Mapping Topoisomerase IV Binding and Activity Sites on the E. coli genome / Distribution des sites de liaison et activité de la Topoisomérase IV sur le génome d’Escherichia coli

El Sayyed, Hafez

26 October 2016

Des liens de caténation sont progressivement crées lors de la réplication de l’ADN et sont responsables de la cohésion des chromatides sœurs. La topoisomérase IV est une topoisomérase de type II impliquée dans la résolution de ces liens de caténation accumulés derrière la fourche de réplication, et lors de la dernière étape de séparation des chromatides sœurs à la fin de la réplication. Nous avons étudié la liaison de la topoIV à l’ADN ainsi que son activité catalytique à l’aide de méthodes de biologie moléculaire et de génomique. Une expérience de ChIPseq a révélé que l’interaction de la topoIV de chez E.coli avec l’ADN est contrôlée par la réplication. Durant la réplication, la topoIV a accès à des centaines de sites sur l’ADN mais ne se lie qu’à quelques sites où elle exerce son activité catalytique. La conformation locale de la chromatine et l’expression des gènes influencent la sélection de certains sites. De plus, une forte liaison et une activité catalytique renforcée a été trouvée au site de résolution des dimers, dif. Le site dif est situé à l’opposé de l’origine de réplication dans le macrodomaine ter. Nous avons montré qu’il existe une interaction physique et fonctionnelle entre la topoIV et la recombinase XerCD, qui agit au site dif. Cette interaction est médiée par MatP, une protéine essentielle dans l’organisation du macrodomaine ter. L’ensemble de ces résultats montre que la topoIV, XerCD/dif et MatP œuvrent ensemble pour permettre l’étape finale de ségrégation des chromosomes lors du cycle cellulaire. / Catenation links between sister chromatids are formed progressively during DNA replication and are involved in the establishment of sister chromatid cohesion. Topo IV is a bacterial type II topoisomerase involved in the removal of catenation links both behind replication forks and after replication during the final separation of sister chromosomes. We have investigated the global DNA-binding and catalytic activity of Topo IV in E. coli using genomic and molecular biology approaches. ChIP-seq revealed that Topo IV interaction with the E. coli chromosome is controlled by DNA replication. During replication, Topo IV has access to most of the genome but only selects a few hundred specific sites for its activity. Local chromatin and gene expression context influence site selection. Moreover strong DNA-binding and catalytic activities are found at the chromosome dimer resolution site, dif, located opposite the origin of replication. We reveal a physical and functional interaction between Topo IV and the XerCD recombinases acting at the dif site. This interaction is modulated by MatP, a protein involved in the organization of the Ter macrodomain. These results show that Topo IV, XerCD/dif and MatP are part of a network dedicated to the final step of chromosome management during the cell cycle.

Topoisomérase IV

Cycle cellulaire

Topologie de l’ADN

Réplication de l’ADN

ChIP-Seq

Décaténation

Chromatides-sœurs

Topoisomerase IV

Cell cycle

DNA topology

DNA replication

ChIP-Seq

Decatenation

Sister chromatids

Clarifying the Role of the CST Complex in DNA Replication and Repair

Brandon Carter Wysong (11519407)

20 December 2021

<p>Ends of linear chromosomes are maintained by specialized structures known as telomeres. These structures are protected by a number of essential protein complexes including the shelterin complex and CST (CTC1 – STN1 – TEN1) complex. CST is an RPA-like ssDNA binding protein that is vital for telomere length maintenance <i>via</i> inhibition of telomerase and stimulation of DNA polymerase α -primase during C-strand fill-in synthesis. CST is also known to possess additional genome-wide roles in regulating DNA replication and repair including helping facilitate replication re-start at stalled forks, activating checkpoint signaling at double-strand breaks, and promoting replication origin firing. Proper and efficient repair of DNA is critical in order to protect the integrity of the genome and prevent extreme mutagenesis. Telomeres have a strong predisposition to oxidative DNA damage in the form of 8-oxoguanine caused by exposure to reactive oxygen species and free radicals. These oxidative lesions are repaired by the base-excision repair (BER) pathway. Previous work has implicated telomeric proteins such as the shelterin complex in mediating BER. Here we show for the first time that the CST complex and individual subunits robustly stimulate a myriad of proteins involved in the BER pathway including Pol β, APE1, FEN1, and LIGI. CST’s ability to augment these BER-associated proteins could be instrumental in promoting efficient DNA repair. Additionally, we find that CTC1 and STN1 are able to significantly enhance the polymerase activity of Pol δ and Pol α on both random-sequence and telomeric-sequence DNA substrates <i>in vitro</i>. What is more, we establish the ability of CST to resolve G4 structure and promote Pol δ synthesis, which we predict is a key feature of CST’s involvement in DNA replication at telomeres, which are known to form replication-inhibiting G4’s. Our results define important mechanistic insight into CST’s role in DNA replication and repair, and provide a strong foundation for future studies relating defective telomere maintenance to aging disorders and cancers which impact human health.</p>

