Global ETD Search

271	Activation of a novel ERK5-NF-kappaB pathway is required for G2/M progression in the cell cycle / Cude, Kelly J. January 2004 (has links) Thesis (Ph. D.)--University of Washington, 2004. / Vita. Includes bibliographical references (leaves 106-122).
272	Understanding the mechanisms underlying force transmission during epithelial cell division / Analyse des mécanismes moléculaires de transmission des forces mécaniques lors la division cellulaire Pinheiro, Diana 19 September 2016 (has links) Au sein d'un tissu épithélial la division cellulaire doit être couplée à la formation de nouvelles jonctions intercellulaires entre les futures cellules-filles, afin de préserver l'intégrité du tissu et maintenir son adhésion et polarité. Chez les vertébrés et les invertébrés, lors de la constriction de l'anneau contractile les jonctions assemblées entre la cellule en division et ses voisines est remodelé. Concomitamment, la myosine non-musculaire II (MyoII) s'accumule dans les cellules voisines y produit la force nécessaire pour juxtaposer les membranes de la cellule en division, définissant ainsi la longueur de la future jonction formée entre les cellules-filles. Dans le cadre de mes travaux de doctorat, j'ai cherché à comprendre les mécanismes moléculaires sous-jacents au dialogue entre les cellules épithéliales pendant la division. J'ai montré que chaque division cellulaire est associée à un processus de mécano-transduction qui contrôle la dynamique de la MyoII dans les cellules voisines. Les forces produites par l'anneau contractile allongent localement la membrane des voisines diluant ainsi la concentration d'E-Cadhérine (E-Cad). En retour, cette réduction locale d'E-Cad, couplée à la contractilité intrinsèque des cellules voisines, génère des flux auto-organisés d'actine et myosine, qui conduisent à l'accumulation de MyoII dans les cellules voisines. En montrant que la cytocinèse épithéliale est une source endogène de contraintes mécaniques, mon travail définit un nouveau mécanisme de mécano-transduction qui coordonne les dynamiques d'actine et myosine dans les cellules en division et leurs voisines, et qui est permet de plus le remodelage des jonctions adhérentes. / During epithelial cytokinesis, the remodelling of adhesive cell-cell contacts between the dividing cell and its neighbours has profound roles in the integrity, the arrangement and morphogenesis of proliferative tissues. In both vertebrates and invertebrates, this remodelling requires the activity of non-muscle Myosin II (MyoII) in the interphasic cells neighbouring the dividing cells. However, the mechanisms coordinating cytokinesis and MyoII activity in the neighbours are unknown. Here, we found that, in the Drosophila notum epithelium, each cell division is associated with a mechano-sensing and transmission event controlling MyoII dynamics in the neighbours. We established that the ring pulling forces promote local junction elongation, resulting in a decrease of E-Cadherin (E-Cad) concentration at the ingressing adherens junction (AJ). In turn, the local reduction of E-Cad concentration and the contractility of the neighbouring cells promote self-organized actomyosin flows, ultimately leading to MyoII accumulation at the base of the ingressing AJ. While mechano-sensing has been extensively studied in the context of AJ reinforcement to stabilize the adhesive cell-cell contacts, we propose an alternative mechano-sensing mechanism able to coordinate actomyosin dynamics between epithelial cells and to sustain AJ remodelling in response to mechanical forces. Division cellulaire Jonctions adhérentes Miosine non-musculaire II Flux d'actine et miosine Mécano-transduction Cell division Adheren junctions Actomyosin flows 571.6
273	Mechanism of APC/C activation and substrate specificity in mitosis Zhang, Suyang January 2018 (has links) In eukaryotes, cell proliferation and cell cycle transitions are strictly controlled by the anaphase-promoting complex/cyclosome (APC/C). The APC/C is an E3 ubiquitin ligase that regulates chromatid segregation at the metaphase to anaphase transition, exit from mitosis and the establishment and maintenance of G1. The APC/C’s catalytic activity and substrate specificity are controlled by its interactions with two coactivators, Cdc20 and Cdh1. In contrast to Cdh1, APC/C activation by Cdc20 during mitosis requires hyper-phosphorylation of APC/C subunits by cyclin-dependent kinase (Cdk) and polo kinase. The aim of the first part of this thesis was to understand how mitotic phosphorylation regulates APC/C activity. Using cryo-electron microscopy and biochemical analysis, we found that an auto-inhibitory segment of the Apc1 subunit acts as a molecular switch that in apo unphosphorylated APC/C interacts with a coactivator-binding site (C-box binding site), thereby obstructing engagement of Cdc20. Phosphorylation of the auto-inhibitory segment displaces it from the C-box binding site to relieve APC/C auto-inhibition. Efficient phosphorylation of the auto-inhibitory segment requires the recruitment of the kinase Cdk-cyclin-Cks to a hyper-phosphorylated loop of Apc3. In addition to regulation of APC/C activity by phosphorylation, ordered cell progression is ensured by the ability of the APC/C to target substrate degradation in a defined order. At mitosis onset, degradation of securin and cyclin B1 is inhibited by the spindle assembly checkpoint, exerted by the mitotic checkpoint complex (MCC), whereas both cyclin A2 and Nek2A are not subject to MCC inhibition. The aim of the second part of the thesis was to elucidate the mechanism of how the APC/C achieves its substrate specificity. Our biochemical analysis showed that the resistance of cyclin A2 to MCC inhibition is due to its ABBA motif and the Cdk-associated Cks2 subunit. Furthermore, we found that it is the Cdc20 molecule of the MCC that binds to the ABBA motif to allow for cyclin A2 ubiquitination. Strikingly, mutating all three known degrons (KEN box, D box and ABBA motif) of cyclin A did not affect its ubiquitination by APC/CCdc20. Deletion of a potential novel degron found within residues 60-80 of cyclin A2 impaired cyclin A2 ubiquitination.
