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CHK2 is Negatively Regulated by Protein Phosphatase 2AFreeman, Alyson 31 May 2010 (has links)
Checkpoint kinase 2 (CHK2) is an effector kinase of the DNA damage response pathway and although its mechanism of activation has been well studied, the attenuation of its activity following DNA damage has not been explored. Here, we identify the B'α subunit of protein phosphatase 2A (PP2A), a major protein serine/threonine phosphatase of the cell, as a CHK2 binding partner and show that their interaction is modulated by DNA damage. B'α binds to the SQ/TQ cluster domain of CHK2, which is a target of ATM phosphorylation. CHK2 is able to bind to many B' subunits as well as the PP2A C subunit, indicating that it can bind to the active PP2A enzyme. The induction of DNA double-strand breaks by ionizing radiation (IR) as well as treatment with doxorubicin causes dissociation of the B'α and CHK2 proteins, however, it does not have an effect on the binding of B'α to CHK1. IR-induced dissociation is an early event and occurs in a dose-dependent manner. CHK2 and B'α can re-associate hours after DNA damage and this is not dependent upon the repair of the DNA. Dissociation is dependent on ATM activity and correlates with an increase in the ATM-dependent phosphorylation of CHK2 at serines 33 and 35 in the SQ/TQ region. Indeed, mutating these sites to mimic phosphorylation increases the dissociation after IR. CHK2 is able to phosphorylate B'α in vitro; however, in vivo, irradiation has no effect on PP2A activity or localization. Alternatively, PP2A negatively regulates CHK2 phosphorylation at multiple sites, as well as its kinase activity and protein stability. These data reveal a novel mechanism for PP2A to keep CHK2 inactive under normal conditions while also allowing for a rapid release from this regulation immediately following DNA damage. This is followed by a subsequent reconstitution of the PP2A/CHK2 complex in later time points after damage, which may help to attenuate the signal. This mechanism of CHK2 negative regulation by PP2A joins a growing list of negative regulations of DNA damage response proteins by protein serine/threonine phosphatases.
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Mapping of UV-Induced Mitotic Recombination in YeastYin, Yi January 2015 (has links)
<p>In diploid yeast cells, mitotic recombination is very important for repairing double-strand breaks (DSB). When repair of a DSB results in crossovers, it may cause loss of heterozygosity (LOH) of markers centromere-distal to the DSB in both daughter cells. Gene conversion events unassociated with crossovers cause LOH for an interstitial section of a chromosome. Alternatively, DSBs can initiate break-induced replication (BIR), causing LOH in only one of the daughter cells. Mapping mitotic LOH contributes to understanding of mechanisms for repairing DSBs and distribution of these recombinogenic lesions. Methods for selecting mitotic crossovers and mapping the positions of crossovers have recently been developed in our lab. Our current approach uses a diploid yeast strain that is heterozygous for about 55,000 SNPs, and employs SNP-Microarrays to map LOH events throughout the genome. These methods allow us to examine selected crossovers on chromosome V and unselected mitotic recombination events (crossovers, gene conversion events unassociated with crossovers, and BIR events) at about 1 kb resolution across the genome.</p><p>Mitotic recombination can be greatly induced by UV radiation. However, prior to my research, the nature of the recombinogenic lesions and the distribution of UV-induced recombination events were relatively uncharacterized. Using SNP microarrays, we constructed maps of UV-induced LOH events in G1-synchronized cells. Mitotic crossovers were stimulated 1500-fold and 8500-fold by UV doses of 1 J/m2 and 15 J/m2, respectively, compared to spontaneous events. Additionally, cells treated with 15 J/m2 have about eight unselected LOH events per pair of sectors, including gene conversions associated and unassociated with crossovers as well as BIR events. These unselected LOH events are distributed randomly throughout the genome with no particular hotspots; however, the rDNA cluster was under-represented for the initiation of crossover and BIR events. Interestingly, we found that a high fraction of recombination events in cells treated with 15 J/m2 reflected repair of two sister chromatids broken at roughly the same position. In cells treated with 1 J/m2, most events reflect repair of a single broken sister chromatid (Chapter 2). </p><p>The primary pathway to remove pyrimidine dimers introduced by UV is the nucleotide excision repair (NER) pathway. In NER, the dimer is excised to generate a 30-nucleotide gap that can be replicated to form DSBs if not