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Analysis of the Nucleioprotein Complexes Essential for P1 Plasmid PartitionVecchiarelli, Anthony 01 September 2010 (has links)
For all organisms, segregation and proper intracellular localization of DNA are essential processes in ensuring faithful inheritance of genetic material. In prokaryotes, several different mechanisms have developed for efficiently moving chromosomal DNA to proper cellular locations prior to cell division, and the same holds true for bacterial plasmids. Low-copy-number plasmids and bacterial chromosomes encode active partition systems to ensure their inheritance within a bacterial cell population. One of the well-studied models of partition is that of the P1 plasmid in E. coli. The partition system encoded by the P1 plasmid is known as parABS - ParA is the partition ATPase, ParB is the partition site binding protein and parS is the partition site. The goal of this thesis was to investigate the nucleoprotein complexes essential in the P1 plasmid partition reaction. First, I examined how a single ParB dimer can bind its complicated arrangement of recognition motifs in parS to initiate the partition reaction. I then characterized a novel ParA interaction with the host nucleoid that is critical for proper P1 plasmid dynamics in vivo. Finally, I demonstrate how ParA can act as an adaptor between the nucleoid and the partition complex; effectively allowing the plasmid to use the nucleoid as a track for its intracellular movement and localization. My thesis work provides evidence towards a model that explains the P1 plasmid partition mechanism.
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Analysis of the Nucleioprotein Complexes Essential for P1 Plasmid PartitionVecchiarelli, Anthony 01 September 2010 (has links)
For all organisms, segregation and proper intracellular localization of DNA are essential processes in ensuring faithful inheritance of genetic material. In prokaryotes, several different mechanisms have developed for efficiently moving chromosomal DNA to proper cellular locations prior to cell division, and the same holds true for bacterial plasmids. Low-copy-number plasmids and bacterial chromosomes encode active partition systems to ensure their inheritance within a bacterial cell population. One of the well-studied models of partition is that of the P1 plasmid in E. coli. The partition system encoded by the P1 plasmid is known as parABS - ParA is the partition ATPase, ParB is the partition site binding protein and parS is the partition site. The goal of this thesis was to investigate the nucleoprotein complexes essential in the P1 plasmid partition reaction. First, I examined how a single ParB dimer can bind its complicated arrangement of recognition motifs in parS to initiate the partition reaction. I then characterized a novel ParA interaction with the host nucleoid that is critical for proper P1 plasmid dynamics in vivo. Finally, I demonstrate how ParA can act as an adaptor between the nucleoid and the partition complex; effectively allowing the plasmid to use the nucleoid as a track for its intracellular movement and localization. My thesis work provides evidence towards a model that explains the P1 plasmid partition mechanism.
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Mitotic Dynamics of Normally and Mis-attached Chromosomes and Post-mitotic Behavior of Missegregated ChromosomesHe, Bin 01 June 2015 (has links)
Equal segregation of the replicated genomic content to the two daughter cells is the major task of mitotic cells. The segregation is controlled by a complex system in the cell and relies mainly on the interaction between microtubules (MTs) of the mitotic spindle and kinetochores (KTs), specialized protein structures that assemble on each chromatid of each mitotic chromosome. By combining computational modeling and quantitative light microscopy, we established a quantitative model of the forces and regulators controlling metaphase chromosome movement in the mammalian cell line derived from Potorous tridactylis kidney epithelial cells (PtK1) (Chapter 2). This model can explain key features of metaphase chromosome dynamics and related chromosome structural changes experimentally observed. Moreover, the model made predictions, which we tested experimentally, on how changes in spindle dynamics affect certain aspects of chromosome structure. This quantitative model was next used to study the metaphase dynamics of chromosomes with erroneous KT-MT attachments (Chapter 3). Once again, the model predictions were tested experimentally and showed that erroneous KT-MT attachment alters the dynamics not only of the mis-attached KT, but also of its sister KT. Even more strikingly, experimental data showed that the presence of a single mis-attached KT could perturb the dynamics of all other, normally attached, KTs in anaphase. Chapter 3 also describe how MT poleward flux ensures correct KT-MT attachment and correct chromosome segregation. Indeed, reduced flux is associated with an increase in merotelically attached anaphase lagging chromosomes (LCs). These LCs form micronuclei (MNi) upon mitotic exit. The final effort of this work focused on the fate of MNi and micronuclated (MNed) cells (Chapter 4). Experimental observations showed that most of the chromosomes in MNi missegregated at the cell division following MN formation and that frequently the chromatin in the MN displayed delayed condensation. This work, thus, established a direct link between LCs and aneuploidy through the MN cell cycle. / Ph. D.
