Global ETD Search

31	Phase separation in giant vesicles Li, Yanhong January 2008 (has links) Giant vesicles may contain several spatial compartments formed by phase separation within their enclosed aqueous solution. This phenomenon might be related to molecular crowding, fractionation and protein sorting in cells. To elucidate this process we used two chemically dissimilar polymers, polyethylene glycol (PEG) and dextran, encapsulated in giant vesicles. The dynamics of the phase separation of this polymer solution enclosed in vesicles is studied by concentration quench, i.e. exposing the vesicles to hypertonic solutions. The excess membrane area, produced by dehydration, can either form tubular structures (also known as tethers) or be utilized to perform morphological changes of the vesicle, depending on the interfacial tension between the coexisting phases and those between the membrane and the two phases. Membrane tube formation is coupled to the phase separation process. Apparently, the energy released from the phase separation is utilized to overcome the energy barrier for tube formation. The tubes may be absorbed at the interface to form a 2-demensional structure. The membrane stored in the form of tubes can be retracted under small tension perturbation. Furthermore, a wetting transition, which has been reported only in a few experimental systems, was discovered in this system. By increasing the polymer concentration, the PEG-rich phase changed from complete wetting to partial wetting of the membrane. If sufficient excess membrane area is available in the vesicle where both phases wet the membrane, one of the phases will bud off from the vesicle body, which leads to the separation of the two phases. This wetting-induced budding is governed by the surface energy and modulated by the membrane tension. This was demonstrated by micropipette aspiration experiments on vesicles encapsulating two phases. The budding of one phase can significantly decrease the surface energy by decreasing the contact area between the coexisting phases. The elasticity of the membrane allows it to adjust its tension automatically to balance the pulling force exerted by the interfacial tension of the two liquid phases at the three-phase contact line. The budding of the phase enriched with one polymer may be relevant to the selective protein transportation among lumens by means of vesicle in cells. / In der wässrigen Lösung im Inneren von Riesenvesikeln können sich mehrere, räumlich getrennte Phasen ausbilden. Dieses Phänomen könnte im Zusammenhang stehen mit wichtigen Prozessen innerhalb von Zellen, wie etwa Fraktionierung und Sortieren von Proteinen, oder etwa das sog. “Molecular Crowding”. Wir studieren diesen Prozess am Beispiel von zwei unterschiedlichen Polymeren, Polyethylen Glycol (PEG) und Dextran, innerhalb von Riesenvesikeln. Die Dynamik der Phasentrennung dieser eingeschlossenen Polymerlösung lässt sich untersuchen, indem man die Vesikel einer hypertonischen Lösung aussetzt. Durch die Dehydrierung entsteht dabei überschüssige Membranfläche. Je nach Grenzflächenspannung zwischen den koexistierenden Phasen, sowie zwischen der Membran und den beiden Phasen, wird diese überschüssige Fläche entweder zur Ausbildung röhrchenartiger Strukturen verwendet, oder aber es stellen sich morphologische Veränderungen am Vesikel ein. Die Ausbildung der Membranröhrchen ist offenbar gekoppelt an den Phasentrennungsprozess: Die Energie, die bei Phasentrennung frei wird, dient offenbar dazu, die Energiebarriere der Röhrchenbildung zu überwinden. Die Röhrchen können an der Grenzfläche absorbiert werden und dort eine zweidimensionale Struktur ausbilden. Durch kleine Störungen in der Spannung kann die in Form von Röhrchen gespeicherte Membran wieder in deren Oberfläche zurückgezogen werden. Desweiteren wurde in diesem System ein Benetzungsübergang entdeckt, der bisher nur in wenigen experimentellen Systemen beobachtet werden konnte: Erhöht man die Polymerkonzentration, so geht die PEG-reiche Phase von vollständiger zu unvollständiger Benetzung der Membran über. Steht in einem Vesikel, in dem beide Phasen die Membran benetzen, ausreichend überschüssige Membranfläche zur Verfügung, so