Investigation on the Physiological and Pathological Aspects of the Proline-Rich Region of the Microtubule-Associated Protein Tau

Savastano, Adriana

13 December 2019

No description available.

570

Tauopathies

Microtubules

LLPS

ssNMR

NMR

Phosphorylation

Pathological role

Alzheimer´s Disease,

Tau

Neurodegeneration

Structural biology

Nuclear Magnetic resonance

Biologie (PPN619462639)

Optical 3D-Nanometry to Study the Function of Biomolecular Motors in Nanotransport

Nitzsche, Bert

18 December 2008

A major challenge in nanotechnology is the controlled transport of cargo on the nanometer scale. A promising approach to this problem is the use of molecular motors of the cellular cytoskeleton. The aim of this work was to develop a method to characterize the behavior of filamentous nanoshuttles – specifically of motor protein-driven microtubules – in three dimensions (3-D). The main requirements to meet were low impact on the nanotransport system, high spatial and temporal resolution, and versatility. Furthermore, this method was intended to be used to address open questions in the field of nanotransport. In particular, it was firstly attempted to characterize cargo transport in a system currently favored by most studies in the field, where nanoshuttles are powered by the microtubule motor best understood so far – the plus-end-directed kinesin-1. Secondly, the goal was to further the understanding of potential counter-players of kinesin-1 in nanotransport applications - the much less well understood microtubule minus-end-directed motor proteins 22S dynein and the kinesin-14 non-claret disjunctional (ncd). A novel method to study the linear forward motion as well as the axial motion of filamentous nanoshuttles, which are driven by motors of the cell cytoskeleton, has been introduced. The method uses fluorescence interference-based 3-D nanometer tracking of quantum dots as optical probes that are attached to the nanoshuttles. While other recently reported 3-D tracking techniques based on dual-focus imaging offer similar sensitivity, the method here can be easily performed on any standard epi-fluorescence microscope, even with arc lamp illumination, and additionally holds the potential to retrieve absolute height values. It is strongly suggested that the ease of use might help to spread this valuable and versatile tool for a variety of applications, including studies of interactions between single molecules or even intramolecular changes. Specifically, 3-D tracking has been used to visualize and analyze the rotation of microtubules around their longitudinal axis when they are propelled on a motor protein-coated surface. This geometry called gliding assay is currently favored for most proof-of-principle studies that investigate the use of biomolecular motors for transport of nanoscale cargo with the goal to assemble and manipulate nanostructures. The suitability of the method has been proven for kinesin-1 gliding assays, where knowledge of properties of both, microtubules and kinesin-1, allowed a very precise prediction of microtubule rotation, which was matching the actual measured values very well. The microtubule rotation in kinesin-1 gliding assays has turned out to be robust against the attachment of small cargo in the shape of quantum dots (diameter ∼20 nm), but also against the reduction of electrostatic interactions between microtubules and kinesin-1 by cleavage of the tubulin E-hook. The situation was dramatically different when large cargo (beads with diameter of ∼3 µm) was attached to microtubules. In this case, filament rotation was stopped, but otherwise the impact on motility was surprisingly low. In particular, the velocity of the gliding microtubules only decreased to a negligible degree. This shows that in principle