274	Caracterização da interação entre o regulador espacial MinC e seu alvo FtsZ em Bacillus subtilis / Characterization of interaction between the spatial regulator for bacterial division MinC and its target FtsZ in Bacillus subtilis Valdir Blasios Junior 14 August 2014 (has links) A divisão celular bacteriana é orquestrada por FtsZ, uma proteína homóloga à tubulina eucariótica que possui a capacidade de polimerizar e gerar uma estrutura chamada de anel Z. O local onde esta estrutura citoesquelética contrátil é formada determina o futuro sítio de divisão. O complexo MinCD é um dos principais reguladores da posição da divisão, favorecendo a montagem do anel Z precisamente na região medial da bactéria. MinCD age como um inibidor sítio específico da polimerização de FtsZ, atuando preferencialmente nos polos celulares. MinC é a proteína do complexo que atua diretamente sobre FtsZ e inibe sua polimerização. Essa tese elucida a interação entre FtsZ e MinC e sugere o mecanismo exercido por MinC em Bacillus subtilis. Foi triada uma biblioteca de mutantes randômicos de FtsZ para identificação de mutantes resistentes à ação de MinC. Dentre estes, as substituições K243R e D287V, quando caracterizados usando espalhamento de luz e espectroscopia de fluorescência impediram a interação com MinC. Como as mutações estavam localizados em torno das hélices H-9 e H-10 no domínio C-terminal de FtsZ, concluímos que esta região representa o sítio de interação com MinC desta proteína. Como complemento ao mapeamento do sitio de ligação de MinC em FtsZ, identificamos a região de MinC que interage com FtsZ. Para tanto, escolhemos resíduos de MinC para mutagênese e caracterização. A escolha priorizou os resíduos conservados entre espécies Gram-positivas, experimentos de RMN, carga e exposição ao solvente dos mesmos. Dentre os resíduos de MinC mutados que afetaram sua capacidade de inibir a polimerização de FtsZ in vitro foram: Y8 e K12 (β-1), K15 (alça-2), H55 (β-3) , H84 (β-4) e K149 (C-terminal). Sendo assim, podemos concluir que a face de interação para FtsZ em MinC de B. subtilis é a única folha β do domínio N-terminal desta proteína. Com base nos sítios mapeados das duas proteínas experimentalmente, criamos um modelo in silico do complexo MinC-FtsZ por docking molecular. De acordo com o modelo gerado, MinC interage com a porção lateral de polímeros de FtsZ. Isto sugere que MinC atue na inibição da formação de feixes de filamentos de FtsZ, impedindo assim a formação de anéis Z funcionais. Esse mecanismo de ação do sistema Min é diferente do proposto para E. coli, no qual MinC interage com a face de polimerização FtsZ-FtsZ e impede a formação de protofilamentos de FtsZ. / Bacterial cell division is orchestrated by FtsZ, a protein homologous to eukaryotic tubulin that has the ability to polymerize and generate a cytoplasmic structure called the Z ring. The subcellular location where this cytoskeletal structure is formed determines the future division site. The MinCD complex is one of the main regulators of the position of cell division, driving the assembly of Z-ring precisely at the medial region of the cell. MinCD acts as a site-specific inhibitor of FtsZ polymerization, blocking Z ring formation at the cell poles. MinC is the protein of the complex that acts directly on FtsZ and inhibits its polymerization. This thesis elucidates the interaction between FtsZ and MinC and suggests the MinC mechanism in Bacillus subtilis. An ftsZ randomly mutagenized library was screened to identify mutants that are resistant to MinC action. Using right-angle light scattering and fluorescence spectroscopy we showed that substitutions K243R and D287V lost the interaction to MinC. These substituted residues clustered around the H-9 and H-10 helices in the C-terminal domain of FtsZ, thus, we conclude that this region is the binding site for MinC. In addition to mapping the MinC binding site on FtsZ, we also identified the FtsZ binding site in MinC. Based on residue conservation, NMR experiments and exposure to solvent, we chose residues of MinC for mutagenesis and characterization. The substituted residues that di srupted MinC ability to inhibit FtsZ polymerization in vitro were: Y8 and K12 (β-1), K15 (turn-2) , H55 (β-3), H84 (β-4) and K149 (C-terminal). Thus, we conclude that the binding site of MinC for FtsZ is located on the β only sheet at the N-terminal domain of MinC from B. subtilis. Finally, based on the binding sites of the two proteins mapped experimentally, we created a model of the complex between MinC and FtsZ by molecular docking. According to the generated model, MinC interacts with the lateral portion of FtsZ polymers. This indicates that MinC should inhibit assembly of higher order FtsZ polymers, thereby preventing the formation of a functional Z-ring. This mechanism of Min is different from that proposed in E. coli, in which MinC interacts with FtsZ polymerization interface and inhibits FtsZ protofilament formation. Anel Z Citoesqueleto Divisão celular FtsZ Interação proteína-proteína MinC Cell division Cytoskeleton FtsZ MinC Protein-protein interaction Z-ring
275	Efeito antimitótico de um derivado de pirimidinona no desenvolvimento embrionário de ouriços-do-mar Oliveira, Dalliane Macedo Lopes de 28 May 2015 (has links) Submitted by Vasti Diniz (vastijpa@hotmail.com) on 2017-09-08T12:30:20Z No. of bitstreams: 1 arquivototal.pdf: 3898148 bytes, checksum: 4bd5b276470027c8968ec023cab6d4fd (MD5) / Made available in DSpace on 2017-09-08T12:30:20Z (GMT). No. of bitstreams: 1 arquivototal.pdf: 3898148 bytes, checksum: 4bd5b276470027c8968ec023cab6d4fd (MD5) Previous issue date: 2015-05-28 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPES / Cancer is characterized by uncontrolled cell growth of a particular tissue, which invades and impairs healthy cells functions. Chemotherapy is the main cancer treatment, and consists of drug administration that interferes in several metabolic pathways, leading to cancer cell death. Among the main chemotherapy drugs, antimitotics directly affect cell division. This study aimed to investigate the effect of a pyrimidinone derivative (4-4-chloro-phenyl)-2-(-4-methoxy-phenyl)-6-oxo-1,6-dihydropyrimidine- 5-carbonitrile, Py-09) on embryonic development of the sea urchin Echinometra