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Evidence for a Dynamic Adaptor Complex between the P1 Plasmid and Bacterial Nucleoid Promoted by ParA and ParB Partition ProteinsHavey, James C. 21 August 2012 (has links)
P1 prophage is stably maintained in E. coli as a low-copy-number plasmid. Stable maintenance of P1 is dependent on the function of the plasmid encoded partition system, parABS. ParA is the partition ATPase, ParB is the partition-site binding protein, and parS is the partition site. The concerted action of these proteins results in dynamic movement of the plasmid over the bacterial nucleoid, which results in its stable maintenance. Plasmid movement has been proposed to be caused by interactions between parS bound ParB and nucleoid bound
ParA. In this thesis, I have identified a complex of ParA, ParB, and DNA that is capable of promoting plasmid stability. ParA, ParB, DNA interactions required the ATP bound conformation of ParA. The ParA-ParB-DNA complex was dynamically regulated by nucleotide hydrolysis, which promoted complex disassembly. Complex formation resulted from the cooperative binding of ParA and ParB to DNA. ParA-ParB and ParB-DNA interactions were both necessary for complex formation. ParA-ParB-DNA complex size was regulated by ParB stimulation of ParA-ATP hydrolysis. Microscopy demonstrated that complexes resulted in the association of multiple DNA molecules due to protein binding. The properties of complex assembly, dynamics, and DNA grouping lead me to propose a model where associations between ParA bound to the bacterial nucleoid and the partition complex mediated plasmid movement and localization.
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Evidence for a Dynamic Adaptor Complex between the P1 Plasmid and Bacterial Nucleoid Promoted by ParA and ParB Partition ProteinsHavey, James C. 21 August 2012 (has links)
P1 prophage is stably maintained in E. coli as a low-copy-number plasmid. Stable maintenance of P1 is dependent on the function of the plasmid encoded partition system, parABS. ParA is the partition ATPase, ParB is the partition-site binding protein, and parS is the partition site. The concerted action of these proteins results in dynamic movement of the plasmid over the bacterial nucleoid, which results in its stable maintenance. Plasmid movement has been proposed to be caused by interactions between parS bound ParB and nucleoid bound
ParA. In this thesis, I have identified a complex of ParA, ParB, and DNA that is capable of promoting plasmid stability. ParA, ParB, DNA interactions required the ATP bound conformation of ParA. The ParA-ParB-DNA complex was dynamically regulated by nucleotide hydrolysis, which promoted complex disassembly. Complex formation resulted from the cooperative binding of ParA and ParB to DNA. ParA-ParB and ParB-DNA interactions were both necessary for complex formation. ParA-ParB-DNA complex size was regulated by ParB stimulation of ParA-ATP hydrolysis. Microscopy demonstrated that complexes resulted in the association of multiple DNA molecules due to protein binding. The properties of complex assembly, dynamics, and DNA grouping lead me to propose a model where associations between ParA bound to the bacterial nucleoid and the partition complex mediated plasmid movement and localization.