Biochemistry

Cell Biology

Proteins and Peptides

CST Complex

DNA Replication

DNA Repair

Telomere Biology

Base Excision Repair

C-strand Fill-in

BER

Telomeres

CTC1

STN1

TEN1

Plasticité du programme spatio-temporel de réplication au cours du développement et de la différenciation cellulaire / Plasticity of human replication program during differentiation in relation with change in gene expression and chromatin reorganization

Julienne, Hanna

11 December 2013

Le séquençage du génome humain, il y a maintenant 12 ans, a mis en lumière la complexité des mécanismes des processus nucléaires tels que la transcription, la réplication ou l'organisation de la chromatine. Depuis, afin de mieux comprendre ces processus, un ensemble sans cesse croissant de données sur le noyau cellulaire a été produit et mis en ligne par un nombre important de laboratoires de par le monde. Ces données sont à la fois d'une richesse extraordinaire et d'une complexité embarrassante. Dans cette thèse, nous mettons à profit l'ensemble de ces données afin de mieux comprendre les déterminants nucléaires du programme spatio-temporel de réplication. Pour cela nous utilisons pas moins d'une centaine de profils épigénétiques ChiP-seq le long des chromosomes humains et dans diverses lignées cellulaires pour caractériser la structure primaire de la chromatine. Nous démontrons, à l'aide d'outils issus des statistiques multivariées, que l'immense complexité potentielle de ces jeux de données peut être réduite à quatre états chromatiniens principaux et ce dans toutes les lignées cellulaires somatiques étudiées. Cette classification simple, robuste et néanmoins complète est un excellent point d'appui pour l'étude de la réplication. Les quatre états principaux de chromatine sont répliqués à des moments distinct de la phase S (leur « timing » de réplication est différent) et ont un contenu en gènes drastiquement différents. Leur répartition spatiale le long du génome est structurée et est particulièrement visible dans les domaines où le « timing » de réplication dessine un U comme signature de l'existence d'un gradient de polarité des fourches de réplication. Ces U-domaines de la taille du Mpb recouvrent 50% du génome humain et les quatre états chromatiniens principaux se succèdent du bord au centre de ces U-domaines. Les mêmes techniques statistiques appliquées au cas d'une lignée embryonnaire révèlent aussi l'existence de quatre états principaux de chromatine mais de nature différente. La classification en quatre états s'avèrent alors très utile pour comparer l'épigénétique d'une lignée somatique à celle d'une lignée embryonnaire. Aussi, les spécificités du programme de réplication embryonnaire sont mises en rapport avec les spécificités de l'organisation de la chromatine dans cette lignée cellulaire. En particulier, notre étude révèle le rôle majeur de l'histone variant H2AZ dans la pluripotence. / The sequencing of the human genome, twelve years ago, revealed the complexity of the mechanisms underlying nuclear process such as transcription, replication and chromatin organization. In the past few years, to delineate better these processes, datasets on the cell nucleus were gathered and made available online by numerous laboratories around the world. These datasets are, at once, extraordinarily rich and daunting to handle. In this thesis, we take advantage of these datasets to understand better the nuclear determinants of the replication program. We analyze not less than a hundred ChiP-seq profiles along human chromosomes in several cell lines to characterize the primary structure of chromatin. We demonstrate, when using tools from multivariate statistics, that the immense potential complexity of these datasets can be reduced to four prevalent chromatin states in all studied somatic cell lines. This simple and comprehensive classification is an excellent starting point for the study of replication. The four prevalent chromatin states are replicated at different moments of the S-phase (they have a different replication “timing”) and have drasticaly different gene contents. Their spatial repartition along the genome is structured, especially in domains where the timing replication is U-shaped. These megabase sized U-domains cover 50% of the human genome and the four prevalent chromatin states succeed each other from their borders to their center. The same statistical techniques applied on an embryonic stem cell (ESC) also reduced the epigenetic complexity to four prevalent chromatin states which are qualitatively different from the ones in somatic cells. We further show that the specificities of embryonic replication program are link to the specificities of embryonic chromatin. Importantly, our study reveals that the histone variant H2AZ plays a major role in pluripotency.