filled in before DNA replication. The NER gap can also be expanded by Exo1p to form single stranded gaps greater than one kilobase. Alternatively, in the absence of NER, unexcised dimers could result in blocks of DNA replication forks. Resolving the stalled replication fork could lead to recombinogenic breaks. In Chapter 3 and Chapter 4, we analyzed recombination events in strains defective in various steps of processing of UV-induced DNA damage, including exo1 and rad14 mutants. </p><p>In Chapter 3, I show that Exo1p-expanded NER gaps contribute to UV-induced recombination events. Interestingly, I also found that Exo1p is also required for the hotspot activity of a spontaneous crossover hotspot involving a pair of inverted Ty repeats. In addition to its role of expanding a nick to a long single-stranded gap, Exo1p is also a major player in DSB end resection. Therefore, I examined the gene conversion tract lengths in strains deleted for EXO1. I found that, although crossover-associated gene conversion tracts become shorter in the exo1 mutant as expected, noncrossover tract lengths remained unaffected. As a result, noncrossover tracts are longer than crossover tracts in the exo1 mutant while the opposite result was observed in the wild-type strains. I proposed models to rationalize this observation.</p><p>In Chapter 4, to investigate whether the substantial recombinogenic effect in UV in G1-synchronized cells requires NER, we mapped UV-induced LOH events in NER-deficient rad14 diploids treated with 1 J/m2. Mitotic recombination between homologs was greatly stimulated, which suggests that dimers themselves can also cause recombination without processing by NER. We further show that UV-induced inter-homolog recombination events (noncrossover, crossover and BIR) depend on the resolvase Mus81p, and are suppressed by Mms2p-mediated error-free post-replication repair pathway. </p><p>The research described in Chapters, 2, 3, and 4 are in the publications Yin and Petes (2013), Yin and Petes (2014), and Yin and Petes (2015), respectively.</p> / Dissertation
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Réparation des cassures double-brin et variabilité chromosomique chez Streptomyces / Double-strand break repair and chromosomal variability in StreptomycesHoff, Grégory 13 December 2016 (has links)
Rayons ionisants, dessiccation, ou encore métabolites secondaires exogènes sont autant de facteurs qui peuvent engendrer des dommages à l’ADN chez les bactéries du sol, notamment en provoquant la formation de cassures double-brin (DSB), préjudice majeur pour une cellule. Chez les procaryotes, l’évolution a sélectionné deux principaux mécanismes de réparation des DSB, à savoir la recombinaison homologue (RH) et le non-homologous end joining (NHEJ). La RH est un mécanisme quasi-ubiquiste dans le monde bactérien qui repose sur l’utilisation d’une copie intacte de la molécule endommagée comme matrice pour la réparation de la DSB. Contrairement à la RH, le NHEJ n’est présent que chez 20 à 25% des bactéries et est considéré comme un mécanisme mutagène puisque la réparation de la DSB se fait sans matrice homologue et peut entrainer l’ajout ou la délétion de nucléotides au site de cassure. Chez la bactérie modèle Mycobacterium, seuls deux acteurs sont nécessaires pour la réparation par NHEJ. Ainsi, un dimère de protéine Ku se fixe sur la cassure puis recrute la protéine multifonctionnelle LigD, qui catalyse le traitement puis la ligation des extrémités grâce à ses domaines polymérase, nucléase et ligase. Les mécanismes de réparation des DSB chez les Streptomyces étaient peu connus à l’initiation de ce travail. Cette bactérie présente des caractéristiques génomiques remarquables avec notamment un chromosome linéaire de grande taille (6 à 12 Mb). En ce qui concerne la RH, nous avons focalisé nos recherches sur les étapes tardives (post-synaptiques) et étudié le rôle du complexe RuvABC et de RecG impliqués chez Escherichia coli dans la migration de la croix de Holliday et de sa résolution. La construction de mutants simples et multiples a montré que bien que les gènes codant ces protéines soient très conservés chez les Streptomyces, leur déficience ne se traduit chez Streptomyces ambofaciens que par une faible baisse de la recombinaison suite à un événement de conjugaison. Aucune baisse de l’efficacité de recombinaison intrachromosomique n’a en revanche été observée. Ces résultats suggèrent que des acteurs alternatifs majeurs sont encore à découvrir chez les Streptomyces. Le décryptage du mécanisme de NHEJ chez S. ambofaciens constitue une première dans ce genre bactérien. Une étude génomique exhaustive a permis de révéler la très grande diversité du nombre d’acteurs potentiels de ce mécanisme (Ku, LigDom, PolDom, NucDom) et de l’organisation des gènes qui les codent.. L’analyse fonctionnelle a révélé