Global ETD Search

331	Negative Regulation of Polarity Establishment in Saccharomyces cerevisiae Miller, Kristi E. 24 June 2019 (has links) No description available. Molecular Biology Cellular Biology
332	WNT7A and EGF Alter Myogenic Differentiation in hiPSCs Derived from Duchenne Muscular Dystrophy Patients Madana, Maria 22 June 2023 (has links) Duchenne Muscular Dystrophy (DMD) is a disorder caused by loss-of-function mutations in dystrophin, a critical protein that maintains muscle fiber integrity. Our lab discovered that dystrophin-deficient skeletal muscle stem cells, also known as satellite cells, cannot generate enough myogenic progenitors for proper muscle regeneration. Previously, we demonstrated that WNT7A, a protein expressed during muscle regeneration, stimulates symmetric division of satellite cells, and gives rise to two daughter satellite cells. Conversely, epidermal growth factor (EGF) induces asymmetric division, which generates one daughter satellite cell and one committed precursor cell. We aimed to investigate these satellite cell division mechanisms following WNT7A or EGF treatment in a human model using healthy and DMD-patient derived hiPSCs differentiated into the myogenic lineage. The presence of satellite-like cells was confirmed in both lines by their characteristic expression of PAX7 and other myogenic markers. Intriguingly, DMD-patient hiPSCs precociously differentiated compared to healthy control human induced pluripotent stem cells (hiPSCs). More notably, WNT7A treatment had a potent effect on the DMD differentiated cells. High content analysis revealed an expansion of the satellite-like cell pool as observed by a higher number of PAX7+ cells within the total population and gene expression analysis demonstrated a significant increase in global PAX7 expression. In contrast, EGF treatment reduced the number of PAX7+ cells and increased the proportion of MYOG+ cells within the myogenic population, indicating an increase in myogenic progenitors. Taken together, WNT7A and EGF can alter the myogenic differentiation program of healthy and DMD-patient derived hiPSCs by modulating the satellite-like cell division dynamics. Skeletal Muscle Stem Cells Satellite Cells Duchenne Muscular Dystrophy WNT7A Epidermal Growth Factor Symmetric Division Asymmetric Division Human Induced Pluripotent Stem Cells Cell Differentiation Myogenesis Cell Division
333	Probabilistic Multi-Compartment Deformable Model, Application to Cell Segmentation Farhand, Sepehr 12 July 2013 (has links) Indiana University-Purdue University Indianapolis (IUPUI) / A crucial task in computer vision and biomedical image applications is to represent images in a numerically compact form for understanding, evaluating and/or mining their content. The fundamental step of this task is the segmentation of images into regions, given some homogeneity criteria, prior appearance and/or shape information criteria. Specifically, segmentation of cells in microscopic images is the first step in analyzing many biomedical applications. This thesis is a part of the project entitled "Construction and profiling of biodegradable cardiac patches for the co-delivery of bFGF and G-CSF growth factors" funded by National Institutes of Health (NIH). We present a method that simultaneously segments the population of cells while partitioning the cell regions into cytoplasm and nucleus in order to evaluate the spatial coordination on the image plane, density and orientation of cells. Having static microscopic images, with no edge information of a cytoplasm boundary and no time sequence constraints, traditional cell segmentation methods would not perform well. The proposed method combines deformable models with a probabilistic framework in a simple graphical model such that it would capture the shape, structure and appearance of a cell. The process aims at the simultaneous cell partitioning into nucleus and cytoplasm. We considered the relative topology of the two distinct cell compartments to derive a better segmentation and compensate for the lack of edge information. The framework is applied to static fluorescent microscopy, where the cultured cells are stained with calcein AM. Cell segmentation Multi-compartment geometric model Fluorescent microscopy Computer Vision Computer vision Bioinformatics Image processing -- Mathematical models Geometrical models Fluorescence microscopy Diagnostic imaging -- Digital techniques Cell division