wird sich eine Phase aus dem Vesikelkörper herauswölben, was zur Trennung der beiden Phasen führt. Dieser benetzungsinduzierte Auswölbungsprozess wird durch die Oberflächenenergie bestimmt und von der Membranspannung moduliert. Dies konnte experimentell an Vesikeln gezeigt werden, die zwei Phasen beinhalten, indem durch eine Mikropipette ein Unterdruck erzeugt wurde. Die Oberflächenenergie kann durch Auswölbung einer der Phasen signifikant verringert werden, da die Kontaktfläche zwischen den koexistierenden Phasen verkleinert wird. Die Elastizität der Membran erlaubt es, die Spannung automatisch anzupassen, sodass die ziehende Kraft ausgeglichen wird, die durch die Grenzflächenspannung der beiden flüssigen Phasen an der drei-Phasen Kontaktlinie ausgeübt wird. Die Auswölbung einer durch Polymere angereicherten Phase könnte relevant sein für den selektiven Transport von Proteinen mit Vesikeln in der Zelle. Membranröhrchen Benetzungsübergang Knospung Vesikel Phasentrennung membrane tube wetting transition budding vesicle phase separation Physics
32	Deciphering the Role of Aft1p in Chromosome Stability Hamza, Akil 25 January 2012 (has links) The Saccharomyces cerevisiae iron-responsive transcription factor, Aft1p, has a well established role in regulating iron homeostasis through the transcriptional induction of iron-regulon genes. However, recent studies have implicated Aft1p in other cellular processes independent of iron-regulation such as chromosome stability. In addition, chromosome spreads and two-hybrid data suggest that Aft1p interacts with and co-localizes with kinetochore proteins, however the cellular implications of this have not been established. Here, we demonstrate that Aft1p associates with the kinetochore complex through Iml3p. Furthermore, we show that Aft1p, like Iml3p, is required for the increased association of cohesin with the pericentromere and that aft1Δ cells display sister chromatid cohesion defects in both mitosis and meiosis. Our work defines a new role for Aft1p in the sister chromatid cohesion pathway. Aft1 Iml3 kinetochore cohesion cohesin centromere chromosome stability Ctf19 Chl4 Scc1 mitosis meiosis Rec8 budding yeast
33	Deciphering the Role of Aft1p in Chromosome Stability Hamza, Akil 25 January 2012 (has links) The Saccharomyces cerevisiae iron-responsive transcription factor, Aft1p, has a well established role in regulating iron homeostasis through the transcriptional induction of iron-regulon genes. However, recent studies have implicated Aft1p in other cellular processes independent of iron-regulation such as chromosome stability. In addition, chromosome spreads and two-hybrid data suggest that Aft1p interacts with and co-localizes with kinetochore proteins, however the cellular implications of this have not been established. Here, we demonstrate that Aft1p associates with the kinetochore complex through Iml3p. Furthermore, we show that Aft1p, like Iml3p, is required for the increased association of cohesin with the pericentromere and that aft1Δ cells display sister chromatid cohesion defects in both mitosis and meiosis. Our work defines a new role for Aft1p in the sister chromatid cohesion pathway. Aft1 Iml3 kinetochore cohesion cohesin centromere chromosome stability Ctf19 Chl4 Scc1 mitosis meiosis Rec8 budding yeast
34	Identification of a Genetic Network in the Budding Yeast Cell Cycle / Identifiering av ett gennätverk i jästcellcykeln Fransson, Martin January 2004 (has links) By using AR/ARX-models on data generated by a nonlinear differential equation system representing a model for the cell-cycle control system in budding yeast, the interactions among proteins and thereby also to some extent the genes, are sought. A method consisting of graphical analysis of differences between estimates from two local linear models seems to make it possible to separate a set of linear equations from the nonlinear system. By comparing the properties of the estimations in the linear equations a set of approximate equations corresponding well to the real ones are found. A NARX model is tested on the same system to see whether it is possible to find the dependencies in one of the nonlinear differential equations. This approach did, for the choice of model, not work. Reglerteknik Genetic network Budding yeast cell Auto regression State-space model Reglerteknik Automatic control Reglerteknik
