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Transcriptional Regulation of the Glycogen Phosphorylase-2 Gene in <I>Dictyostelium discoideum</i>Warner, Nikita 25 September 1999 (has links)
The expression of the <I>glycogen phosphorylase- 2</I> gene (<I>gp2</I>) is initiated during early development and regulated by the extracellular morphogens cAMP and Differentiation Inducing Factor (DIF-1) [1-3]. Glycogen phosphorylase- 2 catalyzes the breakdown of glycogen reserves in developing cells to generate glucose precursors required for the synthesis of the end products of differentiation [4-6]. Thus, the expression of <I>gp2</I> is a significant event for cellular differentiation. The sequence of the <I>gp2</I> promoter, like other <I>Dictyostelium</I> promoters, has an AT-rich bias (88%) [7]. Previous deletional analyses of the promoter provided a map of the regions that contained transcriptional regulatory elements. The regions thus identified contained either "TAAAAATGGA" or C-rich repeat sequences [2]. These regions were dissected further by site-directed mutagenesis (SDM) to better define the physical boundaries of the regulatory elements. It was shown that the mutation of either one of the C-rich repeats resulted in a dramatic drop of about 95% in reporter gene levels. These data strongly suggested that both the C-rich repeats of <I>gp2</I> functioned as transcriptional regulatory elements. I have identified and purified a factor called TF2 that demonstrates a high specificity for a C-rich transcriptional regulatory element, the 5' C box. TF2 was first detected with electrophoretic mobility shift assays of DEAE chromatographic fractions of cell-free extracts. The specificity of TF2 for the 5' C box was tested by competition analysis using six other oligonucleotides. Purification of TF2 was achieved by ion-exchange chromatography, DNA affinity chromatography, gel filtration chromatography, and preparative SDS-PAGE. SDS-PAGE analysis indicated an apparent subunit molecular weight of 28 kDa. The apparent molecular weight of the native protein as estimated by gel filtration was about 53 kDa. This suggested that TF2 binds gp2 as a homodimer. A cDNA clone of the tf2 gene was provided by the Japanese <I>Dictyostelium</I> cDNA project. This allowed me to synthesize probes for Southern and Northern blot analyses. Southern blot analysis indicated that there is only one form of the <I>tf2</I> gene. Northern analysis showed little or no expression of <I>tf2</I> in undifferentiated cells. During development <I>tf2</I> expression increases up to a maximum at 8 h, then decreases in later stages. Attempts to disrupt the gene suggest that <I>tf2</I> mutation may be lethal. / Ph. D.
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Generation of cDNA libraries of amoeba, 8 hour, and 12 hour stages of Dictyostelium discoideumChanchao, Chanpen 18 November 2008 (has links)
A critical event during the life cycle of Dictyostelium discoideum is glycogen turnover. This process is catalyzed by glycogen phosphorylase-2 (gp-2). Since gp-2 expression is first induced during the transition from growth to differentiation, understanding how this gene is controlled may provide some insight into the process of differentiation. In order to identify the trans-acting factors responsible for activating gp-2 expression, cDNA plasmid libraries of amoebae, and cells at 8 h and 12 h of development were generated. The long-term goals of this project involve screening expression libraries with identified cis-acting elements from the gp-2 promoter to yield the DNA binding proteins responsible for gene regulation. For this approach to succeed, a high-quality cDNA library is essential. The library must contain full-length cDNA that represents the complexity of mRNA present during the developmental stage of interest. Hence, all three libraries were subjected to extensive testing prior to and following cloning. RNA quality and the fidelity of the time points were determined by Northern blot analysis and by RTPCR for several marker genes. Following cDNA synthesis, the cDNA was assessed for complexity and full-length synthesis by PCR and radioactive primer extension, respectively. Ligation of the cDNA into a vector was performed using several ratios of vector:insert in order to ensure that long cDNA species were included in the plasmid library. Finally, the presence of the marker genes was confirmed by PCR amplification of plasmid extracted from bacteria transformed with the plasmid library. / Master of Science
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Cloning and Characterization of Replication Protein A from Dictyostelium discoideumWen, Xiao 08 May 1997 (has links)
The gene encoding the Dictyostelium replication protein A large subunit (DdRPA1) has been cloned by screening of an EcoR I partial genomic library and a Hind III genomic sub-library. The complete nucleotide sequence, including the promoter region of the gene has been obtained by sequencing. Though the DdRPA1 protein has a size shift during development, 62 kDa in undifferentiated cells and 81 kDa in differentiated cells; they are the products of the same gene. Northern blot analysis revealed that the expression level of the DdRPA1 was constant throughout differentiation and the size of mRNA is the same at all stages, corresponding to a 81 kDa protein. Thus, it seems that the size change between the 62 kDa and 81 kDa is probably due to posttranslational modification, most likely, proteolytic cleavage. The transcription start site for both sizes of DdRPA1 has been identified at 306 bp upstream of the coding sequence by primer extension reaction.