Chromatine

Statistique multivariées

Réplication de l'ADN

Génome humain

Cellule souche embryonnaire

Différenciation

Epigénomique

Chromatin

Multivariate statistics

DNA replication

Human genome

Embryonic stem cell

Differentiation

Epigenomics

Die Kalkulation kalkulierbarer Mutationen

Drechsel, Dieter

09 August 2012

Bei der Replikation monotoner DNA - Sequenzen tritt theoretisch ein Vorgang auf, den wir als „Basenkonkurrenz“ bezeichnen: Da sich an jeder Replikations-Stelle mehrere Basenbausteine bewerben, aber immer nur einer benötigt wird, bewerben sich die übrig gebliebenen Bausteine an den jeweils nächsten Replikations - Positionen und erlangen wegen der fortwährenden Beschleunigung durch elektrostatische Anziehung immer größere kinetische Energien. Das führt dazu, dass an einer bestimmten Stelle der replizierenden monotonen Sequenz der eine Partner der Wasserstoffbrückenbindung ein hohes Energieniveau erreicht. Es wird berechnet, dass sich dadurch kurzzeitig eine sehr hohe Bindungsenergie zwischen den beiden Partnern der Wasserstoffbrückenbindung einstellt, wodurch der in dieser kurzen Zeitspanne wirkende DNA-Reparaturmechanismus unterdrückt wird. Die Auswirkungen der hohen Basenkonkurrenz – Energien werden berechnet (hohe Bindungsenergien der Wasserstoffbrückenbindungen, Tunnelvorgänge, irreparable Mutationen). Die Folgen dieser Erscheinung sind Tumorbildung, Alterung, Veränderung der DNA – Struktur, Beeinflussung der Evolution, worauf im Einzelnen eingegangen wird. Es zeigt sich, dass die negativen Auswirkungen der Basenkonkurrenz vorwiegend bei zu niedriger Viskosität des Zellplasmas auftreten.

info:eu-repo/classification/ddc/540

ddc:540

Maintenance of Constitutive and Inactive X Heterochromatin in Cancer and a Link to BRCA1: A Dissertation