microtubules driven by processive motors like kinesin-1 can make flexible, responsive and effective molecular shuttles for nanotransport applications. In addition, the results might indicate that in vivo kinesin-1 molecules, which transport cargo along microtubules, can likewise flexibly respond to an axial force by deviating from their path parallel to the protofilament axes. Two microtubule minus-end-directed motors that might be employed to counteract kinesin-1 in engineered nanotransport systems are dynein and ncd. Both motors have been found to be capable of generating torque causing short-pitched microtubule rotation in gliding motility assays. The results for 22S dynein helped to resolve controversial findings of earlier reports about the ability of 22S dynein to generate torque. However, it turned out difficult to establish conditions where the movement of the dynein-driven nanoshuttles was homogeneous and reproducible. In contrast, motility in ncd gliding assays looks much more promising. The obtained results supported previous reports of torque generation by ncd. Moreover, a strong dependence of rotational pitches of gliding microtubules on ATP concentration was found. The reason could be that ncd motors in the nucleotide-free microtubule-bound state impede the forward movement of gliding microtubules stronger than the axial motion. To fully understand the nature of this effect, further research is required. Most likely, this will substantially contribute to the understanding of ncd function in vivo. Furthermore, the possibility of tuning the rotation of microtubules acting as nanoshuttles might provide a means to increase control of processes like cargo-loading and unloading. / Eine große Herausforderung auf dem Gebiet der Nanotechnologie ist der kontrollierte und präzise Transport von nanoskaligen Objekten. Der Einsatz von molekularen Motoren des zellulären Zytoskeletts hat sich dabei als vielversprechender Ansatz erwiesen. Ziel der hier vorgelegten Arbeit war die Entwicklung einer Methode, um das Verhalten von filamentartigen Nanotransportern - speziell von Mikrotubuli, die durch Motorproteine über Oberflächen bewegt werden - in drei Dimensionen (3-D) zu charakterisieren. Die Hauptkriterien waren dabei eine geringe Störung des zu untersuchenden Systems, hohe räumliche und zeitliche Auflösungen sowie die generelle Anwendbarkeit für Einzelmolekülstudien. Ein weiteres Ziel war es, die entwickelte Methode zur Beantwortung offener Fragen bezüglich des Nanotransports mittels Zytoskelett-basierter Motoren einzusetzen. Insbesondere sollte das System aus Mikrotubuli und dem Motorprotein Kinesin-1, welches für die meisten aktuellen Studien zum Thema Nanotransport herangezogen wird, untersucht werden. Schließlich sollten neue Erkenntnisse über weniger gut erforschte Motorproteine, speziell über 22S Dynein und das Kinesin-14 „Non-claret disjunctional“ (Ncd), gewonnen werden. Beide Motoren könnten in Nanotransportsystemen als Gegenspieler von Kinesin-1 agieren. In der vorliegenden Arbeit wird eine neuartige, auf Fluoreszenz-Interferenz basierende 3-D Nanometertrackingmethode beschrieben. Auf deren Grundlage wird es möglich, die Bewegung von einzelnen fluoreszenten Partikeln nahe einer reflektierenden Oberfläche mit einer Genauigkeit im Nanometerbereich zu verfolgen. Im Vergleich zu anderen kürzlich vorgestellten 3-D Techniken, welche auf bifokaler optischer Mikroskopie basieren und ähnliche Genauigkeiten zulassen, ist die hier vorgestellte Methode mit deutlich geringerem Aufwand auf der Basis eines herkömmlichen Epi-Fluoreszenzmikroskops umsetzbar. Dabei kann die Fluoreszenzanregung wahlweise mit einer Bogenlampe oder einem Laser erfolgen. Weiterhin besteht die Möglichkeit, nicht nur Differenzwerte (wie bei bifokaler Mikroskopie), sondern