A PCR fragment representing 27% of the gene encoding the DdRPA middle size subunit (DdRPA2) has been generated by using the degenerate primers. This PCR fragment has been cloned and sequenced. The mRNA for this subunit corresponds to a protein of about 35 kDa. A decrease of the DdRPA2 mRNA expression level during differentiation was found by comparison between undifferentiated and differentiated cells.
In Dictyostelium, replication protein A is a heterotrimeric protein that can bind with specific DNA sequences in a stage-dependent pattern. These DNA sequences were identified as the cis-acting regulatory sites in differentiation-related genes, including the glycogen phosphorylase 2 gene (gp2). Therefore, it is possible that DdRPA is not only a single-stranded DNA binding protein that is used in multiple essential DNA metabolic processes, such as DNA replication, repair and recombination in undifferentiated cells, but also involved in the transcriptional regulation process during differentiation. / Master of Science
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Cellular Sorting of the Dictyostelium discoideum SlugFlowerday, Erin 07 August 2024 (has links) (PDF)
Dictyostelium discoideum (Dd) cells are amoeba cells that feed on soil or plant leaf matter bacteria. They divide freely in the presence of food. When starved, cell division is ended, and cells transition from unicellular to multicellular organisms initiated by a chemoattractant, cyclic adenosine monophosphate (cAMP). This study intricately examines cellular sorting within the Dd slug, focusing on individual cell dynamics. Represented as oriented ellipsoids, these cells maintain constant volume through a viscoelastic structure. Applying force to specific semi-axes reveals predictable deformations, highlighting the relationship between force and deformation rate. Manipulating damping coefficients and spring constants uncovers insights into cell viscosity and stiffness. Exploring the effects of a cell's active force and cone angle revealed that a cone angle less than 10 degrees or greater than 30 degrees and an active force less than 2N or greater than 6N of the prestalk cells led to unsatisfactory conditions, resulting in insufficiently directed cell movement, and an inability to achieve the desired cell sorting patterns within the slug. This work guides exploring diverse cellular behaviors, advancing the understanding of complex biological phenomena within a concise framework.
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The Dictyostelium discoideum RACK1 orthologue has roles in growth and developmentOmosigho, N.N., Swaminathan, Karthic, Plomann, M., Müller-Taubenberger, A., Noegel, A.A., Riyahi, T.Y. 28 February 2020 (has links)
Yes / Background: The receptor for activated C-kinase 1 (RACK1) is a conserved protein belonging to the WD40 repeat
family of proteins. It folds into a beta propeller with seven blades which allow interactions with many proteins. Thus
it can serve as a scaffolding protein and have roles in several cellular processes.
Results: We identified the product of the Dictyostelium discoideum gpbB gene as the Dictyostelium RACK1 homolog.
The protein is mainly cytosolic but can also associate with cellular membranes. DdRACK1 binds to phosphoinositides
(PIPs) in protein-lipid overlay and liposome-binding assays. The basis of this activity resides in a basic region located in
the extended loop between blades 6 and 7 as revealed by mutational analysis. Similar to RACK1 proteins from other
organisms DdRACK1 interacts with G protein subunits alpha, beta and gamma as shown by yeast two-hybrid, pulldown, and immunoprecipitation assays. Unlike the Saccharomyces cerevisiae and Cryptococcus neoformans RACK1
proteins it does not appear to take over Gβ function in D. discoideum as developmental and other defects were not
rescued in Gβ null mutants overexpressing GFP-DdRACK1. Overexpression of GFP-tagged DdRACK1 and a mutant
version (DdRACK1mut) which carried a charge-reversal mutation in the basic region in wild type cells led to changes
during growth and development.
Conclusion: DdRACK1 interacts with heterotrimeric G proteins and can through these interactions impact on
processes specifically regulated by these proteins. / This work was supported by the DFG and SFB670. TYR acknowledges support from the Professorinnen Program of the University of Cologne.