lucunter. Adult animals were collected at João Pessoa coast, Paraíba, Brazil and kept in filtered sea water under constant air flow. Gametes or embryos were treated with Py-09 and the effects of the compound were analyzed on fertilization, embryonic development, mitochondrial membrane potential (ΔΨm), production of reactive oxygen species (ROS) and ABC transporters activity. Py-09 (12.5 μM) inhibited around 60% fertilization of pretreated eggs. However, treatment of sperm with Py-09 did not affect fertilization rate. Treatment of zygotes with Py-09 inhibited the early embryonic development in a time and dose-dependent pattern, with the maximum effect at 50 μM (EC50 = 12.5 μM). Morphological changes were observed in the pattern of embryos cleavage (unequal cleavage) and at larval stages (irregular distribution and cracks of spicules and pigment cells leakage). Py-09 induced the loss of ΔΨm without altering ROS intracellular levels. The assays with ABCB1 and ABCC1 transporters inhibitors (Reversin 205 and MK571, respectively) showed that Py-09 is not ABC proteins substrate. The intracellular calcein accumulation assay and PY-09/vinblastine association demonstrated Py-09 was not able to increase intracellular calcein fluorescence levels and that the compound did not reverse MXR phenomenon. In summary, this study demonstrated that the Py-09 features a remarkable antimitotic activity, producing changes both in morphology and cell physiology. Further studies are needed for a better understanding of the mechanism of action of the compound, and research on the potential of Py-09 as pharmacological tool for in vitro studies, as well as its therapeutic use. / O câncer é caracterizado pelo crescimento descontrolado de células de um determinado tecido, que invadem e comprometem, funcionalmente, células sãs do organismo. A quimioterapia é o principal tratamento do câncer, consistindo na administração de drogas que interferem em diversas vias metabólicas, ocasionando a morte celular. Dentre os principais quimioterápicos, os antimitóticos são drogas que afetam, diretamente, a divisão celular.O presente trabalho teve como objetivo investigar a atividade antimitótica de um derivado de pirimidinona (Py-09) no desenvolvimento embrionário do ouriço-do-mar Echinometra lucunter. Animais adultos foram coletados na costa João Pessoa, Paraíba, Brasil, mantidos em água do mar filtrada sob fluxo de ar constante. Os gametas foram coletados por injeção intracelomática de KCl. Os gametas ou embriões foram tratados com Py-09 e foi analisada a atividade do composto sobre a fertilização, o desenvolvimento embrionário, o potencial de membrana mitocondrial interna (ΔΨm), a produção de espécies reativas de oxigênio (ROS) e a atividade de transportadores ABC. O Py-09 (12,5 μM) inibiu, em cerca de 60%, a fertilização de óvulos previamente tratados com o composto. No entanto, o tratamento dos espermatozoides com o Py-09 não afetou a taxa de fertilização. O tratamento dos zigotos com o Py-09 inibiu o desenvolvimento embrionário inicial, apresentando um efeito antimitótico dose e tempo-dependente, atingindo um efeito máximo na concentração de 50 μM (CE50 = 12,5 μM). Foram observadas alterações morfológicas no padrão de clivagem dos embriões (clivagem desigual) e em estágios larvais (distribuição irregular e fissuras das espículas e extravasamento de células pigmentares).O tratamento com Py-09 promoveu a perda do ΔΨm, sem, entretanto, alterar os níveis intracelulares de ROS. O ensaio com os inibidores dos transportadores ABCB1 e ABCC1 (Reversina 205 e MK571, respectivamente) mostrou que o Py-09 não é substrato de proteínas ABC. Por outro lado, o ensaio de acúmulo intracelular de calceína e os ensaios de associação do Py-09 com a vimblastina demonstraram que o mesmo não reverte o fenômeno MXR, uma vez que o composto não foi capaz de aumentar os níveis de fluorescência intracelular da calceína, e a associação Py-09 (12,5 μM)/vimblastina (100 e 400 nM) apresentou o mesmo efeito inibitório da vimblastina per se.Em suma, o presente trabalho demonstrou que o Py-09 apresenta uma marcante atividade antimitótica, acarretando alterações tanto na morfologia quanto na fisiologia celular.Estudos adicionais são necessários para um maior entendimento do mecanismo de ação do composto, e para a investigação acerca do potencial do Py- 09 como ferramenta farmacológica para estudos in vitro, assim como para o seu uso terapêutico. Antimitótico Pirimidinona Fertilização Desenvolvimento embrionário Divisão celular Antimitotic Pyrimidinone Fertilization Embryonic development Cell division CIENCIAS BIOLOGICAS::BIOLOGIA GERAL
276	Estudo genético da interação entre as proteínas FtsZ e SpoIIE em Bacillus subtilis / Genetic study of the interaction between the FstZ and SpoIIE proteins in Bacillus subtilis Maxwell de Castro Durvale 12 November 2013 (has links) Um dos principais componentes envolvidos no processo de divisão celular bacteriana é FtsZ, uma proteína homóloga à tubulina eucariótica. FtsZ polimeriza no interior da célula formando um anel ao qual dá-se o nome de anel Z, responsável pelo recrutamento de diversas outras proteínas de divisão, formando o divisomo. Como meio de sobrevivência sob condições adversas, alguns procariotos, como B. subtilis, podem sofrer um tipo de diferenciação celular que forma um organismo em estado latente, conhecido como esporo. A primeira etapa da formação do esporo é a mudança da posição do anel Z para mais próximo a um dos pólos da célula, produzindo duas células com tamanhos diferentes. SpoIIE é uma proteína fosfatase integral de membrana, que se localiza especificamente no septo assimétrico de uma célula em processo de esporulação. Além de um papel na ativação do fator de transcrição de esporulação σF, SpoIIE se liga a FtsZ e a auxilia na formação do septo assimétrico. Para definirmos a região de FtsZ responsável pela interação com SpoIIE, neste trabalho foram realizados ensaios de duplo-híbrido utilizando vetores com domínios de ativação e de ligação ao DNA do fator de transcrição GAL4 de levedura fusionados a diferentes porções de FtsZ, bem como a SpoIIE. Esses experimentos não forneceram informações sobre interação entre essas proteínas, já que através deles não foi possível reproduzir o resultado positivo