334	Determining Molecular Mechanisms of Cell Division in Fission Yeast by Testing Major Assumptions of the Search, Capture, Pull, and Release Model of Contractile-Ring Assembly Coffman, Valerie Chest 24 July 2013 (has links) No description available. Cellular Biology Genetics Molecular Biology cytokinesis node contractile ring formin myosin fission yeast centromere Cnp1 Cse4 kinetochore quantitative microscopy cell division tetrad fluorescence microscopy
335	Caractérisation et identification du site dif chez Caulobacter crescentus Farrokhi, Ali 10 1900 (has links) La plupart des espèces bactériennes possèdent un chromosome circulaire qui est répliqué de façon bidirectionnelle au cours du cycle cellulaire. Bien que la réplication et la ségrégation du chromosome bactérien se développent simultanément, la ségrégation du chromosome s’accomplit après la fin de la réplication et avant la fermeture du septum. La circularité du chromosome bactérien et le grand nombre d’événements de recombinaison homologue donnent lieu à la création des dimères de chromosome dans une fraction de la population cellulaire. Chez Escherichia coli et Bacillus subtilis, la dimérisation des chromosomes se produit respectivement dans 15% et 25% des cas. Un chromosome dimérique doit être résolu avant la fermeture du septum. Chez les espèces bactériennes les plus étudiées, les chromosomes dimériques sont résolus par un système de recombinaison site spécifique hautement réservé incluant deux recombinases à tyrosine, XerC et XerD, et un site génomique dans la région terminus du génome bactérien, appelé le site dif (deletion induced filamentation). L’organisation spatio-temporelle du système de recombinaison site spécifique Xer/dif et l’activation de ce dernier sont réglementées par la protéine transmembranaire impliquée dans la division cellulaire, FtsK. D’autre part, des études récentes ont mis en évidence l’existence de plusieurs éléments mobiles appelés IMEXs (Integrative Mobile Elements Exploiting Xer), capables d’exploiter le système Xer/dif pour leur intégration dans le génome bactérien. Chez E. coli, des déficiences dans la résolution des dimères de chromosome se terminent par le guillotinage du chromosome dimérique au cours de la division cellulaire, ce qui entraîne l’induction de la réponse SOS chez les cellules filles et la mort de ces dernières. Dans cette thèse, le site dif a été identifié et caractérisé chez Caulobacter par une combinaison d’approches in vivo et in vitro. Fait intéressant, il a été démontré que chez Caulobacter, contrairement à E. coli, la perturbation du système Xer/dif ne mène pas au guillotinage du chromosome, et les cellules portant un système Xer/dif défectueux contourne cette déficience en adoptant un nouveau mode de cycle cellulaire. De plus, notre analyse comparative entre les terminus des souches sauvages de C. crescentus a également permis de révéler la présence d’un IMEX putatif de 71 kb dans le terminus de C. crescentus NA1000. / Most bacteria possess a single circular chromosome which is replicated bidirectionally during the cell cycle. Although replication and segregation of the chromosome in bacteria develops simultaneously, the segregation of the chromosome occurs after the completion of replication and before the closure of the septum. The circularity of the bacterial chromosome and the high number of homologous recombination events that occur during replication result in the creation of chromosome dimers in a fraction of the cell population. In Escherichia coli and Bacillus subtilis, chromosome dimer formation occurs, respectively, in 15% and 25% of the cell population during replication, which needs to be resolved before the closure of division septum. In most of the well-studied bacterial species, chromosome dimers are resolved by a highly conserved site-specific recombination system which employs two tyrosine recombinases, XerC and XerD, and a recombination genomic site located in the terminus region of the bacterial chromosome called dif (deletion induced filamentation). The temporo-spatial organization of the Xer/dif site-specific recombination system, along with its activation, is regulated by a cell division transmembrane