absolute Werte in der Höhendimension zu messen. Im Ergebnis wurde ein mit geringem Aufwand umsetzbares, gleichwohl hochgradig genaues und vielseitig einsetzbares Werkzeug geschaffen, welches ideal für Studien der Interaktionen von Einzelmolekülen oder auch intramolekularer Dynamik geeignet ist. Mit Hilfe der hier vorgestellten 3-D Trackingmethode wurden die Rotationen von Mikrotubuli um ihre Längsachse während des Gleitens auf mit Motorproteinen besetzten Oberflächen analysiert. Diese Geometrie wird derzeit bevorzugt in Studien eingesetzt, welche den Einsatz von biomolekularen Motoren für den Transport von nanoskaligen Objekten untersuchen und das Ziel verfolgen, Nanostrukturen zu erzeugen und zu manipulieren. Die Ergebnisse zu Rotationen von Mikrotubuli, welche über mit Kinesin-1 besetzte Oberflächen bewegt werden, sind konsistent mit (i) der Eigenschaft von Kinesin-1 sich entlang der Protofilamente von Mikrotubuli zu bewegen und (ii) der Superhelixstruktur von in vitro rekonstituierten Mikrotubuli. Dies belegt die Eignung der Methode für die Charakterisierung von Nanotransportsystemen. Die Rotation von Mikrotubuli, welche durch Kinesin-1 angetrieben werden, hat sich sowohl beim Transport von kleinen Objekten in Form von Quantum Dots (Durchmesser ca. 20 nm) als auch bei der Reduktion elektrostatischer Wechselwirkungen zwischen Kinesin-1 und Mikrotubuli durch Verdau der Tubulin-C-Termini als stabil erwiesen. Ein vollkommen anderes Bild ergab sich für den Transport von großen Objekten (Durchmesser ca. 3 µm). In diesem Fall wurde die Rotation der Filamente angehalten. Unerwarteterweise war jedoch die Vorwärtsbewegung der Mikrotubuli und insbesondere deren Geschwindigkeit kaum betroffen. Dies zeigt, daß Mikrotubuli, welche von prozessiven Motoren wie Kinesin-1 angetrieben werden, das Potential zu responsiven, flexiblen und effektiven molekularen Shuttles besitzen. Außerdem weisen die Ergebnisse darauf hin, daß Kinesin-1-Moleküle, welche in vivo Frachten entlang von Mikrotubuli transportieren, auf seitwärts gerichtete Kräfte reagieren können, indem sie von ihrem intrinsisch vorgegebenen Pfad parallel zur Protofilamentachse des Mikrotubulus abweichen. Zwei Motoren, die sich im Gegensatz zu Kinesin-1 in Richtung des Minus-Endes von Mikrotubuli bewegen, sind 22S Dynein und Ncd. Sie sind somit als Gegenspieler von Kinesin-1 in Nanotransportsystemen prädestiniert. Beide Motoren können, ebenso wie Kinesin-1, die Translokation von Mikrotubuli über Oberflächen sowie damit verbundene Rotationen von Mikrotubuli verursachen. Im Gegensatz zu Kinesin-1 tritt die Rotation unabhängig von einer Superhelixstruktur der Mikrotubuli auf. Die Ergebnisse für 22S Dynein lösen Widersprüche zwischen früheren Studien auf, indem sie belegen, daß dieser Motor Rotationen von Mikrotubuli erzeugen kann. Jedoch scheint es unter Verwendung von 22S Dynein nicht möglich zu sein, Bedingungen zu schaffen, unter welchen sich Mikrotubuli in geeigneter Weise als Nanoshuttles homogen und reproduzierbar bewegen. Der Einsatz von Ncd ist hier deutlich erfolgversprechender. Die in diesem Falle erlangten Erkenntnisse bezüglich der Erzeugung von Rotationen von Mikrotubuli decken sich mit früheren Studien. Ein bislang unbekannter, bemerkenswerter Effekt ist dabei ein Rückgang in der Länge der Rotationsperioden mit sinkender ATP-Konzentration. Die mit dem heutigen Wissensstand über den mechanochemischen Zyklus von Ncd konsistente Erklärung ist, daß Ncd-Motoren im nukleotidfrei an Mikrotubuli gebundenen Zustand die Vorwärtskomponente der Bewegung von gleitenden Mikrotubuli stärker hemmen als die Rotationskomponente. Möglicherweise kann die sich hieraus ergebende Möglichkeit der Regulierung der Rotation von Mikrotubuli dazu eingesetzt werden, das Be- und Entladen von Nanoshuttles zu steuern.