descrito na literatura. Como alternativa ao duplo-hibrido para identificarmos o sítio de interação entre as duas proteínas, criamos uma triagem genética capaz de identificar mutantes de FtsZ que não interagem com SpoIIE, fazendo uso de uma biblioteca de mutantes de FtsZ já disponível no laboratório. Foi padronizada uma técnica de microscopia em larga escala em placas de 96 poços, que permitiu a triagem de mais de mil de mutantes de FtsZ, em busca de um em que SpoIIE-GFP induzido não localizasse no anel Z em célula vegetativa. Porém todos os mutantes triados ainda localizavam SpoIIE-GFP. Paralelamente, foi realizada uma triagem de supressão, utilizando como ponto de partida um mutante de SpoIIE que perdeu capacidade de interagir com FtsZ e buscando mutações em FtsZ que reestabelecessem a interação com SpoIIE mutante. Foram triados cerca de 35000 mutantes nesse ensaio, dentre os quais dezoito apresentaram o fenótipo esperado para um supressor. No entanto, todos os candidatos selecionados tratavam-se de falsos-positivos. O motivo que leva esses candidatos a apresentarem o fenótipo esperado sem reestabelecer a interação entre as duas proteínas ainda é desconhecido. A fim de confirmar se não haveria outras proteínas do divisomo responsáveis por intermediar a interação entre FtsZ e SpoIIE, foram feitos experimentos de co-localização de FtsZ e SpoIIE na ausência de DivIB e FtsA. Em ambos os casos SpoIIE ainda localiza no divisomo, descartando a possibilidade de que DivIB e FtsA sejam mediadores da interação FtsZ-SpoIIE. Por fim, foram realizados experimentos de co-localização de SpoIIE com mutantes de FtsZ previamente identificados em outros experimentos em nosso laboratório. Nesse experimento foi identificado que a expressão de SpoIIE-GFP induzida por IPTG é capaz de reestabelecer a frequência de divisão no mutante FtsZ-R376T, que normalmente é deficiente na formação de divisomos. Esse resultado reforça a idéia de que essas proteínas interagem diretamente, e sugere que SpoIIE é capaz de reestabelecer a atividade de FtsZ em um mutante que apresente falhas na polimerização. / One of the major components involved in bacterial cell division is FtsZ, a protein homologous to the eukaryotic tubulin. FtsZ polymerizes inside the cell forming a ring to which is given the name Z ring, wich is responsible for the recruitment of several other proteins division, forming the divisome. As a means of survival under adverse conditions, some prokaryotes such as B. subtilis may undergo a type of cell differentiation that results in an organism in a latent state, known as a spore. The first stage of the spore formation is to change the Z ring position closer to the poles of the cell, producing two cells of different sizes. SpoIIE is an integral membrane phosphatase protein, which is specifically located in the septum of an asymmetric cell in sporulation process. In addition to a role in the activation of the sporulation transcription factor σF, SpoIIE binds to FtsZ and assists in the formation of the asymmetric septum. To define the FtsZ region responsible for interaction with SpoIIE, in this work we performed tests using two-hybrid vectors with activation and DNA binding domains of the yeast transcription factor GAL4 fused to different portions of FtsZ and SpoIIE. These experiments did not provide information on the interaction between these proteins, since through them it was not possible to reproduce the positive results reported in the literature. As an alternative to the two-hybrid to identify the site of interaction between the two proteins, we created a genetic screening that can identify FtsZ mutants that cannot interact with SpoIIE, using a library of FtsZ mutants already available in the laboratory. We standardized a large scale microscopy using 96-well plates, allowing the screening of over a thousand mutants of FtsZ in search of a induced SpoIIE-GFP which would no longer localize at the vegetative cell Z ring. However, all the screened mutants still localized SpoIIE-GFP. In parallel, we performed a screening of suppression, using as a starting point a SpoIIE mutant that lost the ability to interact with FtsZ and searching for mutations in FtsZ that would reestablish interaction with the SpoIIE mutant. We screened approximately 35,000 mutants in this essay, eighteen of which showed the phenotype expected for a suppressor. However, all selected candidates were false positives. The reason why such candidates do show the expected phenotype without reestablishment of the interaction between the two proteins is still unknown. In order to confirm whether there would be other divisiome proteins responsible for mediating the interaction between FtsZ and SpoIIE, co-localization experiments were made using FtsZ and SpoIIE in the absence of DivIB and FtsA. In both cases SpoIIE still located in divisome, ruling out the possibility that DivIB and FtsA are essencial mediators of the SpoIIE-FtsZ interaction. Finally, co-localization experiments were carried out with SpoIIE and FtsZ mutants previously identified in other experiments in our laboratory. In this experiment it was identified that the expression of IPTG-induced SpoIIE-GFP is able to restore the division frequency in the FtsZ-R376T mutant, which normally is deficient in the formation of divisomes. This result reinforces the idea that these proteins interact directly, and suggests that SpoIIE is able to restore the activity of FtsZ in a mutant that presents defect in polymerization. Bacillus subtilis Divisão celular Esporulação FtsZ Interação entre proteínas SpoIIE Bacillus subtilis Cell division FtsZ Protein interaction SpoIIE Sporulation