protein, FtsK. In E. coli, deficiencies in the resolution of chromosome dimers result in the guillotining of the dimeric chromosome during the cell division leading to the continuous induction of SOS response in the daughter cells and the death of the latter ones. In my thesis, the dif site in Caulobacter is identified and characterized by a combination of in vitro and in vivo approaches. Interestingly, it was observed that, unlike E. coli, in Caulobacter perturbations in the chromosome dimer resolution system do not result in the guillotining of the chromosome dimers. Instead, Caulobacter cells bearing deficiencies in the resolution of dimeric chromosomes adopt a new mode of cell cycle to bypass this deficiency. Xer dif dimères de chromosome Caulobacter division cellulaire ségrégation chromosomique chromosome dimers cell division chromosome segregation
336	Microtubule arrays and cell divisions of stomatal development in Arabidopsis Lucas, Jessica Regan 16 July 2007 (has links) No description available. Arabidopsis stomata stoma stomate guard cell patterning microtubule PPB Preprophase Band Phragmoplast Cell division Cytokinesis too many mouths tonneau2 M to G1 interface cytokinesis-interphase transition
337	Functional characterization of asymmetric cell division associated genes in hematopoietic stem cells and bone marrow failure syndromes Chan, Derek January 2020 (has links) Hematopoietic stem cells (HSCs) are critical to the development of the hematopoietic system during ontogeny and maintaining hematopoiesis under steady-state. Several genes implicated in asymmetric cell division (ACD) have been found to influence HSC self-renewal in normal hematopoiesis and various leukemias. From a separate survey of genes associated with ACD, I now present the results from dedicated functional studies on two genes – Arhgef2 and Staufen1 – in HSCs and identify their potential contributions to benign hematopoietic disorders. Specifically, I present evidence that demonstrates a conserved role of Arhgef2 in orienting HSC division, the loss of which leads to HSC exhaustion that may underlie and contribute to the pathogenesis of Shwachman-Diamond syndrome. I also identify Staufen1 as a critical RNA-binding protein (RBP) in HSC function, downregulation of which elicits expression signatures consistent with clinical anemias reminiscent of aplastic anemia and/or paroxysmal nocturnal hemoglobinuria. I end by reviewing how RBPs function in HSCs and discuss future research directions that could further elucidate how bone marrow failure syndromes arise at the stem cell level. / Thesis / Doctor of Philosophy (PhD) Hematopoietic stem cell Bone marrow failure Asymmetric cell division Arhgef2 Staufen1 Shwachman-Diamond syndrome Aplastic anemia Paroxysmal nocturnal hemoglobinuria RNA-binding protein
338	Hierarchical regulation of spindle size during early development Rieckhoff, Elisa Maria 24 February 2021 (has links) During embryogenesis, a single cell gives rise to a multi-cellular embryo through successive rounds of cell division. As cells become smaller, cellular organelles adapt their sizes accordingly. The size of the mitotic spindle—the microtubule-based structure controlling these divisions—is particularly important as it determines the distance over which chromosomes are segregated. To perform its function properly, spindle size scales with cell size. However, we still lack a mechanistic understanding of the underlying microtubule-based processes that regulate spindle scaling. In this thesis, I combined quantitative microscopy and laser ablation in zebrafish embryos and Xenopus laevis egg extract encapsulated in oil droplets. My measurements revealed the influence of microtubule length dynamics, transport, and nucleation on cell size-dependent spindle scaling. Strikingly, I discovered a hierarchical regulation of spindle size. In large cells, microtubule nucleation exclusively scales spindle size relative to cell size by changing the number of microtubules within the spindle. In small cells, microtubule dynamics fine-tune spindle size by modulating microtubule length. To understand the mechanism of spindle scaling, I proposed a theoretical model based on a limiting number of microtubule nucleators and microtubule-associated proteins that regulate microtubule length. The transition from nucleation- to dynamics-based scaling requires that microtubule number and the number of microtubule-associated proteins that promote microtubule growth scale differently with cell size. This can be achieved by sequestering an inhibitor of microtubule nucleation to the cell membrane, which is consistent with my measurements of microtubule nucleation. The differential regimes of spindle scaling modulated by microtubule nucleation and dynamics imply a gradual change in spindle architecture, which may ensure faithful chromosome segregation by spindles of all sizes. info:eu-repo/classification/ddc/570 ddc:570