info:eu-repo/classification/ddc/620

ddc:620

How Kinesin-1 Deals With Roadblocks: Biophysical Description and Nanotechnological Application

Korten, Till

10 December 2009

Proteins have been optimized by evolution for billions of years to work on a nanometer scale. Therefore, they are extremely promising for nanotechnological applications. Cytoskeletal filaments propelled by surface-attached motor proteins have been recently established as versatile transport platforms for nano-sized cargo in molecular sorting and nano-assembly devices. However, in this gliding motility setup, cargo and motors share the filament lattice as a common substrate for their activity. Therefore, it is important to understand the influence of cargo-loading on transport properties. By performing single molecule stepping assays on biotinylated microtubules, it was shown that kinesin-1 motors first stop and then detach when they encounter a streptavidin obstacle on their path along the microtubule. Consequently, the deceleration of streptavidin coated microtubules in gliding assays could be attributed to an obstruction of kinesin-1's path on the microtubule rather than to "frictional" streptavidin-surface interactions. The insights gained by studying kinesin-1's behavior at obstacles were then used to demonstrate a novel sensing application: Using a mixture of two distinct microtubule populations that each bind a different kind of protein, the presence of these proteins was detected via speed changes in the respective microtubule populations. In future applications, this detection scheme could be combined with other recent advancements in the field, creating highly integrated lab-on-a-chip devices that use microtubule based transport to detect, sort and concentrate analytes. It has been envisioned that the kinesin-1-microtubule system could be used for even more complex appliances like nano-assembly lines. However, currently available control mechanisms for kinesin-1 based transport are not precise enough. Therefore, improved temporal control mechanisms for kinesin-1 were investigated: Using a polymer that changes its size in solution with temperature, starting and stopping of gliding microtubules was demonstrated. In combination with local heating by light, this effect could be used to control the gliding of single microtubules. Finally, a strategy to create photo-switchable kinesin-1 was developed and tested for feasibility using molecular modeling.

info:eu-repo/classification/ddc/570

ddc:570

High performance photonic probes and applications of optical tweezers to molecular motors

Jannasch, Anita

21 December 2012

Optical tweezers are a sensitive position and force transducer widely employed in physics and biology. In a focussed laser, forces due to radiation pressure enable to trap and manipulate small dielectric particles used as probes for various experiments. For sensitive biophysical measurements, microspheres are often used as a handle for the molecule of interest. The force range of optical traps well covers the piconewton forces generated by individual biomolecules such as kinesin molecular motors. However, cellular processes are often driven by ensembles of molecular machines generating forces exceeding a nanonewton and thus the capabilities of optical tweezers. In this thesis I focused, fifirst, on extending the force range of optical tweezers by improving the trapping e fficiency of the probes and, second, on applying the optical tweezers technology to understand the mechanics of molecular motors. I designed and fabricated photonically-structured probes: Anti-reflection-coated, high-refractive-index, core-shell particles composed of titania. With these probes, I significantly increased the maximum optical force beyond a nanonewton. These particles open up new research possibilities in both biology and physics, for example, to measure hydrodynamic resonances associated with the colored nature of the noise of Brownian motion. With respect to biophysical applications, I used the optical tweezers to study the mechanics of single kinesin-8. Kinesin-8 has been shown to be a very processive, plus-end directed microtubule depolymerase. The underlying mechanism for the high processivity and how stepping is affected by force is unclear. Therefore, I tracked the motion of yeast (Kip3) and human (Kif18A) kinesin-8s with high precision under varying loads. We found that kinesin-8 is a low-force motor protein, which stalled at loads of only 1 pN. In addition, we discovered a force-induced stick-slip motion, which may be an adaptation for the high processivity. Further improvement in optical tweezers probes and the instrument will broaden the scope of feasible optical trapping experiments in the future.

info:eu-repo/classification/ddc/530

ddc:530

Charakterizace PTEN domény vybraných forminů II. třídy Arabidopsis / Characterization of the PTEN domain of selected Arabidopsis class II formins