277	Estudo do processo de divisão em Bacillus subtilis por microscopia de fluorescência vital / Study of cell division in Bacillus subtilis by fluorescence microscopy Guilherme Louzada Silva Meira 23 June 2010 (has links) A divisão celular em B. subtilis inicia-se pela formação de um complexo multiprotéico, o divisomo, no sítio onde a bactéria irá se dividir. FtsZ é a primeira proteína a se localizar no futuro sitio de divisão, formando uma estrutura em anel (anel Z) que se estende por toda a circunferência da célula. O anel Z funciona como um arcabouço responsável por recrutar outras quinze proteínas de divisão que irão participar da montagem do divisomo. Nesta tese, utilizamos abordagens quantitativas e qualitativas de microscopia de fluorescência vital para estudarmos duas questões ainda não esclarecidas sobre o funcionamento do divisomo. A primeira delas é como o divisomo é montado. Para estudarmos a montagem do divisomo nós realizamos ensaios de co-localização entre o anel Z (FtsZ-mCherry) e as proteínas ZapA, EzrA, FtsW, FtsL, YpsB , DivIVA, e MinC fusionadas a GFP. Quanto maior a freqüência de co-localização entre FtsZ e outra proteína de divisão, mais inicial é a participação da proteína na formação do divisomo. Portanto, a medida da freqüência de co-localização entre o anel Z e as proteínas componentes do divisomo permite que se deduza uma cinética da montagem deste complexo. Estes ensaios demonstraram uma freqüência de co-localização de 97,33% para ZapA; 98,31% para EzrA; 83,90% para FtsW; 78,43% para FtsL; 50% para YpsB; 41,7% para DivIVA e 31,64% para MinC. Estes resultados sugerem que o divisomo seja formado em três etapas. ZapA e EzrA se associam ao divisomo imediatamente após a formação do anel Z, em seguida FtsW e FtsL são recrutados para o divisomo, e por último YpsB, DivIVA, MinC associam-se ao divisomo. A segunda questão que investigamos nesta tese foi o mecanismo da mudança de posição do divisomo que ocorre durante a esporulação em B. subtilis. Na fase de esporulação a célula divide-se assimetricamente, com a formação do septo próxima a um dos pólos. Durante o crescimento vegetativo a divisão não ocorre próxima aos pólos por causa da ação das proteínas MinC, MinD e DivIVA, importantes reguladores espaciais da divisão. MinCD e DivIVA são inibidores da formação do anel Z que durante o crescimento vegetativo se localizam nos pólos das células.. Uma hipótese para explicar o uso dos sítios polares para a divisão durante a esporulação seria que as proteínas MinCD e DivIVA seriam removidas dos pólos celulares. Para testarmos esta hipótese, estudamos a localização das proteínas MinCD e DivIVA durante a esporulação. Nossos resultados demonstraram que MinCD e DivIVA se re-localizam e saem dos pólos celulares durante a esporulação. Porém esta dinâmica ocorre após a formação do anel Z assimétrico, sugerindo que o anel Z seja insensível a estes inibidores durante a esporulação. Por ensaios genéticos em B. subtilis demonstramos que a proteína SpoIIE, conhecida como provável proteína responsável por promover a formação do septo assimétrico, seja capaz de contrapor a ação de MinC no início da esporulação. Dessa maneira nós propomos um novo modelo de mudança da divisão simétrica para assimétrica durante a esporulação, diferentemente da simples saída do complexo MinCD dos pólos como é proposto na literatura. / Bacillus subtilis division begins through the formation of a multiprotein complex, the divisome, at the site of division. FtsZ is the earliest known protein to localize to the future division site where the protein forms a ring-like structure (Z-ring) that extends around the circumference of the cell. The Z-ring functions as a scaffold and recruits about fifteen other division proteins that compose the divisome. In this work, we used quantitative and qualitative methods of vital fluorescence microscopy to study two questions that have not been elucidated about the divisome dynamics. The first is how divisome is assembled. To address that problem, we made co-localization between Z-ring (FtsZ-mCherry) and proteins ZapA, EzrA, FtsW, FtsL, YpsB, DivIVA, and MinC fused to GFP. Higher is the match between GFP fusions to Z-ring, earlier is the assembly of division proteins to divisome. Therefore, the co-localization frequency between Z ring and divisome proteins will allow us to deduce the assemble kinetics of the divisome. This assays showed a co-localization frequency of 97,33% for ZapA; 98,31% for EzrA; 83,90 for FtsW; 78,43% for FtsL; 50% for YpsB; 41,7% for DivIVA and 31,64% for MinC. This data suggests that the divisome does not assemble in two but in three steps. ZapA and EzrA assemble into the divisome immediately after Z ring formation, secondly FtsW and FtsL were recruited to the divisome, and finally YpsB, DivIVA, MinC associated with the divisome. The second question that we investigated in this work is the mechanism responsible for change the divisome position that occurs during sporulation in B. subtilis. In sporulation the cell divides asymmetrically, with a septum formation near poles. During vegetative grown the divisiome does not occur near poles because of MinC, MinD and DivIVA action, relevant for spatial regulation of division. MinCD and DivIVA are inhibitors of Z ring formation that during vegetative growth are located at poles. A hypothesis to explain the use of polar sites for division during sporulation would be that MinCD and DivIVA would be removed from cellular poles. To test this hypothesis, we studied the location of MinCD and DivIVA proteins during sporulation. Our results demonstrated that MinCD and DivIVA re-localize and leave to cell poles during sporulation. However this process occurs after asymmetric Z ring formation, suggesting that Z ring would be unresponsive to this inhibitors during sporulation. Through genetics assays in B. subtilis we demonstrated that SpoIIE protein, known to probably play a role in asymmetric septum formation, would be able to contrapose MinC action during early sporulation. Therefore, we propose a novel model for change the symmetric to asymmetric division during sporulation, unlike the release of MinCD from pole proposed in the literature. Bacillus subtilis Complexo MinCD Divisão celular Divisomo Esporulação FtsZ SpoIIE Bacillus subtilis Cell division Divisome FtsZ MinCD complex SpoIIE Sporulation