35	Characterization of four septin genes, and detection of genetic interactions between WdCDC10 and chitin synthase genes during yeast budding in the polymorphic mold, Wangiella (Exophiala) dermatitidis Park, Changwon 28 April 2015 (has links) Septins are a highly conserved family of eukaryotic proteins having significant homology within and among species. In the budding yeast, Saccharomyces cerevisiae, a septin-based hierarchy of proteins is required to localize chitin in the bud neck prior to septum formation. However, this process has not been clarified in a filamentous, conidiogenous fungus capable of yeast growth, such as Wangiella dermatitidis, a polymorphic agent of human phaeohyphomycosis. Prior studies of this melanized mold showed that some chitin synthase mutants (wdchsΔ) have defects in yeast septum formation, suggesting that the septins of W. dermatitidis might functionally associate with some of its chitin synthases (WdChsp). To test this hypothesis, four vegetative septin homologs of S. cerevisiae were cloned from W. dermatitidis and designated WdCDC3, WdCDC10, WdCDC11, and WdCDC12. Of the four, only WdCDC3 functionally complemented completely a strain of S. cerevisiae with a ts mutation in the corresponding gene, although WdCDC12 did so partially. Functional characterizations by mutagenesis of the four W. dermatitidis septin genes revealed that resulting mutants (wdcdc[delta]) each had unique defects in yeast growth and morphology, indicating that each septin carried out a distinct function. Furthermore, when a wdcdc10[delta] mutation was introduced into five different wdchs[delta] strains, weak genetic interactions were detected between WdCDC10 and WdCHS3 and WdCHS4, and a strong interaction between and WdCHS5. Cytological studies showed that WdChs5p was mislocalized in some septin mutants, including wdcdc10[delta]. These results confirmed that in W. dermatitidis septins are important for proper cellular morphogenesis, cytokinesis, and especially septum formation through associations with some chitin synthases. / text Septin genes Genetic interactions WdCDC10 Chitin synthase genes Yeast budding Wangiella (Exophiala) dermatitidis
36	Functional interactions of chromosome segregation factors with the 2 micron plasmid : possible evolutionary link between the plasmid portioning locus and the budding yeast centromere Huang, Chu-Chun 01 June 2011 (has links) The 2 micron plasmid of Saccharomyces cerevisiae is a multi-copy circular DNA genome that resides in the nucleus and exhibits nearly chromosome-like stability in host populations. Several host factors are required for equal plasmid segregation during cell division. One of them is cohesin (a multi-subunit protein complex) which mediates sister chromatid cohesion, a crucial mechanism for faithful segregation of replicated chromosomes in eukaryotes. The 2 micron plasmid mimics chromosomes in assembling cohesin at its partitioning locus. Studies on minichromosomes (centromere containing plasmids) reveal that cohesin forms a ring that embraces replicated sister centromeres topologically rather than physically. The functional similarities between chromosome and plasmid segregation prompted us to examine whether the topological mechanism proposed for centromere-mediated replicative cohesion is also true in the case of the plasmid. In the present study, we have characterized the nature and stoichiometry of cohesin's association with the 2 micron plasmid. Another host factor required for equal plasmid segregation is the CenH3 histone variant Cse4, so far considered to be uniquely associated with centromeric nucleosomes. Cse4 provides an epigenetic landmark at centromeres, and is required for assembly of the kinetochore complex. Surprisingly, Cse4 also interacts with the 2 micron plasmid partitioning locus. We have now functionally characterized this interaction, which can be preserved even in an ectopic, chromosomal context. The steady state level of Cse4 is highly limiting in yeast due to ubiquitin-mediated proteolysis. Only