Přerostová, Sylva

January 2011

Formins are proteins facilitating formation of actin filaments. They affect structure of cytoskeleton and participate in cytokinesis and tip growth. There are 2 classes of formins in Arabidopsis thaliana, which include FH1 and FH2 (Formin Homology 1 and 2) domain. Formins of the class I have usually a transmembrane domain on N-terminus. Due to this fact they can interact with membranes. Some formins from the class II include PTEN domain (Phosphatase and Tensin Homolog) derived from sequences of PTEN proteins which has lost the function of phosphatase. It is assumed this domain can bind on a membrane via the phosphatase section or C2 domain. This thesis was focused on the formin AtFH13 from the class II in Arabidopsis thaliana and on its PTEN domain. There were analyzed differences between mutants and wild-types in length of roots in seedlings and in size of seeds and seed coats, and observed the effect of dexamethasone on the length of roots on AtFH13. PTEN domain of the formin was isolated from cDNA, cloned to a vector and fused with YFP. The tagged protein was visualized by the method of transient expression in epidermal cells in the leaves of Nicotiana benthamiana. No big differences were observed between plants mutant in the gene AtFH13 and wild-type in choice parameters. Dexamethasone did't influence...

Hydrolasy závislé na zinku: Studium struktury a funkce glutamátkarboxypeptidasy II a histondeacetylasy 6 / Zinc-Dependent Hydrolases: Structure-Function Study of Glutamate Carboxypeptidase II and Histone Deacetylase 6

Škultétyová, Ľubica

January 2018

Zinc-binding proteins represent approximately one tenth of the proteome and a good portion of them are zinc-dependent hydrolases. This thesis focuses on biochemical and structural characterization of glutamate carboxypeptidase II (GCPII) and histone deacetylase 6 (HDAC6), two members of the zinc-dependent metallohydrolase superfamily. We describe here their interactions with natural substrates and inhibitors. GCPII is a homodimeric membrane protease catalyzing hydrolytic cleavage of glutamate from the neurotransmitter N-acetylaspartylglutamate (NAAG) and dietary folates in the central and peripheral nervous systems and small intestine, respectively. This enzyme is associated with several neurological disorders and also presents an ideal target for imaging and treatment of prostate cancer. GCPII inhibitors typically consist of a zinc-binding group (ZBG) linked to an S1' docking moiety (a glutamate moiety or its isostere). As such, these compounds are highly hydrophilic molecules therefore unable to cross the blood-brain barrier and this hampers targeting GCPII to the central nervous system. Different approaches are adopted to alter the S1' docking moiety of the existing inhibitors. As a part of this thesis, we present different strategies relying on replacement of the canonical P1' glutamate residue...

Roles of the Mother Centriole Appendage Protein Cenexin in Microtubule Organization during Cell Migration and Cell Division: A Dissertation

Hung, Hui-Fang

03 August 2016

Epithelial cells are necessary building blocks of the organs they line. Their apicalbasolateral polarity, characterized by an asymmetric distribution of cell components along their apical-basal axis, is a requirement for normal organ function. Although the centrosome, also known as the microtubule organizing center, is important in establishing cell polarity the mechanisms through which it achieves this remain unclear. It has been suggested that the centrosome influences cell polarity through microtubule cytoskeleton organization and endosome trafficking. In the first chapter of this thesis, I summarize the current understanding of the mechanisms regulating cell polarity and review evidence for the role of centrosomes in this process. In the second chapter, I examine the roles of the mother centriole appendages in cell polarity during cell migration and cell division. Interestingly, the subdistal appendages, but not the distal appendages, are essential in both processes, a role they achieve through organizing centrosomal microtubules. Depletion of subdistal appendages disrupts microtubule organization at the centrosome and hence, affects microtubule stability. These microtubule defects affect centrosome reorientation and spindle orientation during cell migration and division, respectively. In addition, depletion of subdistal appendages affects the localization and dynamics of apical polarity proteins in relation to microtubule stability and endosome recycling. Taken together, our results suggest the mother centriole subdistal appendages play an essential role in regulating cell polarity. A discussion of the significance of these results is included in chapter three.