278	Etude du rôle de la région terminale du chromosome dans le positionnement, la ségrégation du chromosome et le contrôle de la division cellulaire chez Escherichia coli / Study of the role of the ter region in chromosome positioning, chromosome segregation and control of cell division in Escherichia coli Lebailly, Elise 30 September 2016 (has links) Escherichia coli, comme la majorité des bactéries, possède un unique chromosome circulaire. Au moins une copie du chromosome doit être transmise à chacune des cellules filles avant la division cellulaire afin d'assurer une prolifération cellulaire correcte. Une couplage spatio-temporel précis de la ségrégation avec la division cellulaire est donc nécessaire pour assurer la bonne répartition des deux chromosomes après réplication. La région terminale du chromosome (ter) est la dernière à être répliquée et ségrégée, et migre du pôle vers le centre de la cellule au moment de la mise en place du septum de division, à la fin du cycle cellulaire. Les loci de la région ter présentent une période de cohésion post-réplicative étendue. Cette cohésion étendue est contrôlée par la protéine MatP, qui se fixe spécifiquement au niveau des sites matS, présents uniquement dans ter. MatP se fixe à l'ADN sous forme de dimère, via son domaine N-terminal, et tétramérise via son domaine C-terminal. La tétramérisation est stimulée par la liaison à l'ADN et permet le pontage de deux sites matS distants. MatP interagit aussi avec ZapB, un composant du divisome, la machinerie protéique participant à la formation du septum. Alors que la tétramérisation de MatP semble importante pour la compaction de la région ter, son interaction avec ZapB, qui est localisée au septum via ZapA et FtsZ, participe au positionnement et à la cohésion étendue de cette région. Le couplage de la région ter avec le divisome est essentiel pour le bon déroulement de nombreux évènements tardifs du cycle cellulaire : (i) la ségrégation active, ordonnée et progressive de la région ter par FtsK, un composant du divisome, (ii) la résolution des dimères de chromosomes via la recombinaison spécifique de site XerCD/dif, activée par FtsK, (iii) la résolution des liens d'intercaténation par la TopoIV et (iv) la régulation positive de l'assemblage du divisome en absence des régulateurs négatifs MinCDE et SlmA. Pendant ma thèse, je me suis tout d'abord intéressée au rôle de MatP dans la structuration globale du chromosome. En utilisant un système permettant de visualiser deux loci marqués avec un site parSp1 et un site parSpMT1, reconnu par ParBp1 et ParBpMT1 spécifiquement, nous avons analysé le positionnement et l'orientation du chromosome dans la cellule. Nous avons montré que MatP est nécessaire au positionnement et à l'orientation de tout le chromosome à la fin du cycle cellulaire. La localisation de SlmA dans des souches wt et DeltamatP prouve que l'inactivation de MatP, induisant une mauvais positionnement du chromosome, s'accompagne d'une défaut de localisation de SlmA, et induit donc une inhibition de la division. Ces résultats pris ensemble montre que MatP, SlmA et leur communication à travers la structuration globale du chromosome sont importants pour le management du chromosome et le contrôle de la division cellulaire. En collaboration avec l'équipe d'Olivier Espeli, nous avons utilisé des méthodes de génomiques et de biologie moléculaire pour caractériser la régulation de la TopoIV au cours du cycle cellulaire d'E. coli. Nous avons montré qu'au site dif, les activités de fixation et de clivage de la TopoIV sont améliorées par la présence des recombinases XerCD et de MatP. L'amélioration de l'activité de la TopoIV favorise la décaténation des chromosomes nouvellement répliqués et assure, en lien avec d'autres processus, la séparation précise des chromosomes frères. Ces résultats permettent de mieux comprendre le réseau d'interactions dédiées au management du chromosome à la fin du cycle cellulaire, et l'influence du management du chromosome sur le contrôle de la division cellulaire. / Escherichia coli, as the majority of bacteria, has a unique circular chromosome. Faithfull cell proliferation requires that a least one copy of the chromosome is transmitted to sister cells prior to cell division. A strict temporal and spatial coupling of chromosome segregation with cell division is thus required to ensure the accurate separation of the two fully replicated chromosomes. The terminal region of the chromosome (ter) is the last one to be replicated and segregated, and moves from the pole to the middle of the cell where the division septum is formed, at the end of the cell cycle. Loci of the ter region display an extended cohesion period. This extended cohesion is controlled by the MatP protein, which binds specific matS sites restricted to the ter region. MatP binds DNA as a dimer and forms tetramers via its N-terminal and C-terminal domains respectively. Tetramerisation is stimulated by binding to DNA and pairs remote matS sites. MatP also interacts with ZapB, a component of the divisome, the protein machinery that contributes to septum formation. While tetramerisation of MatP appears important for compacting the ter region, its interaction with ZapB, which is localized at the septum via ZapA and FtsZ, is involved in the positioning and the extended cohesion of this region. The linkage of the ter region with the divisome is required for the success of many later events of the cell cycle : (i) the active, ordered and progressive segregation of the ter region by FtsK, a component of the divisome, (ii) resolution of chromosome dimers via the site-specifique recombination XerCD/dif, activated by FtsK, (iii) the resolution of intercatenation links by TopoIV and (iv) the positive regulation of divisome assembly in the absence of the negative regulators MinCDE and SlmA. During my thesis, I first studied the role of MatP in the chromosome management. By using pairs of loci tagged with parSp1 and parSpMT1 sites recognized by cognate ParB-XFP proteins, we directly analysed chromosome positioning and orientation in the cell. We show that MatP is required for normal positioning and orientation of the whole chromosome at the end of the cell cycle. The localisation of SlmA in wt and Delta matP strains proves that inactivation of MatP leads to inaccuracy of nucleoid positioning accompanied by defects in SlmA localisation, and thus induces division inhibition. Take together, these results show that MatP, SlmA and their interplay are important for chromosome management and control of cell division in E. coli. In collaboration with O. Espeli's team, we have used genomic and molecular biology methods to characterize TopoIV regulation during the E. coli cell cycle. We show that at the dif site, TopoIV binging and cleavage are enhanced by the presence of the XerCD recombinases and MatP. This enhancement of TopoIV activity at dif promotes decatenation of fully replicated chromosomes and ensure, through interaction with other processes, accurate separation of sister chromosomes. These results provide insight into the protein network dedicated to the final step of chromosome management during the cell cycle, and how the chromosome management is linked to cell division. Ségrégation des chromosomes Division cellulaire Région ter MatP SlmA TopoIV Chromosome segregation Cell division Escherichia coli Ter region MatP SimA TopoIv