que l’ensemble des acteurs étaient impliqués dans la réponse à l’exposition à un faisceau d’électrons accélérés, connus pour induire, entre autre, la formation de DSB. La génération de DSB, par coupure endonucléasique I-SceI, a par ailleurs permis de mettre en évidence au niveau moléculaire des réparations de type NHEJ (délétions ou insertions de quelques nucléotides, intégration de fragments d’ADN). Les cassures dans les régions terminales du chromosome sont accompagnées de grandes délétions (jusqu’à 2,1 Mb) et de réarrangements de grande ampleur incluant circularisations du chromosome et amplifications d’ADN. Les conséquences de la réparation de DSB chez S. ambofaciens sont en tous points similaires aux réarrangements observés spontanément ou par comparaison des génomes des espèces types. Ainsi, il est possible de lier la plasticité du génome à la réparation de DSB. En outre, l’intégration de matériel génétique exogène serait favorisée au cours de la réparation NHEJ ce qui donnerait à ce système de réparation une place importante dans le processus de transfert horizontal, mécanisme d’évolution majeur chez les bactéries / Ionizing radiation, desiccation or exogenous secondary metabolites are all factors that can cause DNA damage in soil bacteria, especially by triggering double strand breaks (DSB), the most detrimental harm for the cell. In prokaryotes, evolution selected two main DSB repair pathways, namely homologous recombination (HR) and non-homologous end joining (NHEJ). HR is almost ubiquitous in bacteria and relies on an intact copy of the damaged DNA molecule as a template for DSB repair. In contrast to HR, NHEJ is only present in 20 to 25% of bacteria and is considered as a mutagenic pathway since DSB repair is performed without the need of any template and can lead to nucleotide addition or deletion at DSB site. In the bacterial model Mycobacterium, two partners are sufficient for a functional NHEJ pathway. Thus, Ku protein dimer recognizes and binds the DSB and then recruits the multifunctional LigD protein for extremities treatment and ligation thanks to its polymerase, nuclease and ligase domains. At the beginning of this work, few informations on DSB repair in Streptomyces were available. This bacteria exhibits remarkable genomic features including a large linear chromosome (6 to 12 Mb). Regarding HR, we focused on the late stage (post-synaptic step) in studying the role of RuvABC complex and RecG, involved in branch migration and Holliday junction resolution in E. coli. Construction of single and multiple mutants showed that although the genes encoding these proteins are highly conserved in Streptomyces, their deficiency in Streptomyces ambofaciens only results in a mild decrease of recombination after conjugation events. Besides, no decrease of intrachromosomal recombination efficiency could be observed. These results suggest that major alternative factors are still to be discovered in Streptomyces. This work was also the first occasion to decipher a NHEJ pathway in Streptomyces. An exhaustive genomic study revealed a great diversity in the number of factors potentially implicated in this pathway (Ku, LigDom, PolDom, NucDom) and in the organization of their encoding genes. Functional analyses revealed that all the factors, whatever they are conserved or not between species, were involved in the response to electron beam exposure, known to induce, amongst other things, DSB formation. Generation of DSB by I-SceI endonuclease cleavage was also used to evidence at a molecular level NHEJ type DSB repair (deletions or insertions of several nucleotides, integration of DNA fragments). Targeted breaks in the terminal regions of the chromosome were accompanied by large deletions (up to 2.1 Mb) and major rearrangements including chromosome circularizations and DNA amplifications. Consequences of DSB repair in S. ambofaciens are in all points similar to chromosome rearrangements observed spontaneously or by comparing genomes of different species. Thus, it is possible to link the genome plasticity to DSB repair. In addition, the integration of exogenous genetic material would be favoured during NHEJ repair which would give this repair system a major role in the horizontal transfer process, known to be a main evolution mechanism in bacteria
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Lentivirus-meditated frataxin gene delivery reverses genome instability in Friedreich ataxia patient and mouse model fibroblastsKhonsari, Hassan January 2015 (has links)