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Regulation of glycogen phosphorylase genes in Dictyostelium discoideumSucic, Joseph F. 06 June 2008 (has links)
The cellular slime mold, Dictyostelium discoideum, provides an ideal model system to study eukaryotic development, cell differentiation, and aging. A crucial developmental event in Dictyostelium is glycogen degradation. The degradation of glycogen provides glucose monomers that are used to synthesize structural components necessary for cellular differentiation. Glycogen degradation is catalyzed by glycogen phosphorylase, and two developmentally regulated glycogen phosphorylase activities have been discovered in Dictyostelium. Glycogen phosphorylase 1 (gp-1) activity is predominant early in development, and is dependent upon 5’ AMP as a positive allosteric modifier; glycogen phosphorylase 2 (gp-2) activity peaks late in development and is independent of 5° AMP. I showed that these two glycogen phosphorylase activities are associated with unique proteins that are the products of two distinct, but related, genes. Both genes were observed to be typical Dictyostelium genes in a number of respects. The gp-1 and gp-2 enzymes were also found to be similar to glycogen phosphorylases from other organisms. I also examined the developmental expression of these genes and found that both mRNAs are developmentally regulated; gp-1 mRNA levels fluctuate during development, while gp-2 mRNA levels increase late in development. The expression of the gp-1 and gp-2 genes is regulated by exogenous cAMP. Exogenous cAMP enhances the level of gp-1 mRNA, apparently through a mechanism that requires intracellular cAMP signaling. Specific DNA sequence elements appear to be required for maximal vegetative and late developmental expression of gp-1. Exogenous cAMP induces the appearance of gp-2 mRNA via a mechanism that appears to be independent of intracellular cAMP signaling. Repeated TA-rich sequences located between nucleotides 193 and 305 upstream of the transcriptional start site are necessary for maximal cAMP induction of gp-2. I also examined the cell type specific expression of gp-1 and gp-2. gp-1 is expressed predominantly in pre-stalk cells. gp-2 1s expressed in both cell types in a temporally regulated fashion; this type of expression has not been reported for other Dictyostelium genes, but, given the importance of glycogen degradation in both stalk and spore cells, it is not inconceivable that such regulation 1s necessary. / Ph. D.
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Caractérisation des corps multilamellaires sécrétés par Dictyostelium discoideumPaquet, Valérie 19 April 2018 (has links)
Les amibes sont des eucaryotes unicellulaires qui ingèrent des bactéries par phagocytose pour se nourrir. Les proies sont dégradées au cours de la maturation des phagosomes. Cependant, certaines bactéries pathogènes intracellulaires résistent à la phagocytose. Dans l'amibe, les bactéries acquièrent un enrobage multilamellaire protéolipidique provenant de la cellule hôte appelé corps multilamellaires (CML). Une fois exocytées, les bactéries enrobées sont plus résistantes à divers stress. À ce jour, le mécanisme d'enrobage bactérien reste toujours nébuleux. En utilisant l'amibe modèle Dictyostelium discoideum, il a été possible de reproduire la formation de CML et de les analyser en microscopie. Par la création d'un protocole de production et de purification des CML, les protéines totales ont été extraites des structures puis analysées par spectrométrie de masse. Plus de 24 protéines ont été identifiées comme composantes des CML. L'identification de ces protéines va permettre de mieux comprendre le mécanisme d'enrobage bactérien.