centromere-associated Cse4 is protected from this regulatory turnover control. We find that, in contrast to the situation with centromeres, association of Cse4 with the 2 micron plasmid is highly sub-stoichiometric but still promotes equal plasmid segregation. We also find that Cse4 induces an unusual right handed DNA writhe at the plasmid partitioning locus, as it does at the centromere. Our findings suggest that the plasmid has designed strategies to minimize the utilization of host factors that are in short supply. They signify the advantage of clustering and group behavior in the evolutionary success of a multi-copy selfish genome. Finally, they also suggest the possible emergence of the yeast centromere and the plasmid partitioning locus from a common ancestral sequence. / text Plasmid segregation Chromosome segregation Selfish DNA Budding yeast Saccharomyces Cohesin Cse4 Centrosomes Plasmids
37	Formation of Dicentric and Acentric Chromosomes, by a Template Switch Mechanism, in Budding Yeast Paek, Andrew Luther January 2010 (has links) Chromosomal rearrangements occur in all organisms and are important both in the evolution of species and in pathology. In this dissertation I show that in Saccharomyces cerevisiae, or budding yeast, one type of chromosomal rearrangement occurs when inverted repeats fuse, likely during DNA replication by a novel mechanism termed "faulty template switching". This fusion can lead to the formation of either a dicentric or acentric chromosome, depending on the direction of the replication fork. Dicentric chromosomes are inherently unstable due to their abnormal number of centromeres, and thus undergo additional chromosomal rearrangements and chromosome loss. Acentric Chromosomes Budding Yeast Dicentric Chromosomes Genome Instability Inverted Repeats Template Switching
38	Initiating the Spindle Assembly Checkpoint Signal: Checkpoint Protein Mad1 Associates with Outer Kinetochore Protein Ndc80 in Budding Yeast Weirich, Alexandra 14 June 2013 (has links) The spindle assembly checkpoint (SAC) is an evolutionarily conserved mechanism that delays the initiation of anaphase by inhibiting the Anaphase Promoting Complex (APC) until all kinetochores have achieved bipolar attachment on the mitotic spindle. Mad1-3, Bub1, and Bub3, components of the SAC, are conserved from yeast to humans. These proteins localize to unattached kinetochores, though it is unknown with which kinetochore proteins they interact and how these interactions transduce information about microtubule attachement. Here, purification of the checkpoint proteins from Saccharomyces cerevisiae suggests that Mad1 interacts with the outer kinetochore protein Ndc80 in a SAC, cell cycle, and DNA dependent manner. Ndc80 is thought to mediate attachment of kinetochores to microtubules so the interaction between Mad1 and Ndc80 suggests a mechanism by which cells sense kinetochore-microtubule attachment. The SAC is of special importance in some types of cancer where genetic damage and aneuploidy is correlated with mutated SAC genes. A better understanding of the SAC mechanism will aid in the development of targetted cancer therpeutics. protein purification anaphase promoting complex spindle assembly checkpoint Mad1 Ndc80 Budding Yeast mass spectrometry
39	Deciphering the Role of Aft1p in Chromosome Stability Hamza, Akil 25 January 2012 (has links) The Saccharomyces cerevisiae iron-responsive transcription factor, Aft1p, has a well established role in regulating iron homeostasis through the transcriptional induction of iron-regulon genes. However, recent studies have implicated Aft1p in other cellular processes independent of iron-regulation such as chromosome stability. In addition, chromosome spreads and two-hybrid data suggest that Aft1p interacts with and co-localizes with kinetochore proteins, however the cellular implications of this have not been established. Here, we demonstrate that Aft1p associates with the kinetochore complex through Iml3p. Furthermore, we show that Aft1p, like Iml3p, is required for the increased association of cohesin with the pericentromere and that aft1Δ cells display sister chromatid cohesion defects in both mitosis and meiosis. Our work defines a new role for Aft1p in the sister chromatid cohesion pathway. Aft1 Iml3 kinetochore cohesion cohesin centromere chromosome stability Ctf19 Chl4 Scc1 mitosis meiosis Rec8 budding yeast