339	Regulation of the Principal Cell Division Protein FtsZ of Escherichia Coli by Antisense RNA and FtsH Protease Anand, Deepak January 2014 (has links) (PDF) The PhD thesis is on the studsy of the influence of the ftsZ antisense RNA and FtsH protease on the synthesis and function of the Escherichia coli cytokinetic protein, FtsZ, which mediates septation during cell division. Thus, it involves three molecules, FtsZ, ftsZ antisense RNA, and FtsH protease. While the E. coli ftsZ antisense RNA is being identified and structurally and functionally characterised for the first time, there has been some earlier studies in the laboratory in which the FtsH protease was found to have influence on the presence of the FtsZ rings at the mid-cell site. The Chapter 1 is the Introduction to the thesis presented in 3 parts –Part 1A, 1B, and 1C, introducing FtsZ and bacterial cell division, bacterial antisense RNAs, and FtsH protease, respectively. The Chapter 2 gives the description of the Materials and Methods used in the study. The Chapter 3 presents the identification, structural and functional characterisation of the ftsZ cis-antisense RNA, and its role in the regulation of FtsZ protein levels. Initially, the expression of cis-encoded antisense RNA from E. coli ftsZ loci was demonstrated during the different growth phases of the bacterium (RT-PCR/qPCR data). Antisense RNA is expressed from three promoters (primer extension and promoter probe data) on the complementary strand of the ftsZ coding region and terminates at the singletrand te complementary toftsAthegenethat 3’islocatedregionupstreamof theofftsZ the gene. Induced overexpression of a portion (423 bp) of the antisense RNA, spanning the ftsZ AUG codon and the ribosome binding site of ftsZ mRNA, from pBS(KS) could downregulate the synthesis of FtsZ protein to approximately 30%, leading to cell division arrest and filamentation of the cells at 42°C. This effect was less dramatic at 30ºC, probably due to less melting of the antisense RNA. Immunostaining performed on the induced culture did not show FtsZ ring formation after overnight induction whereas reduction in the proportion of the cells carrying FtsZ rings could be clearly observed after 2 hrs of induction. Real time PCR analysis performed for relative quantitation of ftsZ mRNA and ftsZas RNA from different growth phases (0.2 to 2.5 OD600 nm) showed growth phase dependent expression of the antisense RNA. While the levels of ftsZas RNA were found to be high at lower OD cultures or early growth phase cultures, the levels were found to be low at the late log phase and stationary phase cultures. Thus, when the cells are actively dividing and therefore need more FtsZ, the levels of the ftsZas RNA are high, while the cells are not actively dividing and therefore the FtsZ levels are low, the levels of the ftsZas RNA are low. At any phase of the growth, the ratio of the ftsZ mRNA to the ftsZas RNA was always found to be 6:1. Thus, the physiological role the ftsZas RNA is to maintain the availability of the ftsZ mRNA at a level that is commensurate with the requirement for the FtsZ protein during the different stages of the cell growth and division. The Chapter 4 is on the study of the possible mechanism behind the influence of FtsH protease on the presence of FtsZ rings at the mid-cell site during septation in cell division. Immunostaining for FtsZ in the mid-log phase E. coli cells showed that 82% of the AR3289 (ftsH wild type) cells possessed FtsZ rings, while only 18% of the AR3291 (ftsH-null maintained viable by a suppressor mutation) cells showed Z-rings. While the AR3289 cells showed a cell doubling time of 20 min, the AR3291 cells had a cell doubling time of 45 min. The