Pageau, Gayle Jeannette

13 June 2007

The development of cancer is a multi-step process which involves a series of events, including activation of oncogenes and loss of tumor suppressor function, leading to cell immortalization and misregulated proliferation. In the last few years, the importance of epigenetic defects in cancer development has become increasingly recognized. While most epigenetic studies focus on silencing of tumor suppressors, this thesis addresses defects in the maintenance of silenced heterochromatin in cancer, particularly breast cancer. Breast cancer is a leading cause of cancer in women and many familial cases have been linked to mutations in the breast cancer susceptibility genes, BRCA1 and BRCA2. BRCA1 has been linked to DNA repair as well as multiple other cellular processes, including cell cycle checkpoints, ubiquitination, centrosome function, and meiotic silencing of the XY body. This work began with a particular interest in the report that BRCA1 was linked to the failed maintenance of random X-inactivation in female somatic cells, via a role in supporting XIST RNA localization to the inactive X chromosome (Xi). XIST RNA is a non-coding RNA that fully coats or “paints” the Xi and induces its silencing. Work presented in Chapter II substantially clarifies the relationship of BRCA1 to XIST RNA, based on several lines of experimentation. Loss of BRCA1 does not lead to loss of XIST RNA in these studies, nor did reconstitution of HCC1937 BRCA1-/- tumor cells with BRCA1 lead to XIST RNA localization on Xi, although an effect on XIST RNA transcription is possible. Studies of BRCA1 localization with Xi showed that BRCA1 has a limited association with the Xi in ~3-10% of cells, it rarely colocalizes with XIST RNA to a significant extent, but rather is in close apposition to a small part of the XIST RNA/Xi territory. Additionally, analysis of several breast cancer cell lines revealed mislocalization of XIST RNA in some breast cancer cell lines. Many studies have examined BRCA1 foci that form following DNA damage and demonstrated that these are sites of repair. However, whether the numerous large foci consistently present in normal S-phase nuclei were storage sites or had any function was unknown. In Chapter III, I demonstrate that the BRCA1 foci in normal S-phase nuclei associate overwhelmingly with specific heterochromatic regions of the genome. More specifically, BRCA1 foci often associate with centromeric or pericentromeric regions in both human and mouse cells. In human cells BRCA1 foci often appear juxtaposed to centromeric signal, whereas in mouse, BRCA1 often rings or paints the large chromocenters, clusters of DAPI-dense pericentric and centric heterochromatin. Using PCNA and BrdU as markers of replication, I demonstrate that BRCA1 preferentially associates with the chromocenters during their replication, although high-resolution analysis indicates that BRCA1 and PCNA foci rarely directly overlap. Interestingly, cells with defects in BRCA1 were found to have lagging chromosomes and DNA bridges which nearly always contained satellite DNA, which is consistent with the possibility that BRCA1 deficit contributes to failed separation of sister chromatids at the centromere. This is consistent with other recent reports that BRCA1 is necessary for DNA decatenation by topoisomerase II during routine replication and with my demonstration that topoisomerase II also accumulates on pericentric heterochromatin (PCH) during replication. Chapter IV presents recent work which reveals that RNA is commonly expressed from the centric/pericentric heterochromatin and appears to be linked to its replication. In mouse cells RNA from heterochromatic sequences is readily detected using a broad molecular cytological assay for repeat transcription (the COT-1 RNA assay). In addition to a more dispersed nucleoplasmic signal from euchromatic nuclear regions, distinct localized foci of repeat RNA are detected with COT1 probe or pancentromeric probe. Further analysis with the minor satellite (centromere proper) and the major satellite (comprising the larger pericentric heterochromatin) reveals that the large RNA foci often contain these satellite sequences, long thought to be essentially silent. These foci generally associate with the PCH of chromocenters, and produce various patterns similar to BRCA1- including a larger signal partially painting or ringing the chromocenter in a fraction of cells. In conjunction again with PCNA staining, it was possible to determine that the major satellite RNAs associate with the chromocenters during replication. While the satellite RNA co-localizes precisely with PCNA, neither of these co-localizes at high resolution with BRCA1, although they all are present on replicating chromocenters contemporaneously. These findings show that satellite RNAs are more widely expressed in normal cells than previously thought and link their expression to replication of centromere-linked heterochromatin. Finally, Chapter V presents three lines of recent results to support a major concept forwarded in this manuscript: that loss of Xi heterochromatin may reflect defects in the broader heterochromatic compartment, which may be manifest at multiple levels. I provide evidence using two new assays that both the peripheral heterochromatic compartment and the expression and silencing of satellite repeats is commonly compromised in cancer, although this appears to vary among cancer lines or types. The final results connect back to the question with which I began: what maintains XIST RNA localization to the chromosome in normal cells. These results demonstrate for the first time that Aurora B Kinase activity, mediated by Protein Phosphatase 1 (PP1) during interphase, controls the interphase retention and mitotic release of XIST RNA from the chromosome, likely linked to chromatin modifications such as H3Ser10 phosphorylation. As Aurora B Kinase is commonly over-expressed in cancer and is linked to chromatin changes, this exemplifies one type of mechanism whereby broad epigenetic changes in cancer may impact XIST RNA localization and the maintenance of heterochromatin more generally. This thesis represents a melding of cancer biology with the study of X inactivation and heterochromatin, with findings of fundamental interest to both of these fields.

BRCA1 Protein

Chromosomes, Human, X

Heterochromatin

RNA, Untranslated

Centromere

DNA Replication

Protein-Serine-Threonine Kinases

Academic Dissertations

Dissertations, UMMS

Life Sciences

Medicine and Health Sciences

Compartimentation du cycle viral du bactériophage SPP1 dans le cytoplasme de la bactérie Gram-positive Bacillus subtilis. / Compartmentalization of bacteriophage SPP1 replication and assembly in the Gram-positive bacterium Bacillus subtilis.