Heat-Shock Proteins

Cell Division

Cell Movement

Cell Polarity

Centrioles

Centrosome

Endosomes

Epithelial Cells

Microtubule-Organizing Center

Microtubules

Cenexin

Dissertations, UMMS

Cell Biology

Cellular and Molecular Physiology

Validation of synthetic lethal hits of microtubule targeting agents

Di Lalla, Matthew

05 1900

Les microtubules, composants clés du cytosquelette des cellules eucaryotes, sont des polymères de tubuline très dynamiques et impliqués dans une grande variété de processus cellulaires. Leur rôle essentiel dans le cycle cellulaire a fait d’eux une cible validée en thérapie anticancéreuse. Malgré l’efficacité clinique des agents ciblant les microtubules (ACM), les effets secondaires compliquent l’utilisation. Nous avons cherché à identifier des vulnérabilités génétiques qui peuvent être exploitées pour diminuer la dose requise tout en maintenant l'efficacité, et donc réduire les effets secondaires. En collaboration avec le laboratoire Tyers à l’IRIC, nous avons réalisé un criblage génétique basé sur la létalité synthétique avec des agents antiprolifératifs, dont les ACMs. Nous avons sélectionné les gènes dont l’extinction sensibilisait les cellules aux ACMs. J’ai confirmé que l’invalidation de chacun des gènes GNA13, SEPHS1, DLGAP5 et des gènes QRICH1, DLGAP5 sensibilisaient les cellules NALM6 au docétaxel et la vincristine respectivement. En revanche, aucune invalidation de ces gènes n'a augmenté la sensibilité au docétaxel dans les cellules U2OS. En plus de son effet avec le docétaxel, le gène GNA13 s’est distingué être une cible particulièrement intéressante. En effet, la perte complète de GNA13 augmente considérablement la fréquence et la gravité d’erreurs de ségrégation des chromosomes dans les cellules U2OS. Cette augmentation n’a pas été rectifiée à la suite d’un traitement avec la molécule UMK57, connue pour réduire le taux d’erreurs de ségrégation des chromosomes. De manière intéressante, la perte complète de GNA13 augmente également la fréquence des erreurs de ségrégation des chromosomes dans les cellules RPE1, cellules non-cancéreuses et stables au niveau chromosomique. Cela suggère que la perte complète de GNA13 ne nécessite pas de transformation ni d'instabilité chromosomique, comme conditions préalables pour exacerber l'instabilité chromosomique. L’ensemble de ces résultats ouvre une nouvelle voie de stratégies thérapeutiques anticancéreuses, à savoir, le traitement des cancers présentant une mutation des gènes QRICH1, DLGAP5, GNA13, et SEPHS1 avec de faibles doses d’ACMs. En particulier, GNA13 est fréquemment muté dans certains lymphomes. De plus, les résultats obtenus démontrent que la perte complète de GNA13 aggrave l’instabilité chromosomique et par conséquent, pourrait être impliquée dans la cancérogenèse. / Microtubules, key components of the eukaryotic cytoskeleton, are highly dynamic polymers of tubulin implicated in a wide variety of cellular processes. Their essential roles in the cell cycle have made them a valid target in cancer therapy. Despite the clinical efficacy of microtubule targeting agents (MTA), their use is hampered by side effects. We sought to identify genetic vulnerabilities that can be exploited to decrease the required dose while maintaining efficacy, and therefore reduce side effects. In collaboration with the Tyers laboratory at IRIC, we carried out a genetic screen based on synthetic lethality with antiproliferative agents, including MTAs. We have selected genes whose knockout sensitized cells to MTAs. I have confirmed that the knockout of GNA13, SEPHS1, DLGAP5, and QRICH1, DLGAP5, sensitize NALM6 cells to docetaxel and vincristine respectively. However, no knockout of these genes increased the sensitivity to docetaxel in U2OS cells. In addition to its effect with docetaxel, GNA13 stood out as being a particularly exciting target. GNA13 knockout increased the frequency and severity of chromosome segregation errors in U2OS cells. This increase was not corrected following treatment with UMK57, a molecule known to reduce the rate of chromosome segregation errors. Interestingly, the GNA13 knockout also increased the frequency of chromosome segregation errors in non-cancerous and chromosomally stable RPE1 cells. This suggests that GNA13 does not require transformation nor chromosomal instability as prerequisites for exacerbating chromosomal instability. Overall, these results open up a new avenue of anticancer therapeutic strategies, namely, the treatment of cancers presenting mutations in QRICH1, DLGAP5, GNA13, and SEPHS1 with lower doses of MTAs. In particular, GNA13 is frequently mutated in certain lymphomas. In addition, the results obtained demonstrate that GNA13 knockout exacerbates chromosomal instability and, therefore, could be involved in carcinogenesis.