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Role of Poly-(ADP-ribose)-ylation signaling pathway in the chromatin remodeling after DNA damage / Étude de la voie de signalisation Poly-(ADP-ribose)-ylation dans les mécanismes de remodelage de la chromatine suite aux dommages à l'ADNSellou, Hafida 30 September 2016 (has links)
Chaque cellule humaine est constamment soumise à des agressions extérieures comme l'exposition aux rayons Ultra-Violets, agents chimiques, etc. ou endogènes provenant de la production de métabolites par la cellule elle-même. Ces agressions induisent des dommages dans l'ADN. Ces dommages, s'ils ne sont pas réparés correctement, peuvent induire un dérèglement des fonctions de base de la cellule qui peut alors devenir cancéreuse. Pour réparer leur ADN, les cellules activent divers mécanismes de réparation et établissent une signalisation au niveau des sites endommagés. Dans le noyau, l'ADN est associé à des protéines appelées histones pour former la chromatine. La chromatine se caractérise par différents niveaux d'organisation, aboutissant à la formation d'une structure très compacte. Cette compaction élevée de la chromatine peut représenter une barrière pour la machinerie de réparation. En effet, pour être réparé, l'ADN endommagé doit être accessible à la machinerie de réparation. Pour cela, les cellules ont développé des mécanismes permettant d'accéder à l'ADN endommagé. Ces mécanismes de réponse aux dommages à l'ADN impliquent l'activation de voies de signalisation. L'un des signaux précurseurs activés après dommage à l'ADN est la Poly-ADP-Ribosylation (PARylation). La PARylation est une modification post-traductionnelle composée d'une répétition de petites molécules appelées Poly-ADP-Riboses, qui s'accrochent notamment sur les histones pour signaler la présence de cassures dans l'ADN et permettent ainsi de recruter les protéines impliquées dans la réparation des dommages. Lorsque l'ADN est endommagé, l'activation de processus de réparation induit de manière précoce le recrutement de facteurs de remodelage de la chromatine. Le rôle exact de la signalisation via la PARylation durant les étapes précoces de la réponse aux dommages à l'ADN et plus particulièrement lors du remodelage de la chromatine reste encore mal caractérisé. Durant ma thèse, j'ai utilisé des techniques avancées en microscopie pour étudier la dynamique de la chromatine après induction de dommages à l'ADN. J'ai ainsi tenté d'élucider le rôle de la PARylation dans le mécanisme de remodelage de la chromatine au niveau des dommages dans l'ADN, en recherchant des facteurs permettant d'altérer de manière spécifique la dynamique de la chromatine. Cette méthodologie nous a permis d'identifier différents facteurs impliqués dans le remodelage de la chromatine après dommage à l'ADN. / In each human cell, many thousands of DNA lesions arise every day, challenging continuously the genome integrity. The majority of these lesions results from byproducts of normal cell metabolism or DNA replication, but they are also induced by exposure to radiations and genotoxic chemicals. The integrity of the genome is preserved by a plethora of different DNA damage signalling and repair machinery arranged by the cells. In the cell nucleus, DNA associates with scaffolding proteins to form the chromatin. The chromatin is tightly packed in the nucleus through several levels of organization. Such high-packing state poses a significant challenge for the repair machinery. Indeed, the damaged DNA needs to be accessible to repair proteins, and for that, cells have developed several mechanisms to allow the access to the damaged chromatin. The early steps of the DNA damage response involve the activation of proteins that are part of signalling pathways. One of the proteins activated upon DNA damage is PARP1, which synthetizes long and branched chains of ADP-ribose (poly-ADP-ribose or PAR) on itself and other chromatin factors, including histones. The activation of PARP1 leads to the recruitment of several effectors involved in DNA repair and chromatin remodeling. However the exact function of the PAR-signalling during early DNA damage response and in particular during chromatin remodeling at DNA breaks remains unclear. During my PhD, I used advanced fluorescent imaging tools to study in living cells the dynamics of chromatin in the nucleus at a local scale upon DNA damage. I used these tools to study PAR-dependent chromatin relaxation after DNA damage and to screen factors that selectively alter the dynamic behaviour of the damaged chromatin. This methodology allowed us to identify PAR-dependent factors involved in the local chromatin remodeling upon DNA damage.