Labarde, Audrey

20 June 2019

Les virus bactériens (bactériophages), durant leur co-évolution avec les bactéries, ont su trouver de nombreuses voies pour détourner les machineries cellulaires dans le but de se multiplier efficacement. L’infection par le phage dès son entrée dans le cytoplasme est un bouleversement pour la bactérie en termes de ressources monopolisées à ses dépens et probablement de restructuration de l’espace cytoplasmique. Dans ce travail de thèse, l’impact de l’infection de la bactérie Gram-positive Bacillus subtilis par le bactériophage SPP1 a été étudié.La réplication de l’ADN est initiée par des protéines précoces virales. Elle mène au chargement de l’hélicase virale gp40 sur l’origine de réplication de SPP1 dont les brins d’ADN ont été ouverts par la protéine de liaison à l’origine, gp38. Le réplisome bactérien est ensuite recruté de manière massive au sein de l’usine de réplication formant un foyer défini dans le cytoplasme bactérien. L’interaction de gp40 avec les protéines cellulaires DnaX et DnaG assure fort probablement le recrutement du complexe cellulaire au foyer de réplication. La quantité d’ADN viral synthétisée représente presque 500 copies d’ADN viral par bactérie après 30 minutes d’infection, ce qui est équivalent à la taille de 5 génomes de B. subtilis. Des études de FRAP (Fluorescence Recovery After Photobleaching) montrent que l’usine de réplication est très dynamique. Ce comportement est inhibé par la présence de HPUra montrant qu’il dépend de la présence d’un réplisome actif.Les concatémères résultant de la réplication de l’ADN viral sont le substrat pour l’encapsidation du génome de SPP1 dans des procapsides préformées. La maturation de ces procapsides en particules virales infectieuses suit une voie d’assemblage spécifique. Deux protéines rapportrices de différentes étapes de cette voie ont été suivies : la protéine d’échafaudage gp11, présente à l’intérieur de la procapside avant encapsidation de l’ADN, et la protéine auxiliaire gp12, qui se fixe à la surface de la capside pendant l’encapsidation. Les procapsides colocalisent partiellement avec l’usine de réplication du génome viral. Après encapsidation de l’ADN, les capsides vont s’accumuler dans des foyers de stockage qui ont une localisation indépendante du foyer de réplication. Cette organisation est également observée dans des bactéries très allongées où deux régions de stockage sont retrouvées situées de part et d’autre de l’usine de réplication mais éloignées des pôles cellulaires. La microscopie électronique combinée à des immuno-marquages révèlent que cette compartimentation corrèle avec une réorganisation majeure de l’ultrastructure du cytoplasme bactérien.L’assemblage et la dynamique des foyers viraux dans la bactérie ont été suivis pendant toute la durée du cycle viral dans un système de microfluidique. Elle montre que les étapes de réplication de l’ADN viral et la formation de la particule du phage sont des processus compartimentés dans le cytoplasme de la bactérie tant spatialement que temporellement. Bien que la croissance cellulaire soit retardée, les bactéries continuent de s’allonger et de se diviser pendant l’infection par SPP1. Le virus exploite donc de manière efficace les machineries cellulaires et l’architecture de la bactérie pour une multiplication optimale. Ces stratégies sont probablement utilisées par de nombreux phages pour remodeler la cellule bactérienne à leur avantage. / During the co-evolution of viruses and cells, viruses exploited numerous ways to hijack cell machineries for their optimal multiplication and dissemination. Phage infection is a major challenge to bacteria, exploiting extensively cellular biosynthetic ressources and possibly re-organizing the cytoplasm space. The work in this thesis investigated the cellular impact of infection by SPP1, a well-characterized model tailed bacteriophage that infects the Gram-positive bacterium Bacillus subtilis.Viral DNA replication is initiated by early phage proteins whose activity culminates in loading of the SPP1 helicase gp40 at the melted phage origin of replication. The bacterial replisome is then massively recruited to the phage replication factory that is localized at a defined position of the cytoplasm. The interaction of gp40 with its two cellular partners DnaX and DnaG mediates most likely the hijacking of the B. subtilis replication machinery. More than 500 copies of the viral genome are synthesized within 30 minutes after initiation of infection, which is roughly the equivalent to five B. subtilis genomes. FRAP (Fluorescence Recovery After Photobleaching) experiments showed that the viral DNA factory is highly dynamic, a behavior that depends on active DNA replication.The concatemers resulting from DNA replication are the substrate for encapsidation of the SPP1 genome into preformed procapsids. Maturation of procapsids to infectious viral particles follows a defined pathway. The SPP1 scaffolding protein gp11, that occupies the interior of the procapsid before DNA packaging, and gp12, that binds to capsids during DNA packaging, were followed to dissect the steps of this process. Procapsids partially co-localize with DNA replication factories. After packaging the DNA-filled capsids fully segregate to spatially distinct warehouses where viral particles accumulate. Recruitment of SPP1 proteins to these compartments recapitulates the sequential order of their assembly to build the viral particle. The replication factory is most frequently flanked by two warehouses. Such pattern is also observed in very elongated cells where the viral compartments remain localized nearby each others and far from the bacterial poles. Immuno-electron microscopy of cryo-sections from infected cells highlights a complete remodelling of the bacterial cytoplasm dedicated to virus multiplication.The assembly and dynamics of the SPP1 replication factory and virions warehouses were visualized during the complete phage infection cycle in microfluidics experiments. The viral compartments are well individualized in the cytoplasm both in terms of space and time. Although bacterial growth is retarded, cells continue to elongate and to divide during SPP1 infection. Structuration of viral factories appears as a very efficient way for SPP1 to exploit bacterial resources and cytoplasmic space to optimize its multiplication. This strategy might be widely used by phages for remodelling the bacterial cell.