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Dynamique de la formation des corps multilamellaires et de l'enrobage de bactéries par différents protozoairesDurocher, Alicia 27 January 2024 (has links)
Plusieurs protozoaires, des eucaryotes unicellulaires ubiquitaires, sont des prédateurs de bactéries. Cependant, les relations bactéries-protozoaires sont complexes et peuvent donner lieu à des interactions particulières. Certains protozoaires, dont l’amibe sociale Dictyostelium discoideum, peuvent produire des corps multilamellaires (CML) lorsqu’ils digèrent des bactéries. Ces structures avaient initialement été identifiées comme des déchets métaboliques, mais il a été suggéré qu’elles pourraient avoir des rôles supplémentaires. Ce ne sont pas toutes les bactéries qui sont digérées par tous les protozoaires, et certaines bactéries résistantes à la digestion peuvent être enrobées dans les corps fécaux de ces protozoaires. Les corps fécaux partagent des similitudes avec les CML. Ce projet de maîtrise visait à éclairer certains aspects des interactions bactéries protozoaires,en caractérisant la voie phagocytique d’amibes sociales environnementales afin d’examiner leur production potentielle de CML, et en analysant l’impact de différentes caractéristiques bactériennes sur la morphologie de l’enrobage par des ciliés. Ces objectifs furent atteints en cultivant les protozoaires d’intérêt en présence de bactéries digestibles(pour la production de CML) ou non (pour l’enrobage) et en faisant appel à diverses méthodes de microscopie. Nos résultats montrent que les quatre isolats d’amibes sociales environnementales, qui appartiennent tous au genre Dictyostelium, mais qui présentent des caractéristiques différentes, peuvent produire des CML lorsque cultivés sur bactéries digestibles. Pour l’étude de la morphologie de l’enrobage de bactéries, les résultats suggèrent que l’hydrophobicité de surface et la taille de l’espèce bactérienne seraient les caractéristiques ayant le plus fort impact sur la morphologie des corps fécaux. Toutefois, il n’est pas exclu que d’autres facteurs interviennent également, incluant des facteurs qui n’étaient pas à l’étude dans ce projet. Ces résultats approfondissent notre compréhension des relations bactéries-protozoaires, mais de nombreuses autres questions sont toujours sans réponse et le développement de méthodes d’analyse plus raffinées sera primordial pour répondre à ces questions. / Many protozoa, ubiquitous unicellular eukaryotes, are predators of bacteria. However, bacteria-protozoa relationships are complex and can lead to some particular interactions. Some protozoa, including the social amoeba Dictyostelium discoideum, can produce multilamellar bodies (MLBs) upon digesting bacteria. These structures were initially identified as metabolic waste, but it has been suggested that they could have additional roles. Not all bacteria can be digested by all protozoa, and some digestion-resisting bacteria can be packaged into the fecal bodies produced by protozoa. These fecal bodies share similarities with MLBs. This master’s project was meant to shed a light on some aspects of bacteria-protozoa interactions, by characterizing the phagocytic pathway of some environmental social amoebae and by analyzing the impact of bacterial characteristics on the morphology of bacteria packaging. These objectives were met by cultivating the protozoa species of interest with either digestible bacteria (for MLB production) or undigestible bacteria (for packaging) and using diverse microscopy methods. Our results show that the four environmental isolates of social amoebae, belonging to the Dictyostelium genus but presenting distinct characteristics, can produce MLBs upon growth on digestible bacteria. As for the study of bacteria packaging morphology, results suggest that a bacteria’s surface hydrophobicity and cell size are the characteristics impacting packaging morphology the most. However, it is not excluded that other factors may intervene as well, including some not considered in this project. These results bring new understanding to bacteria protozoa relationships, but many questions remain. The development of more refined analysis method will be paramount to answering these.
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Análise do perfil de expressão de serina/treonina fosfatases e prospecção da função biológica para algumas dessas enzimas em Dictyostelium discoideum / Analysis of serine/threonine phosphatases expression profile and biological function prospection for some of these enzymes in Dictyostelium discoideumMartins, Layla Farage 13 December 2010 (has links)