mass doubling time of AR3289 and AR3291 were 24 min and 54 min, respectively. These distinct differences were found in spite of the suppressor mutation suppressing all the deleterious effects of the lack of the essential protease, FtsH. Complementation of the ftsH-null cells (AR3291) with the wild type FtsH but not with the ATP-binding or ATPase, or protease-defective mutants of FtsH, restored the FtsZ ring status to about 80% of the cells. The growth rate of AR3291 was also partly restored to comparable to that of the wild type cells upon complementation. Western blotting for FtsZ, and the FtsZ-stabilising proteins, FtsA and ZipA, showed that the ftsH-null cells have low levels of FtsA, as compared to those in the isogenic wild type cells (AR3289). The levels of FtsZ and ZipA were comparable in both the cells. Quantitative PCR performed for different cell division genes within the dcw cluster showed no sign of change in the ftsA transcript levels in the ftsH-null cells, suggesting that the low levels of FtsA in the ftsH-null cells were not due to transcriptional downregulation. Further experiments showed that the half-life of FtsA protein in the AR3289 cells was 45 min, while that in the AR3291 cells was 24 min. This experiment showed that the low levels of FtsA in the ftsH-null cells was due to the low half-life of FtsA in the cells. Growth synchronisation of the AR3289 and AR3291 cells showed that the levels of FtsA prior to cell division stage do not increase in the ftsH-null cells as much as in the isogenic wild type cells. Thus, the ftsH-null cells must be somehow managing the division through the partial stabilisation of FtsZ rings by ZipA. Interestingly, immunostaining for FtsH in AR3289 cells showed the presence of FtsH at the mid-cell site, as co-localised with FtsZ, for a brief period prior to cell constriction. These observations suggest the involvement of FtsH in cell division process. The faster degradation of FtsA in the absence of FtsH protease implies that another protein, which may be a protease that directly degrades FtsA or a chaperone that helps the unfolding of FtsA for degradation, might be the substrate of FtsH protease. The absence of FtsH protease brings up the levels of this unknown protein, which in turn facilitates (if it is a chaperone) degradation of or directly degrades (if it is a protease) FtsA. This model for the link among FtsH, FtsA levels, and the presence of FtsZ has been proposed based on the observations. Thus, the present study reveals for the first time an FtsA-linked role for FtsH protease in the presence of FtsZ ring at the mid-cell site and hence in bacterial septal biogenesis. The thesis is concluded with the list of salient findings, publications, and references. Bacterial Proteins Mycobacterium smegmatis - Bacterial Antisense RNAs Bacterial Cell Division FtsZ Antisense RNA FtsH Protease Bacterial Cell Septation FtsZ Rings Bacterial FtsH Protease Bacterial Septal Biogenesis ftsZ Gene Microbiology and Cell Biology
340	Un criblage ciblant de nouveaux facteurs impliqués dans l’assemblage mitotique des chromosomes dans le nématode C. elegans Ranjan, Rajesh 04 1900 (has links) La division cellulaire est un processus fondamental des êtres vivants. À chaque division cellulaire, le matériel génétique d'une cellule mère est dupliqué et ségrégé pour produire deux cellules filles identiques; un processus nommé la mitose. Tout d'abord, la cellule doit condenser le matériel génétique pour être en mesure de séparer mécaniquement et également le matériel génétique. Une erreur dans le niveau de compaction ou dans la dynamique de la mitose occasionne une transmission inégale du matériel génétique. Il est suggéré dans la littérature que ces phénomènes pourraient causé la transformation des cellules cancéreuses. Par contre, le mécanisme moléculaire générant la coordination des changements de haut niveau de la condensation des chromosomes est encore incompris. Dans les dernières décennies, plusieurs approches expérimentales ont identifié quelques protéines conservées dans ce processus. Pour déterminer le rôle de ces facteurs dans la compaction des chromosomes, j'ai effectué un criblage par ARNi couplé à de l'imagerie à haute-résolution en temps réel chez l'embryon de C. elegans. Grâce à cette technique, j'ai découvert sept nouvelles