Friedreich ataxia (FRDA) is a progressive neurodegenerative disease with primary sites of pathology in the large sensory neurons of the dorsal root ganglia (DRG) and dentate nucleus of the cerebellum. FRDA is also often accompanied by severe cardiomyopathy and diabetes mellitus. FRDA is caused by loss of frataxin (FXN) expression, which is due to GAA repeat expansion in intron 1 of the FXN gene. Frataxin is a mitochondrial protein important in iron-sulphur cluster (ISC) biogenesis and in the electron transport chain (ETC). As a consequence of impaired mitochondrial energy metabolism, FRDA cells show increased levels of and sensitivity to oxidative stress, which is known to be associated with genome instability. In this study, we investigated DNA damage/repair in relation to FXN expression via immunostaining of γ-H2AX, a nuclear protein that is recruited to DNA double strand breaks (DSBs). We found FRDA patient and YG8sR FRDA mouse model fibroblasts to have inherently elevated DNA DSBs (1.8 and 0.9 foci/nucleus) compared to normal fibroblasts (0.6 and 0.2 foci/nucleus, in each case P < 0.001). By delivering the FXN gene to these cells with a lentivirus vector (LV) at a copy number of ~1/cell, FXN mRNA levels reached 48 fold (patient cells) and 42 fold (YG8sR cells) and protein levels reached 20 fold (patient cells) and 3.5 fold (YG8sR cells) that of untreated fibroblasts, without observable cytotoxicity. This resulted in a reduction in DNA DSB foci to 0.7 and 0.43 (in each case P < 0.001) in human and YG8sR fibroblasts, respectively and an increase in cell survival to that found for normal fibroblasts. We next irradiated the FRDA fibroblasts (2Gy) and measured their DSB repair profiles. Both human and mouse FRDA fibroblasts were unable to repair damaged DNA. However, repair returned to near normal levels following LV FXN gene transfer. Our data suggest frataxin may be important for genome stability and cell survival by ensuring ISC for DNA damage repair enzymes or may be required directly for DNA DSB repair.
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Elucidating the role of altered DNA damage response in Nup98-associated leukaemiaNilles, Nadine 01 March 2018 (has links)
Acute myeloid leukaemia is a heterogeneous disease characterized by uncontrolled proliferation of neoplastic haematopoietic precursor cells, which leads to the disruption of normal haematopoiesis and bone marrow failure. Impaired haematopoiesis is often associated with balanced chromosomal translocations that involve the nucleoporin Nup98 fused to around 30 different partner genes, such as the homeobox genes HOXA9 and PMX1. Nup98-associated AML is characterized by poor prognosis and poor treatment outcome for the patients. The aim of the study was to elucidate the mechanisms underlying chemotherapy-resistance. Previous experiments showed that the expression of Nup98 fusion proteins leads to changes in nuclear organization. Based on these observations, we hypothesize that the expression of Nup98 fusion proteins affect DNA double-strand break (DSB) repair. Our work shows that the expression of Nup98-HoxA9 and Nup98-HHEX in U2OS cells does not induce any DSBs. Further, we examined the repair phenotype of exogenously induced DSBs. Experiments carried out using etoposide (ETO) or neocarzinostatin (NCS) revealed that Nup98 fusion proteins affect non-homologous end joining (NHEJ). The second major DSB repair pathway, homologous recombination (HR), remains unaffected by Nup98 fusion proteins. The repair phenotype showed that at most timepoints analyzed, cells expressing Nup98 fusion proteins present less DSBs that control cells. We further performed single cell gel electrophoresis assays, also called COMET assay. This assay determines the amount of broken DNA at the single cell level. COMET assays showed that cells expressing Nup98-HoxA9 get equally damaged as control cells. Taken together, these results show that Nup98-HoxA9 induces faster DNA repair by affecting NHEJ. Additional experiments, pointed toward a role of p53 in the effect of Nup98 fusion proteins on DSB repair. Monitoring the repair phenotype in a wild-type and p53 depletion background, revealed that the effect of Nup98-HoxA9 on NHEJ is partially p53 dependent. A further search for the potentially implicated factor in the accelerated NHEJ remained inconclusive so far. In conclusion, Nup98-HoxA9 induces accelerated NHEJ in a partially p53-dependent manner. / Option Biologie moléculaire du Doctorat en Sciences / info:eu-repo/semantics/nonPublished
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<em>ATM</em>, <em>ATR</em> and Mre11 complex genes in hereditary susceptibility to breast cancerPylkäs, K. (Katri) 10 April 2007 (has links)
Abstract
Mutations in BRCA1 and BRCA2 explain only about 20% of familial aggregation of breast cancer, suggesting involvement of additional susceptibility genes. In this study five DNA damage response genes, ATM, ATR, MRE11, NBS1 and RAD50, were considered as putative candidates to explain some of the remaining familial breast cancer risk, and were screened for germline mutations in families displaying genetic predisposition.