Usines virales

Compartimentation du cycle viral

Réplication de l’ADN

Assemblage de la particule virale

Dynamique

Vidéo-Microscopie

Viral factories

Compartmentalization

DNA replication

Particle assembly

Dynamics

Video-Microscopy

Dynamique cellulaire des protéines de la réplication chez l'archée halophile Haloferax volcanii / Cellular dynamics of the DNA replication proteins in the halophilic archaeon Haloferax volcanii

Delpech, Floriane

17 November 2016

Ce travail de thèse porte sur l’étude de la réplication chez les archées, qui constituent le troisième domaine du vivant avec les bactéries et les eucaryotes. L’organisme modèle que nous avons utilisé est l'archée halophile Haloferax volcanii car les outils génétiques disponibles permettent d’exprimer des protéines fusionnées à la Protéine Fluorescente Verte (GFP) dans cet organisme mésophile et aérobe et ainsi de localiser les protéines d’intérêt dans des cellules vivantes. Nous nous sommes ainsi intéressés à la localisation cellulaire de quatre protéines de la réplication qui ont été fusionnées à la GFP et exprimées sous contrôle de leur propre promoteur : (i) la protéine ‘Flap Endonuclease 1’ (FEN1), qui intervient dans la maturation des fragments d’Okazaki, (ii) la protéine ‘Origin Recognition Complex’ (ORC1) impliquée dans la reconnaissance des origines de réplication, (iii) la protéine ‘Proliferating Cellular Nuclear Antigen’ (PCNA), anneau de processivité des ADN polymérases réplicatives, et (iv) la protéine de fixation à l’ADN simple-brin ‘Replication Protein A’ (RPA2) essentielle à la réplication chez H. volcanii. Seule la protéine PCNA n’a pu être exprimée en fusion avec la GFP, suggérant que la protéine fusion n’est pas fonctionnelle. GFP::Orc1 et GFP::Fen1 ont été exprimées dans la cellule mais ne présentent pas de localisation spécifique reflétant un rôle de ces protéines dans la réplication de l’ADN. En revanche des foyers de fluorescence de la protéine fusion GFP::Rpa2 ont été observés, dont le nombre augmente significativement dans des cellules exposées à l’aphidicoline, drogue inhibant la synthèse de l’ADN et induisant ainsi un stress réplicatif. Cependant une localisation différente de la protéine GFP::Rpa2 a été observée lorsque les cellules sont exposés à la phléomycine, qui induit notamment des cassures double-brin de l‘ADN. Dans ces cellules, GFP::Rpa2 forme un foyer de fluorescence massif qui colocalise avec l’ADN compacté dans la grande majorité des cellules observées. Nos résultats suggèrent donc que la localisation spécifique observée pour GFP::Rpa2 reflète son rôle dans la réparation de l’ADN et/ou le redémarrage des fourche de réplication arrêtées. / The aim of this thesis project was to improve our understanding of DNA replication in archaea, the third domain of life with bacteria and eukarya. The model organism chosen for these studies is the halophilic archaea Haloferax volcanii, a mesophilic aerobe for which genetics tools allow studying in living cells the localization of proteins fused to the Green Fluorescent protein (GFP). Four proteins involved in DNA replication were fused to the GFP and expressed under the control of their own promoter: (i) the ‘Flap Endonuclease 1’ (FEN1), involved in Okazaki fragments maturation, (ii) the ‘Origin Recognition Complex’ (ORC1), involved in DNA replication origin recognition, (iii) the ‘Proliferating Cellular Nuclear Antigen’ (PCNA), processivity factor of replicative DNA polymerases, and (iv) the ‘Replication Protein A’ (RPA2), single-stranded DNA binding protein essential for DNA replication in H. volcanii. Only the PCNA fusion to the GFP was not successful, suggesting that the GFP hinders essential roles of PCNA in DNA replication. Fen1 and Orc1 were successfully fused to the GFP and expressed in living cells, but specific localization in cells related to growth phase, reflecting different replication dynamics, were not observed. In contrast, we could observed fluorescent foci formed by the fully functional GFP::Rpa2 protein that actively responded to DNA damage in H. volcanii cells. The number of these fluorescent foci per cell was constant during cell growth but it significantly increased in cells exposed to aphidicoline, which inhibits DNA synthesis during replication. When cells were treated with phleomycine, a DNA damaging agent mainly causing double-strand breaks, formation of a massive fluorescent focus coinciding with DNA compaction was observed. Our results suggest that the specific cellular localization of GFP::Rpa2 observed reflects Rpa2 roles in DNA repair and/or DNA replication fork restart.

