export, stability and translation. In the present study, we have investigated the possible consequences of relocalization of HuR on cellular processes in the context of HCV infection. We observed that 72h post transfection of infectious HCV-JFH1 RNA, there is an increase in the mRNA levels of some of the validated targets of HuR including the vascular endothelial growth factor A (VEGFA), dual specificity phosphatise 1 (MKP1) and metastasis - associated lung adenocarcinoma transcript (MALAT1). IP-RT assays demonstrated that the association of HuR with VEGFA and MKP1 was higher in HCV-JFH1 RNA transfected cells as compared to the mock transfected cells indicating that increase in HuR association could probably help in stabilization of these mRNAs. Interestingly, we observed that the association of HuR with the lncRNA MALAT1 decreases in the presence of HCV RNA, while its RNA levels increased. Earlier it has been reported that MALAT1 interacts with HuR and was predicted to interact with La. We confirmed the interaction of both HuR and La proteins with MALAT1 RNA in vitro and in the cell culture system. Results from our time course experiments suggest that relocalization of HuR and La upon HCV infection might decrease their association with the nuclear retained MALAT1 RNA leading to significant reduction in MALAT1 RNA levels at the initial time points. However at later time points, MALAT1 was found to be unregulated through activation of the Wnt/beta-catenin pathway as demonstrated using a chemical inhibitor against β-catenin. Since MALAT1 is a known regulator of epithelial mesenchymal transition (EMT) and metastasis, we further studied the physiological consequence of the observed increase in MALAT1 levels upon HCV infection. Cell migration and cell invasion studies suggested that the knockdown of MALAT1 led to the inhibition of HCV- triggered wound healing and matrigel invasion and also rescued the down regulation of E-Cadherin protein levels, an EMT marker. Our study highlights the importance of the lncRNA, MALAT1 in HCV infection and suggests its possible involvement in HCV induced HCC. Investigating the role of miRNAs in HCV pathogenesis and replication miRNAs can also regulate HCV infection and pathogenesis in multiple ways. It is known that under disease conditions, there is aberrant expression of intracellular as well as circulating miRNAs. We have investigated the expression profile of 940 human miRNAs in HCV infected patient serum samples to identify the differentially regulated miRNAs. miR-320c, miR-483-5p and the previously reported miR-125b were found to be upregulated in the serum of cirrhotic and non-cirrhotic HCV infected patient serum samples. All three miRNAs were also unregulated in the cell culture supernatant of HCV infected cells as well as within the HCV infected cells. miR-483-5p was specifically enriched in the exosomes isolated from patient serum samples. Knockdown of miR-320c and miR-483-5p did not have significant effect on HCV replication while knockdown of miR-125b affected HCV replication through regulation of one of its target genes, HuR. We observed that with time, miR-125b levels in HCV-JFH1 RNA transfected cells increase while the HuR protein levels decrease. Using luciferase reporter constructs, we demonstrated that the decrease in HuR protein levels is indeed mediated by miR-125b. Mutations in the target site of miR-125b in the HuR 3‟UTR prevented the down regulation of luciferase activity. Next we tested the effect of silencing miR-125b on HCV replication. Knockdown of miR-125b prevented the reduction in HuR protein levels but with no significant effect on HCV replication. It appeared that the HuR protein already present in the cytoplasm could be sufficient to support HCV replication. Hence similar experiments were carried out in cells depleted of HuR using either siRNA against HuR or a chemical inhibitor of nucleocytoplasmic transport of HuR, Leptomycin B. We observed that when the intracellular levels of HuR are reduced using either of the two approaches, there is a decrease in HCV replication. This is in accordance with the results obtained in the first part of the thesis. However when miR-125b was silenced in HuR depleted cells, we noticed an upregulation in the HuR protein levels by western blot analysis and a consequent increase in HCV RNA levels as quantified by qRT-PCR. From our findings, we can conclude that miR-125b mediated regulation of HuR plays an important role in HCV replication. We hypothesize that this could be a cellular response to HCV infection to which the virus responds by inducing protein relocalization. Altogether, these studies outline the importance of host factors including cellular proteins and non-coding RNAs in the regulation of HCV life cycle and pathogenesis. Results reveal the mechanistic insights into how HCV infection triggers host defense pathways, which are evaded by the virus by counter strategies.

Hepatitis C Virus Infection

Micro RNAs - HCV Infection

RNA Viruses

Hepatitis C Virus Replication

Hepatitis C Virus (HCV) RNA Binding

Viral Proteins

Host Proteins-HCV Infection

Hepatitis C Virus Pathogenesis

Hepatitis C Virus Diagnosis and Therapy

HCV-RNA Translation

HCV - miRNA

HCV Replication

HCV IRES

HCV Pathogenesis

Microbiology and Cell Biology