Analysis of ATM indicated that clearly pathogenic mutations seem to be restricted to those reported in ataxia-telangiectasia (A-T). However, a cancer risk modifying effect was suggested for a combination of two ATM polymorphisms, 5557G>A and IVS38-8T>C, as this allele seemed to associate with bilateral breast cancer (OR 10.2, 95% CI 3.1–33.8, p = 0.001).
The relevance of ATM mutations, originally identified in Finnish A-T patients, in breast cancer susceptibility was evaluated by a large case-control study. Two such alleles, 6903insA and 7570G>C, in addition to 8734A>G previously associated with breast cancer susceptibility, were observed. The overall mutation frequency in unselected cases (7/1124) was higher than in controls (1/1107), but a significantly elevated frequency was observed only in familial cases (6/541, p = 0.006, OR 12.4, 95% CI 1.5–103.3). These three mutations showed founder effects in their geographical occurrence, and had different functional consequences at protein level.
In ATR no disease-related mutations were observed, suggesting that it is not a breast cancer susceptibility gene.
The mutation screening of the Mre11 complex genes, MRE11, NBS1 and RAD50, revealed two novel potentially breast cancer associated alleles: NBS1 Leu150Phe and RAD50 687delT were observed in 2.0% (3/151) of the studied families. The subsequent study of newly diagnosed, unselected breast cancer cases indicated that RAD50 687delT is a relatively common low-penetrance susceptibility allele in Northern Finland (cases 8/317 vs. controls 6/1000, OR 4.3, 95% CI 1.5–12.5, p = 0.008). NBS1 Leu150Phe (2/317) together with a novel RAD50 IVS3-1G>A mutation (1/317) was also observed, both being absent from controls. Loss of the wild-type allele was not observed in the tumors of the studied mutation carriers, but they all showed an increase in chromosomal instability of peripheral T-lymphocytes. This suggests an effect for RAD50 and NBS1 haploinsufficiency on genomic integrity and susceptibility to cancer.