Microtubules

Cancer

Instabilité chromosomique

Mitose

Létalité synthétique

Docétaxel

Vincristine

GNA13

QRICH1

DLGAP5

SEPHS1

Chromosomal instability

Mitosis

Synthetic lethality

Temperature-dependence of microtubule dynamics across Xenopus species

de Gaulejac, Ella

17 May 2023

Eukaryontische Zellen besitzen ein Zytoskelett, ein zelluläres Netzwerk aus Biopolymeren. Unter diesen Biopolymeren sind die Mikrotubuli weitgehend konserviert. Diese aus Tubulin aufgebauten Filamente sind dynamisch und wechseln zwischen Phasen des Wachstums und der Schrumpfung. Die genauen Mechanismen, die die dynamische Instabilität der Mikrotubuli bestimmen, werden noch erforscht. Die Allgegenwart von Mikrotubuli wirft die Frage auf, wie sie in verschiedenen thermischen Umgebungen konservierte Funktionen ausführen können. Um dieser Fragestellung nachzugehen, habe ich verwandte Froscharten mit unterschiedlich temperierten Lebensräumen untersucht: Xenopus laevis (16-22 °C), Xenopus borealis (19-23 °C) und Xenopus tropicalis (22-30 °C). Um zu untersuchen, ob sich die biochemischen Eigenschaften von Tubulin und die Dynamik der Mikrotubuli bei den drei Arten an die Temperatur angepasst hat, habe ich die Methoden der Tubulin-Affinitätsreinigung und die temperaturgesteuerte TIRF-Mikroskopie zur Rekonstitution der Mikrotubuli-Dynamik kombiniert. Dabei habe ich festgestellt, dass bei einer Temperatur von 25°C die Wachstumsgeschwindigkeit der Mikrotubuli im Bezug zur thermischen Nische der einzelnen Arten negativ korreliert. Die Verwendung der Arrhenius-Gleichung zum Vergleich der Aktivierungsenergie der Mikrotubuli-Polymerisation für jede Spezies ergab, dass die freie Energie des Tubulins umso höher ist, je kälter die thermische Nische der Spezies ist. Die Mikrotubuli von X. laevis und X. borealis zeigten eine längere Lebensdauer und wurden häufiger zerstört als die von X. tropicalis. Die Tubuline von X. laevis und X. borealis sind phosphoryliert, im Gegensatz zu X. tropicalis. Die Ergebnisse zeigen, dass sich Xenopus Tubulin und die Dynamik der Mikrotubuli an die Temperatur angepasst haben. Kalt lebende Arten kommen mit der niedrigeren Energie des Milieus zurecht, durch verbessertes Wachstum und Stabilität. / Eukaryotic cells hold a cytoskeleton, a cellular network of biopolymers. Among the filaments of the cytoskeleton, microtubules are widely conserved. Built from tubulin, those filaments are dynamic, alternating between phases of growth and shrinkage. The biochemical properties of tubulin shape the dynamic behavior of microtubules, which is crucial for many cellular processes. The precise mechanisms determining microtubule dynamic instability are still under investigation. The ubiquity of microtubules raises the question of how they can perform conserved functions within various thermal environments. To address this, I turned to closely related frog species living at different temperatures, Xenopus laevis (niche: 16-22°C), Xenopus borealis (19-23°C) and Xenopus tropicalis (22-30°C). To probe whether the biochemical properties of tubulin and microtubule dynamics adapted to temperature across those three species, I combined tubulin affinity purification and temperature-controlled TIRF microscopy of in vitro reconstitution of microtubule dynamics. I found that at 25°C, the microtubule growth velocity inversely correlates with the thermal niche of each species. Adjusting temperature to each species’ endogenous condition modulates the growth rate differences across species. Using the Arrhenius equation to compare the activation energy of microtubule polymerization for each species suggested that the colder the thermal niche of the species, the higher the free energy of its tubulin. Microtubules from the cold-adapted species X. laevis and X. borealis have longer lifetimes and rescue more often than those of X. tropicalis, both at 25°C and at each species’ endogenous condition. X. laevis and X. borealis tubulins are phosphorylated, contrary to X. tropicalis. My results show that Xenopus tubulin and microtubule dynamics have adapted to temperature. Cold-living species cope with the lower energy of the milieu by facilitating growth and stability.