Réplication de l'ADN

Archées

Haloferax volcanii

Microscopie de fluorescence

GFP ( green fluorescent protein)

DNA replication

Archaea

Haloferax volcanii

Fluorescence microscopy

GFP ( green fluorescent protein)

Genetic Study of Checkpoint Defects of the Mus81-1 Mutant in the Fission Yeast Schizosaccharomyces Pombe.

Abrefa, Darlington Osei

January 2019

No description available.

Molecular Biology

Genetics

Microbiology

DNA replication checkpoint

DNA damage checkpoint

Mus81

DNA repair

genetic mutation

cell cycle

phosphorylation

Mrc1

Cds1

Chk1

Fission yeast mutant

MMS

UV

HU

BLM

Molecular Processing of Replication Intermediates in Escherichia Coli after DNA Damage

Belle, Jerilyn Jalana

05 May 2007

Accurate replication of the genome is essential for reproduction in all cells. However, even under normal conditions, the replication machinery may face a variety of impediments that can prevent it from completing its task. The mechanism by which cells overcome these hurdles is likely to vary depending upon the nature of the obstacle. Both UV irradiation and inactivation of replicative proteins in DnaB can inhibit the progression of the DNA replication machinery. However, the mechanism by which replication recovers following UV irradiation is different from the mechanism of recovery following the inactivation of the replicative proteins. Previous results show that following UVinduced damage in Escherichia coli, the replication fork is maintained and protected from extensive degradation by RecF, RecO, and RecR until replication can resume. By contrast, replication does not recover following inactivation of the replication protein DnaB, and the nascent DNA is extensively degraded irrespective of whether RecF is present. In this study, we verified DNA replication arrest by monitoring the total DNA accumulation and rate of DNA synthesis following UV-induced DNA damage and inactivation of thermosensitive replication alleles, such as dnaB266. We measured the amount of nascent DNA degradation, allowing us to determine how the newly synthesized strand of DNA is affected following replication fork arrest. Our data indicate that following inactivation of DnaB266, the replication fork is not maintained and is subject to extensive degradation. The degradation that occurs after DnaB266 inactivation is partially reduced in the absence of RecF-O-R, RecJ, and ExoI, suggesting that DNA processing by these enzymes occurs after DnaB arrest. In addition, two-dimensional agarose gel analysis revealed that unique structural intermediates accumulated following inactivation of DnaB266. These observations indicate that the recovery of replication when impeded by DNA lesions, such as those produced by UVirradiation, is maintained and processed through mechanisms that do not resemble the events occurring when replication proteins are inactivated.

dnaB

temperature sensitivity

dnaE

DNA replication--Effect of radiation on.

DNA damage.

DNA repair.

Microbial enzymes.

Mechanistic studies of enzymes involved in DNA transactions

Stephenson, Anthony Aaron

07 November 2018

No description available.

Cellular Biology

Biophysics

Biology

Biochemistry

DNA replication

DNA repair

DNA polymerase lambda

BRCT

Gene editing

CRISPR-Cas9

enzymology

enzyme kinetics

pre-steady state kinetics

conformational dynamics