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Elucidating Mechanisms of IgH Class Switch Recombination Involving Switch Regions and Double Strand Break JoiningZhang, Tingting January 2011 (has links)
During IgH class switch recombination (CSR) in mature B lymphocytes, activation-induced cytidine deaminase (AID) initiates DNA double strand breaks (DSBs) within switch (S) regions flanking different sets of the IgH locus (IgH) constant \((C_H)\) region exons. End-Joining of DSBs in the upstream donor S region (Sm) to DSBs in a downstream acceptor S region \((S_{acc})\) replaces the initial set of \(C_H\) exons, Cm, with a set of downstream \(C_H\) exons, leading to Ig class switching from IgM to another IgH class (e.g., IgG, IgE, or IgA). In addition to joining to DSBs within another S region, AID-induced DSBs within a given S region are often rejoined or joined to other DSBs in the same S region to form internal switch deletions (ISDs). ISDs were frequently observed in Sm but rarely in \(S_{acc}s\), suggesting that AID targeting to \(S_{acc}s\) requires prior recruitment to Sm. To test this hypothesis, we assessed CSR and ISDs in B cells lacking Sm and found that AID frequently targets downstream \(S_{acc}s\) independently of Sm. These studies also led us to propose an alternative pathway of "downstream" IgE class switching that involves joining of DSBs within the downstream \(S\gamma1\) and \(S\epsilon\) regions as a first step before joining of \(S\mu\) to the hybrid downstream S region. To further elucidate the CSR mechanism, we addressed the long-standing question of whether S region DSBs during CSR involves a direction-specific mechanism similar to joining of RAG1/2 endonuclease-generated DSBs during V(D)J recombination. We used an unbiased high throughput method to isolate junctions between I-SceI meganuclease-generated DSBs at a target site that replaces the IgH \(S\gamma1\) region and other genomic DSBs of endogenous origin. Remarkably, we found that the I-SceI-generated DSBs were joined to both upstream DSBs in \(S\mu\) and downstream DSBs in \(S\epsilon\) predominantly in orientations associated with joining during productive CSR. This process required the DSB response factor 53BP1 to maintain the orientation-dependence, but not the overall levels, of joining between these widely separated IgH breaks. We propose that CSR exploits a mechanism involving 53BP1 to enhance directional joining of DSBs within IgH in an orientation that leads to productive CSR.
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La formation des cassures double-brins méiotiques chez l’espèce modèle Arabidopsis thaliana / Meiotic double-strand breaks formation in the plant model Arabidopsis thalianaVrielynck, Nathalie 10 June 2016 (has links)
La méiose est essentielle pour tous les organismes à reproduction sexuée car cette division cellulaire spécialisée conduit à la formation de gamètes. Au cours de la méiose, la formation de bivalents est une étape clé dans la répartition équilibrée des chromosomes homologues. Dans la majorité des espèces, la formation de ces bivalents repose sur le mécanisme de la recombinaison homologue qui est un mécanisme de réparation des cassures double brin (CDB) de l’ADN. En méiose, la cassure est programmée et provoquée par l’action de Spo11. A.thaliana contient deux homologues SPO11-1 et SPO11-2 qui ne sont pas redondants dans la formation des CDB. Spo11 est une protéine apparentée à la sous-unité A des topoVI d’Archaea. Or, les topoVI d’Archaea fonctionnent en hétérotétramère composé de deux sous-unités A et deux sous-unités B pour former une cassure double brin (CDB) mais jusqu'à mon travail de thèse, aucun homologue méiotique de sous unité B n'avait été identifié. Au cours de ma thèse, j’ai caractérisé la fonction méiotique de la protéine MTOPVIB et montré que c’est un homologue structural de la sous-unité B des TopoVI d’Archaea. Par différentes approches, j’ai montré que MTOPVIB est nécessaire à l’hétérodimérisation de SPO11-1 avec SPO11-2 et je propose que chez A. thaliana, un complexe catalytique de type TopoVI composé de MTOPVIB, SPO11-1, et SPO11-2 est nécessaire à la formation des CDB méiotiques. Chez A. thaliana, en plus de SPO11-1, SPO11-2 et MTOPVIB, quatre autres protéines sont nécessaires à la formation des CDB : PRD1, PRD2, PRD3 et DFO. Par des approches double hybride, j’ai analysé le réseau d’interaction entre ces protéines de « cassure ». Les résultats suggèrent que ces protéines interagiraient au sein d’un « super » complexe essentiel à la formation des CDB méiotiques. / Meiosis is an essential step in sexual reproduction because it leads to the formation of haploid gametes. During meiosis, the formation of bivalents is a key step for the balanced chromosome distribution. In most species, the formation of bivalents lies on the mechanism of homologous recombination that is a repair mechanism for double stranded DNA breaks (DSB). In meiosis, DSB formation is programmed and provoked by the action of Spo11. A.thaliana contains two SPO11-1 and SPO11-2 counterparts which are not redundant in the formation of DSB. Spo11 is related to the A subunit of Archaea topoVI. However, Archaea topoVI operate through a heterotetramer composed of two A subunits and two B subunits but until my thesis work, no meiotic homolog of the B subunit had been identified. During my thesis, I characterized the meiotic function of the new protein MTOPVIB and showed that it shares structural similarities with the B subunit of Archaea TopoVI. Using different strategies, I also demonstrated that MTOPVIB is necessary to the SPO11-1/ SPO11-2 heterodimerization strongly suggesting that in A. thaliana, a catalytic TopoVI like complex is necessary for the formation of meiotic DSB. In addition to SPO11-1, SPO11-2, and MTOPVIB, four other proteins are necessary for the formation of meiotic DSB in A. thaliana : PRD1, PRD2, PRD3 and DFO. By yeast two hybrid approach, I analysed the interaction network between the "DSB" proteins. The results suggest that these proteins could act in a "super" complex which would be essential to the formation of DSBs.