protéines requises pour l'assemblage des chromosomes mitotiques, incluant la Ribonucléotide réductase (RNR) et Topoisomérase II (topo-II). Dans cette thèse, je décrirai le rôle structural de topo-II dans l'assemblage des chromosomes mitotiques et ces mécanismes moléculaires. Lors de la condensation des chromosomes, topo-II agit indépendamment comme un facteur d'assemblage local menant par la suite à la formation d'un axe de condensation tout au long du chromosome. Cette localisation est à l'opposé de la position des autres facteurs connus qui sont impliqués dans la condensation des chromosomes. Ceci représente un nouveau mécanisme pour l'assemblage des chromosomes chez C. elegans. De plus, j'ai découvert un rôle non-enzymatique à la protéine RNR lors de l'assemblage des chromosomes. Lors de ce processus, RNR est impliqué dans la stabilité des nucléosomes et alors, permet la compaction de haut niveau de la chromatine. Dans cette thèse, je rapporte également des résultats préliminaires concernant d'autres nouveaux facteurs découverts lors du criblage ARNi. Le plus important est que mon analyse révèle que la déplétion des nouvelles protéines montre des phénotypes distincts, indiquant la fonction de celles-ci lors de l'assemblage des chromosomes. Somme toute, je conclus que les chromosomes en métaphase sont assemblés par trois protéines ayant des activités différentes d'échafaudage: topoisomérase II, les complexes condensines et les protéines centromériques. En conclusion, ces études prouvent le mécanisme moléculaire de certaines protéines qui contribuent à la formation des chromosomes mitotiques. / Cell division is a fundamental process that continuously happens in all living organisms. In each cell division, genetic material of the parent cell duplicates and segregates to produce genetically identical daughter cells in a process called mitosis. Cells need to condense their genetic material to be able to partition them equally. Any subtle defects, either timing or compaction level, could lead to the unequal inheritance of genetic material, a phenomenon that is believed to be the leading cause of cancerous transformation. However, the precise molecular mechanisms underlying the coordinated changes of higher-order chromosome structure are poorly understood. In the last two decades, various approaches have identified several conserved factors required for chromosome condensation. To define the roles of known and novel factors in this process, I performed an RNAi based screen using high-resolution live imaging of the C. elegans one-cell embryo. Importantly, using an in vivo approach, I discovered seven novel factors required for mitotic chromosome assembly, including Ribonulceotide reducatase (RNR) and DNA topoisomerase II (topo-II). In this thesis, I report a structural role for topo-II in mitotic chromosome assembly and underlying molecular mechanisms. During chromosome condensation process, topo-II acts independently as a local assembly factor leading to global chromosome axis formation, contradicting models that chromosomes organize around preassembled scaffolds, thus representing a novel pathway for chromosome assembly in C. elegans. Furthermore, I also discovered a non-enzymatic role of RNR in the mitotic chromosome assembly process. During this process, RNR is involved in nucleosome stability, and thereby, it allows higher-order chromatin assembly. In this thesis, I also report preliminary data for other novel factors that I discovered in the RNAi based screen for factors involved in chromosome condensation. Importantly, my analyses revealed that the depletion of several proteins results in distinct chromosome condensation phenotypes, indicating that they function in discrete events during mitotic chromosome assembly. In sum, I conclude that metaphase chromosomes are built by the distinct scaffolding activities of three proteins: DNA topoisomerase II, condensin complexes and centromere proteins. Taken together, these studies provide underlying molecular mechanisms contributing to the mitotic chromosome formation. Division Cellulaire Condensation des Chromosomes Ribonucléotide Réductase (RNR) Topoisomérase II (topo-II) Cell Division Chromosome Condensation Topoisomerase II (topo-II) Ribonucleotide Reductase (RNR)

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