A fosforilação reversível de proteínas em resíduos de serina e treonina, catalisada por quinases e fosfatases desempenha papel chave na regulação do crescimento e na diferenciação celular em eucariotos. As serina/treonina proteínas fosfatases (PSTPs) são atualmente divididas em três famílias denominadas PPP (PhosphoProtein Phosphatase), PPM (Phosphoprotein Phosphatase Magnesium-dependent) e FCP/SCP (RNA polymerase II CTD phosphatase), sendo que os membros da família PPP são, frequentemente, holoenzimas compostas de uma subunidade catalítica associada a uma ou mais subunidades reguladoras, as quais definem a função, localização e especificidade ao substrato da fosfatase. Neste trabalho, analisamos, através de RT-qPCR, o perfil de expressão dos genes codificadores de subunidades catalíticas de PPPs de Dictyostelium discoideum (PP1c, PP2Ac, PP4c, PP4c-like, PP6c e PP5c) e de 16 potenciais parceiros moleculares de algumas destas subunidades catalíticas, tais como DdI-2 e DdI-3, sabidamente inibidores da PP1c. Em resposta ao estresse térmico de células da fase de crescimento, detectamos o aumento dos níveis de transcritos de PP4c e PP6c e também de DdI-2, DdI-3 e DDB_G0292194, esta última, uma proteína de função desconhecida que interage com a PP1c em ensaios de duplo-híbrido em leveduras. Por outro lado, durante o estresse hiper-osmótico observamos a diminuição dos níveis de transcritos de quase todos os genes analisados com exceção de DdI-2 e DDB_G0292194. O nível de expressão de DdPP1c, DdI-2, DdI-3 e DDB_G0292194 também foi analisado em resposta ao estresse oxidativo e apenas o DDB_G0292194 foi induzido nesta condição. Os genes de PP1c, PP4, PP5c e PP6c são expressos durante todo o ciclo de vida de D. discoideum, mas a expressão de alguns dos genes analisados aumenta em uma fase definida do ciclo de desenvolvimento como é o caso de DDB_G0292194 que tem níveis de transcritos aumentados na fase de agregação. Este gene codifica uma proteína hipotética de 559 aminoácidos, que apresenta um domínio FHA (ForkHead-Associated) em sua região aminoterminal, além de uma sequência similar ao motivo consenso de ligação à PP1c. Ensaios no sistema de duplo-híbrido em leveduras confirmaram que a interação entre DDB_G0292194 e DdPP1c independe do domínio FHA. Verificamos, também, que o mutante nocaute de DDB_G0292194 apresenta uma morfologia alterada em condições padrões de cultivo, tanto na fase de crescimento como durante o desenvolvimento, além de uma maior sensibilidade ao estresse oxidativo causado pelo peróxido de hidrogênio quando comparado à linhagem selvagem. Em conjunto, nossos resultados evidenciam a importância das PPPs na resposta a diferentes tipos de estresse e para o crescimento e desenvolvimento de D. discoideum. / Reversible phosphorylation of proteins on serine and threonine residues, catalyzed by kinases and phosphatases plays a key role in growth and cell differentiation regulation in eukaryotes. Protein serine/threonine phosphatases (PSTPs) are currently divided into three families named PPP (Phosphoprotein Phosphatase), PPM (Phosphoprotein Phosphatase Magnesium-dependent) and FCP/SCP (RNA polymerase II CTD phosphatase). The PPP family members are often holoenzymes composed of a catalytic subunit associated with one or more regulatory subunits, which define function, localization and substrate specificity of the phosphatase. In this work, we have examined, by RT-qPCR, the expression profile of genes encoding PPP catalytic subunits of Dictyostelium discoideum (PP1c, PP2Ac, PP4c, PP4c-like, PP6c and PP5c) and 16 potential molecular partners for some of these catalytic subunits, such as DdI-2 and DdI-3, both known as PP1c inhibitors. In response to heat stress of growth phase cells, we detected increased levels of transcripts of PP4c and PP6c as well as of DdI-2, DdI-3, and DDB_G0292194, the latter a protein of unknown function that interacts with PP1c in yeast two-hybrid assays. Moreover, during the hyperosmotic stress we observed decreased transcript levels of nearly all genes examined except DdI-2 and DDB_G0292194. The expression level of DdPP1c, DdI-2, DdI-3 and DDB_G0292194 was also analyzed in response to oxidative stress and only DDB_G0292194 was induced in this condition. PP1c, PP4c, PP5c and PP6c genes are expressed throughout growth and development of D. discoideum while transcript levels of some the analysed genes were increased at a defined stage of the developmental cycle as in the case of DDB_G0292194, which increased during aggregation. This gene encodes a hypothetical protein of 559 amino acids bearing a FHA (ForkHead-Associated) domain in its aminoterminal region and a sequence matching the PP1c binding consensus motif. Yeast two-hybrid assays confirmed that DDB_G0292194 and DdPP1c interaction does not depend on FHA domain. We also found that DDB_G0292194 knockout mutant exibits an altered morphology on standard growth and developmental conditions and shows an increased sensitivity to oxidative stress induced by hydrogen peroxide in comparison to the wild type strain. Taken together, our results highlight the importance of PPPs in the response to different types of stress and for growth and development of D. discoideum.
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Directional sensing and chemotaxis in eukaryotic cells - a quantitative study / Directional Sensing und Chemotaxis eukaryotischer Zellen - eine quantitative StudieAmselem, Gabriel 13 October 2010 (has links)
No description available.
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