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Models of chromosome architecture and connection with the regulation of genetic expression / Modèles de l'architecture du chromosome et lien avec la régulation de l'expression génétiqueLe Treut, Guillaume 29 November 2016 (has links)
Plusieurs indices suggèrent que le repliement du chromosome et la régulation de l’expression génétique sont étroitement liés. Par exemple, la co-expression d’un grand nombre de gènes est favorisée par leur rapprochement dans l’espace cellulaire. En outre, le repliement du chromosome permet de faire émerger des structures fonctionnelles. Celles-ci peuvent être des amas condensés et fibrillaires, interdisant l’accès à l’ADN, ou au contraire des configurations plus ouvertes de l’ADN avec quelques amas globulaires, comme c’est le cas avec les usines de transcription. Bien que dissemblables au premier abord, de telles structures sont rendues possibles par l’existence de protéines bivalentes, capable d’apparier des régions parfois très éloignées sur la séquence d’ADN. Le système physique ainsi constitué du chromosome et de protéines bivalentes peut être très complexe. C’est pourquoi les mécanismes régissant le repliement du chromosome sont restés majoritairement incompris.Nous avons étudié des modèles d’architecture du chromosome en utilisant le formalisme de la physique statistique. Notre point de départ est la représentation du chromosome sous la forme d’un polymère rigide, pouvant interagir avec une solution de protéines liantes. Les structures résultant de ces interactions ont été caractérisées à l’équilibre thermodynamique. De plus, nous avons utilisé des simulations de dynamique Brownienne en complément des méthodes théoriques, car elles permettent de prendre en considération une plus grande complexité dans les phénomènes biologiques étudiés.Les principaux aboutissements de cette thèse ont été : (i) de fournir un modèle pour l’existence des usines de transcriptions caractérisées in vivo à l’aide de microscopie par fluorescence ; (ii) de proposer une explication physique pour une conjecture portant sur un mécanisme de régulation de la transcription impliquant la formation de boucles d’ADN en tête d’épingle sous l’effet de la protéine H-NS, qui a été émise suite à l’observation de ces boucles au microscope à force atomique ; (iii) de proposer un modèle du chromosome qui reproduise les contacts mesurés à l’aide des techniques Hi-C. Les conséquences de ces mécanismes sur la régulation de la transcription ont été systématiquement discutées. / Increasing evidences suggest that chromosome folding and genetic expression are intimately connected. For example, the co-expression of a large number of genes can benefit from their spatial co-localization in the cellular space. Furthermore, functional structures can result from the particular folding of the chromosome. These can be rather compact bundle-like aggregates that prevent the access to DNA, or in contrast, open coil configurations with several (presumably) globular clusters like transcription factories. Such phenomena have in common to result from the binding of divalent proteins that can bridge regions sometimes far away on the DNA sequence. The physical system consisting of the chromosome interacting with divalent proteins can be very complex. As such, most of the mechanisms responsible for chromosome folding and for the formation of functional structures have remained elusive.Using methods from statistical physics, we investigated models of chromosome architecture. A common denominator of our approach has been to represent the chromosome as a polymer with bending rigidity and consider its interaction with a solution of DNA-binding proteins. Structures entailed by the binding of such proteins were then characterized at the thermodynamical equilibrium. Furthermore, we complemented theoretical results with Brownian dynamics simulations, allowing to reproduce more of the biological complexity.The main contributions of this thesis have been: (i) to provide a model for the existence of transcrip- tion factories characterized in vivo with fluorescence microscopy; (ii) to propose a physical basis for a conjectured regulatory mechanism of the transcription involving the formation of DNA hairpin loops by the H-NS protein as characterized with atomic-force microscopy experiments; (iii) to propose a physical model of the chromosome that reproduces contacts measured in chromosome conformation capture (CCC) experiments. Consequences on the regulation of transcription are discussed in each of these studies.
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