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Impact of nuclear organization and chromatin structure on DNA repair and genome stability / Impact de l'organisation du noyau et de la structure de la chromatine sur la réparation de l'ADN et la stabilité du génomeBatté, Amandine 29 June 2016 (has links)
L’organisation non-aléatoire du noyau des cellules eucaryotes et la compaction de l’ADN en chromatine plus ou dense peuvent influencer de nombreuses fonctions liées au métabolisme de l’ADN, y compris la stabilité du génome. Les cassures double-brin sont les dommages à l’ADN les plus néfastes pour la cellule. Pour préserver l’intégrité de leur génome, les cellules eucaryotes ont développé des mécanismes de réparation des cassures double-brin qui sont conservés de la levure à l’homme. Parmi ceux-ci, la recombinaison homologue utilise une séquence homologue intacte présente ailleurs dans le génome et peut se diviser en deux sous voies de réparation. La conversion génique transfère l’information génétique d’une molécule à son homologue, tandis que le Break Induced Replication (BIR) établit une fourche de réplication qui peut procéder jusqu’à la fin du chromosome.Mon travail de thèse s’est attaché à caractériser la contribution du statut chromatinien et de l’organisation tridimensionnelle du génome à la réparation des cassures double-brin. L’organisation du noyau de la levure S. cerevisiae ainsi que la propagation de l’hétérochromatine au niveau des régions subtélomériques peuvent être modifiées via la surexpression des protéines Sir3 et sir3A2Q. Nous avons montré que le groupement des télomères accroit la conversion génique entre deux séquences subtélomériques, soulignant le rôle clé de la proximité spatiale et de la recherche d’homologie. Nous avons également constaté que la présence d’hétérochromatine au niveau du site de cassure limite la résection, ce qui permet une disparition plus lente des extrémités, qui resteraient disponibles plus longtemps pour réaliser la recherche d’homologie et achever la réparation. Enfin, nous avons observé que la présence d’hétérochromatine au site donneur diminue l’efficacité de recombinaison et qu’elle doit moduler une étape commune aux deux voies de réparation, à savoir l’invasion de brin. Ces travaux nous ont permis de décrire de nouvelles voies de régulation de la réparation de l’ADN. / The non-random organization of the eukaryotic cell nucleus and the folding of genome in chromatin more or less condensed can influence many functions related to DNA metabolism, including genome stability. Double-strand breaks (DSBs) are the most deleterious DNA damages for the cells. To preserve genome integrity, eukaryotic cells thus developed DSB repair mechanisms conserved from yeast to human, among which homologous recombination (HR) that uses an intact homologous sequence to repair a broken chromosome. HR can be separated in two sub-pathways: Gene Conversion (GC) transfers genetic information from one molecule to its homologous and Break Induced Replication (BIR) establishes a replication fork than can proceed until the chromosome end.My doctorate work was focused on the contribution of the chromatin context and 3D genome organization on DSB repair. In S. cerevisiae, nuclear organization and heterochromatin spreading at subtelomeres can be modified through the overexpression of the Sir3 or sir3A2Q mutant proteins. We demonstrated that reducing the physical distance between homologous sequences increased GC rates, reinforcing the notion that homology search is a limiting step for recombination. We also showed that heterochromatinization of DSB site fine-tunes DSB resection, limiting the loss of the DSB ends required to perform homology search and complete HR. Finally, we noticed that the presence of heterochromatin at the donor locus decreased both GC and BIR efficiencies, probably by affecting strand invasion. This work highlights new regulatory pathways of DNA repair.