40	Caractérisation structurale de la régulation de l'ubiquitine-hydrolase AMSH / Structural basis for AMSH ubiquitine hydrolase regulation Poudevigne, Emilie 24 September 2013 (has links) La voie endo-lysosomale dirige les récepteurs membranaires vers le processus de dégradation lysosomale. En bref, les récepteurs sont marqués par l'ubiquitine, envoyés vers les endosomes précoces puis, pris en charge pas le système ESCRT (Endosomal Sorting Complexes Required for Transport) et intégrés dans des vésicules intraluminales. Ce système est composé des complexes ESCRT-0, I, II, II et VPS4. Certaines protéines ESCRT sont aussi recrutées lors de processus topologiquement similaires comme la cytokinèse ou le bourgeonnment viral de certains virus enveloppés. AMSH (Associated Molecule of the SH3 domain of STAM) est une ubiquitine-hydrolase associée au système ESCRT qui hydrolyse les chaînes d'ubiquitine liées par leur lysine K63. Elle interagit directement avec ESCRT-0 via la sous-unité STAM et avec les membres CHMP1A, 1B et 3 d'ESCRT-III. Bien qu'AMSH pourait recruter ces protéines ESCRT ou être elle-même recrutée par celles-ci, le mécanisme d'activation de son activité d'hydrolase est encore méconnu. Afin de mieux comprendre les bases structurales de l'activation d'AMSH, j'ai essayé danalyser des formes recombinantes de cette protéine par cristallographie aux rayons X et par diffusion des rayons X aux petits angles (SAXS) ce qui m'a permis d'obtenir deux modèles à basse résolution. De plus, j'ai caractérisé par SPR (Surface Plasmon Resonance) les interactions entre AMSH et CHMP1A, 1B et 3 et déterminé les résidus clefs du dernier complexe. Cela a montré que les surfaces d'interaction employées par le domaine MIT d'AMSH ne sont pas les mêmes pour CHMP3 et CHMP1A/1B. J'ai aussi découvert que l'activité enzymatique d'AMSH seule est très faible ce qui impliquerait une auto-inhibition en solution. L'hydrolyse des chaînes d'ubiquitine liées par leur lysine K63 pourrait alors être activée par une construction de STAM comprenant le domaine SH3 ainsi que les domaines liant l'ubiquitine VHS et/ou UIM. / The endosomal pathway targets plasma membrane receptors for lysosomal degradation. Briefly, receptors are tagged by an ubiquitin, delivered to the early endosome and sorted into intraluminal vesicles by the ESCRT (Endosomal Sorting Complexes Required for Transport) machinery, composed of ESCRT-0, -I, -II- -III and the VPS4 complex. Some ESCRts are also recruited during topologically similar processes such as cytokinesis and budding of some enveloped viruses. AMSH (Associated Molecule of the SH3 domain of STAM) is an ESCRT associated ubiquitin-hydrolase which hydrolyses K63-linked ubiquitin chains. AMSH interacts directly with the ESCRT-0 subunit STAM and ESCRT-III members CHMP1A, CHMP1B and CHMP3. Although AMSH may either recruit these ESCRTs are maybe recruited by these ESCRTs, little is known about the activation mechanism of its hydrolase activity. In order to understand the structural basis for AMSH activation I attempted to analyze recombinant forms of AMSH by X-ray crystallography and SAXS, which produced low resolution models of AMSH. I further characterized AMSH interactions with CHMP1A, CHMP1B and CHMP3 by SPR and determined the key residues for interaction. This showed that the AMSH MIT domain employs two different surfaces for CHMP3 and CHMP1A/B interactions. I also found that recombinant AMSH has very poor enzymatic activity on its own, which indicates an auto-inhibited state in solution. K63-linked uibiquitin hydrolysis could be activated by STAM constructs containing the SH3 and ubiquitin binding domains (UIM and/or VHS), which were shown to interact directly with AMSH via SPR. Thus activation of the hydrolase activity by STAM corroborates indirectly the autoinhibited native state. Cristallographie Bourgeonnement viral Ubiquitine hydrolase Système ESCRT Ubiquitine hydrolase Cristallography Viral budding Escrt machinary

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