279	Etude comparative du positionnement du fuseau mitotique dans les espèces de C.elegans et C. briggsae / Comparative study of the mitotic spindle positioning in C. elegans and C. briggsae species Riche, Soizic 09 December 2015 (has links) La division cellulaire asymétrique est un mécanisme fondamental qui assure la diversité cellulaire, le renouvellement des cellules souches et le maintien de l’identité cellulaire. Elle dépend du bon positionnement du fuseau mitotique car il dicte le plan de division des cellules. La première division des embryons de C. elegans, est asymétrique et génère deux cellules fille de taille et devenir différents. Elle consiste en deux étapes : la centration des pronoyaux en prophase puis le déplacement postérieur du fuseau mitotique en anaphase. Lors de l'anaphase le fuseau subit des oscillations transverses plus marquées au pôle postérieur qu’au pôle antérieur. Ces mouvements sont contrôlés par des forces de traction agissant sur les microtubules astraux. Les générateurs de force ont été moléculairement identifiés et sont évolutivement très conservés. Un complexe composé de protéines Gα, liées à GPR (protéine à domaine GoLoco, homologue de LGN/Pins), à LIN-5 (protéine à domaine super-enroulé, homologue de NuMA/Mud) et à la dynéine serait ancré au cortex et activé en début de mitose pour tirer le fuseau. En analysant la première division d’une espèce proche de C. elegans : C. briggsae, on observe des variations de trajectoire du fuseau. Les embryons de C. briggsae présentent un décalage antérieur des noyaux en prophase et les oscillations du fuseau sont réduites en anaphase. La combinaison de perturbations physiques et l'analyse de mutants dans ces espèces, ont montré que ces différences s’expliquent par des changements dans la régulation du complexe ternaire. Mais, nous avons découvert que dans les deux espèces 1) un switch positionnel conservé contrôle le démarrage des oscillations du fuseau, 2) la localisation postérieure de GPR détermine ce switch positionnel, et 3) l'amplitude maximum des oscillations est déterminée en partie par le temps passé dans la phase oscillatoire. Nous avons utilisés ces variants pour corréler les phénotypes, la localisation de GPR et la divergence de séquence entre espèces afin d’identifier les éléments de régulation de cette protéine. Nous avons alors échangé les protéines et construits des protéines chimères entre les deux espèces. Enfin, par optogénétique, nous avons essayé de contrôler la localisation temporelle de GPR et analyser les conséquences sur les mouvements des noyaux et du fuseau. En étudiant la microévolution d'un processus sous-cellulaire, nous avons identifié de nouveaux mécanismes qui contribuent à la compréhension du positionnement du fuseau. / Asymmetric cell division is a fundamental mechanism essential in all organisms to assure cell diversity, stem cell renewal and cellular identity maintenance. It is relying on proper mitotic spindle positioning because it dictates the cell division plan. In C. elegans one-cell embryos, the first division is asymmetric and gives rise to two daughter cells of unequal size and fate. It occurs in two steps: pronuclei centration during prophase and spindle posterior displacement during anaphase. During anaphase, the mitotic spindle undergoes transverse oscillations that are more pronounced for the posterior than the anterior pole. These movements are controlled by pulling forces acting on astral microtubules. The force generators are identified and are evolutionary conserved. A complex made of Gα proteins, linked to GPR (a GoLoco containing protein, the LGN/Pins homologues), LIN-5 (a coiled-coil protein, the NuMA/Mud homologues) and dynein is thought to be anchored at the cortex and activated at the onset of mitosis to pull on the spindle. We identified variations in spindle trajectories by analyzing the outwardly similar one-cell stage embryo of a close relative of C. elegans, C. briggsae. Compared to C. elegans, C. briggsae embryos exhibit an anterior shifting of nuclei in prophase and reduced anaphase spindle oscillations. By combining physical perturbations and mutant analysis in both species, we show that differences can be explained by inter-species changes in the regulation of the cortical Gα/GPR/LIN-5 complex. However, we uncover that in both species 1) a conserved positional switch controls the onset of spindle oscillations, 2) GPR posterior localization may set this positional switch, and 3) the maximum amplitude of spindle oscillations is determined in part by the time spent in the oscillating phase. Interestingly, GPR is poorly conserved at the amino acid level between these species. We use these variants to correlate phenotypes, GPR localization and sequence divergence to identify GPR regulatory elements. To this end, we performed protein replacement between species, as well as analysis of protein chimeras. Finally we tried to use optogenetics in order to control GPR localisation temporally and analyze the consequences on pronuclei and spindle movements during the first division. By investigating microevolution of a subcellular process, we identified new mechanisms that are instrumental to decipher spindle positioning. Division cellulaire asymétrique Positionnement du fuseau Nématodes GPR Évolution des processus cellulaires Asymmetric cell division Spindle positioning Nematodes GPR Evolutionary Cell Biology