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Spécialisation de Ku80c dans le couplage entre coupure et réparation de l’ADN lors des réarrangements programmés du génome chez Paramecium tetraurelia / Specialization of Ku80c in the coupling between DNA break and repair during programmed genome rearrangements in Paramecium tetraureliaAbello, Arthur 29 March 2019 (has links)
Au cours de son cycle sexuel, le cilié Paramecium tetraurelia procède à de massifs réarrangements programmés de son génome (RPG). Ils consistent, entre autres choses, en l’excision de 45 000 séquences précisément délimitées, appelées IES (Internal Eliminated Sequences). La transposase domestiquée Piggymac (Pgm) introduit les cassures double-brin (CDB) à l’extrémité des IES. La réparation très précise de ces dommages est réalisée par la voie de réparation des extrémités non-homologues (NHEJ). Un des acteurs de cette voie est l’hétérodimère Ku70/Ku80. Suite à des duplications globales du génome, la paramécie possède trois gènes KU80, Un seul de ces gènes est induit lors des RPG (KU80c) et une expérience d’ARN interférence (ARNi) contre KU80c montre une complète inhibition de l’introduction des CDB. De plus, des expériences de Co-IP en système hétérologue montrent que Ku70/Ku80c interagit avec Pgm. Ces résultats prouvent le rôle essentiel de Ku dans l’introduction des CDB lors des RPG et soulèvent la question du mécanisme impliqué. Au cours de ma thèse j’ai caractérisé le couplage entre Ku et Pgm en analysant des expériences d’immunofluorescence avec ou sans pré-extraction, permettant de déterminer les interdépendances de ces protéines pour leur localisation et pour leur stabilité nucléaire. Ces approches ont permis de démontrer que Pgm requiert la présence de Ku pour être stablement localisé dans les noyaux lors des RPG. Ku80c partage 74% de sa séquence protéique avec Ku80a. Des expériences de complémentations fonctionnelles surexprimant Ku80a lors des RPG ont montré que Ku80a n’est pas capable ni de se localiser stablement dans les noyaux ni de participer à la stabilisation nucléaire de Pgm. De plus, les RPG sont inhibés. Ces résultats montrent que Ku80c s’est spécialisé dans le couplage avec Pgm pour l’introduction des CDB lors des RPG. L’utilisation de protéines chimériques a permis de déterminer que la spécialisation de Ku80c est portée par son domaine N-terminal ∝-β. / During its sexual cycle, the ciliate Paramecium tetraurelia undergoes massive Programmed Genome Rearrangements (PGR). They consist, among others, in excision of 45,000 precisely delimited sequences, called IES (Internal Eliminated Sequences). A domesticated transposase, PiggyMac (Pgm), introduces double-strand DNA breaks (DSB) at IES ends. The Non Homologous End Joining pathway (NHEJ) handles highly precise repair of DSB. One of the actors of this pathway is the heterodimer Ku70/Ku80. In P. tetraurelia, the KU80 gene is present in three paralogous copies. Only KU80c is specifically expressed during PGR and RNA interferences against KU80c showed a complete inhibition of DNA cleavage. Furthermore, a Co-IP experiment in a heterologous system showed that both Ku70/Ku80c interact with Pgm. These results provide evidence that Ku is an essential partner of Pgm for DSB introduction; raising the question of the activating mechanism involved. During my PhD, I characterized the coupling between Ku and Pgm by analyzing immunofluorescence experiments, with or without pre-extraction, allowing the determination of inter-dependencies between those proteins for their nuclear localization and stability. Those methods demonstrated that Pgm requires the presence of Ku for a stable nuclear localization during the PGR. Ku80c shares 74% of the protein sequence with Ku80a. Functional complementation assays overexpressing Ku80a during the PGR showed that Ku80a is not capable to stably localize in nuclei nor to participate in Pgm nuclear stability. Furthermore, PGR are inhibited. Those results show that Ku80c has specialized for the DSB introduction during PGR. The use of chimeric proteins allowed to determine that Ku80c specialization was carried out by its N terminal domain.
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