280	Influence Of FtsH Protease On The Medial FtsZ Ring In Escherichia Coli Bhatt, Brijesh Narayan 08 1900 (has links) (PDF) FtsH is an essential AAA family Zn++ metalloprotease of Escherichia coli, possessing ATPase-dependent chaperon activity and ATP-dependent protease activity. Heat shock transcription factor Sigma32, LpxC, SecY, and bacteriophage protein CII are some of the substrates of FtsH. Although FtsH is known to influence several cellular processes, the role of FtsH in bacterial cell division had not been identified. FtsZ is the principal cell division protein that marks the cell division site at mid-cell by forming a ring structure. Using a pair of ftsH-null and isogenic wild type strain of E. coli, earlier studies in the laboratory had demonstrated that proteolytic function of FtsH is required for the presence of FtsZ rings at mid-cell site. It was also shown that FtsZ is not a substrate for FtsH protease in vivo. In view of these observations, using a pair of ftsH-null and isogenic wild type strain of E. coli, experiments were carried out to find out the mechanism behind the requirement for FtsH protease for the presence of FtsZ ring at mid-cell site. Viability of the cells having ftsH-null status was maintained by a suppressor mutation at another locus, and was found to be comparable to that of isogenic wild type cells. Immunostaining for FtsZ showed that only 20% cells of ftsH-null strain of E. coli has FtsZ ring at mid-cell site, On the contrary, more than 90% cells of isogenic wild type cells had FtsZ ring at mid-cell site. Live cell imaging with FtsZ-GFP also showed similar results. Low fraction of ftsH-null cells having FtsZ ring was found to be independent of slow growth rate of the cells. Confocal microscopy revealed that ftsH-null cells lacked the normal helical spiral-type structure of FtsZ, unlike the intact FtsZ helices present in isogenic wild type cells. FtsZ protein levels in the membrane and cytoplasmic fractions of ftsH-null cells were found to be same as those in the isogenic wild type cells. Exogenous expression of wild type FtsH in ftsH-null cells could restore FtsZ ring status to normalcy, similar to that in the isogenic wild type cells. However, this restoration could not be accomplished by FtsH mutants, which were lacking in ATP binding, ATPase, or protease activities. FtsA anchors FtsZ to the membrane and a specific FtsZ/FtsA ratio is known to be critical for cell division. Further, FtsA and/or ZipA are required for the stabilisation of FtsZ ring at mid-cell site. The levels of FtsA were found to be lower by more than 2.5-fold in all the membrane and soluble fractions of ftsH-null cells. The levels of FtsA were found restored to normalcy upon complementation with exogenous expression of FtsH. Low levels of FtsA were not due to the slow growth of ftsH-null cells. Exogenous expression of FtsA or FtsA-GFP restored FtsZ in more than 90% of ftsH-null cells. Moreover, FtsA mutants, which are defective in the interaction with FtsZ, did not restore FtsZ rings to normalcy. The levels of ZipA were found to be same in ftsH-null and isogenic wild type cells. Expression of ZipA or ZipA-GFP could restore FtsZ rings to normalcy in ftsH-null cells. These data showed that low FtsA levels might be the reason for low percentage of cells having FtsZ ring in ftsH-null cells. It implied that ftsH-null cells might have been managing FtsZ ring stabilisation with ZipA, to facilitate septation. Real time RT-PCR showed that the levels of ftsA mRNA and those of all the other fts genes, except ftsZ, in the 16-gene dcw cluster, were found to be low in ftsH-null cells. Moreover, real time RT-PCR using specific primers designed for multiple promoters of ftsZ and for the RNaseE processing site, just upstream of ftsZ, showed that the levels of transcripts of the genes upstream to RNaseE site were significantly low and that the levels of ftsZ transcripts, which were downstream to RNaseE site, were unaffected. On the contrary, the levels of mRNAs of fts genes, such as ftsE, ftsX, ftsN, and zipA that were located at another part of the genome, were normal in ftsH-null cells. These observations suggested that the reason for the low levels of FtsA protein might be low levels of ftsA mRNA. In addition, the low levels of other fts mRNAs from the dcw cluster, and probably of the respective proteins, might contribute to the slow growth of ftsH-null cells. The ftsH null strains also showed less compact nucleoids and the nucleoids did not look bilobular. This data suggested that there may be some defect in the compaction of nucleoids in ftsH-null cells. On the contrary, isogenic wild type cells, when grown slow like the growth of ftsH-null cells, had no defect in nucleoid compaction and looked bilobular. The proper compaction of nucleoids could be restored only by wild type FtsH, but not by the protease mutant of FtsH. These observations suggest that proteolytic activity of FtsH might be required for the proper compaction of nucleoids, which in turn might have influence on the placement of FtsZ ring at mid-cell site. In parallel, different percentage of silver stained single-dimension SDS-PAGE showed conspicuous difference in the protein profiles of the membrane and soluble fractions of ftsH-null cells, in comparison to those of isogenic wild type cells. FtsZ co-immuno precipitation (CoIP) of total cell lysates of ftsH-null and isogenic wild type cells showed differential interaction of two proteins, the outer membrane protein A (OmpA) and a 50 kDa protein, between the two strains. The level of OmpA was 2.5-fold high in ftsH-null cells, in comparison to that in isogenic wild type cells. However, overexpression of ompA in isogenic wild type cells did not have any effect on FtsZ rings in isogenic wild type cells. Two-dimensional gel electrophoresis for membrane and soluble fractions of ftsH-null cells, in comparison with that of isogenic wild type cells, showed that several proteins in each fraction were either present or absent between these two strains. Most of these proteins were then identified using MALDI-TOF / LC –MS methods. Identification of these proteins, which were present differentially between ftsH-null and isogenic wild type cells, has revealed existence of many more hitherto unidentified potential substrates of FtsH and therefore cell processes, which FtsH may influence. Bacterial Cell Escherichia Coli FtsH Protease FtsZ Ring Cell Division Genes Bacterial Cell Septation FtsA E. coli Biochemistry

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