Tubulin

Thermische Adaptation

Xenopus

TIRF Mikroskopie

Tubulin

Thermal adaptation

Xenopus

TIRF microscopy

Microtubules

Dynamic instability

in vitro assay

572 Biochemie

ddc:572

Régulation du récepteur nucléaire Nor1 par la SUMOylation et mécanismes de protection neuronale

Gagnon, Jonathan

04 1900

Afin de répondre correctement aux nombreux changements se produisant à chaque instant dans leur environnement, les cellules utilisent une panoplie de messagers moléculaires dont la synchronisation est essentielle à la signalisation cellulaire appropriée. La superfamille des récepteurs nucléaires compte quarante-huit membres impliqués dans ces processus de signalisation et influence ainsi plusieurs fonctions physiologiques. Les récepteurs nucléaires de la sous-famille NR4A composée de Nur77/NR4A1, Nurr1/NR4A2 et Nor1/NR4A3 sont des facteurs critiques du développement et de la maintenance du système nerveux. Nor1/NR4A3 en particulier est essentiel aux processus de guidage axonal et de survie neuronale au niveau de l’hippocampe. Les NR4A se démarquent des autres récepteurs nucléaires puisqu’ils sont considérés comme des récepteurs orphelins constitutivement actifs, ce qui veut dire qu’ils ne nécessitent pas d’interaction avec un ligand afin d’être activés. Il devient ainsi important d’identifier de nouveaux mécanismes de régulation pour cette sous-famille de récepteur afin d’améliorer notre compréhension et potentiellement contrôler leurs activités dans un contexte neuronal. L’activité des récepteurs nucléaires peut être régulée de plusieurs façons, indépendamment de leur association avec un ligand endogène. Les modifications post-traductionnelles représentent un aspect crucial de la signalisation cellulaire permettant de réguler la fonction des protéines cibles de manière spécifique au contexte. La SUMOylation et la phosphorylation sont des exemples de modifications post-traductionnelles avec le potentiel de réguler l’activité transcriptionnelle, la stabilité et l’expression des gènes cibles des récepteurs nucléaires. Dans cette thèse, l’impact de la SUMOylation retrouvée sur un motif consensus ainsi que sur un motif non-consensus de SUMOylation phosphorylé du récepteur Nor1 est étudié. Dans la première étude, un motif de SUMOylation non-consensus nouvellement découvert sur Nor1 est décrit. Ce nouveau motif nommé pSuM a été identifié pour la première fois sur le récepteur nucléaire des estrogènes ERβ et sur le récepteur farnésoÏde FXR. Nous avons identifié un motif pSuM situé à la lysine 137 de Nor1 qui sert de cible fonctionnelle de SUMO2. Le pSuM se démarque du motif de SUMOylation consensus puisqu’il nécessite une phosphorylation afin d’être SUMOylé. Dans le cas de Nor1, nos résultats démontrent que la sérine 139 est phosphorylée par la voie des MAPK. La SUMOylation sur ce site mène à une réduction de l’activité transcriptionnelle et du recrutement à la chromatine de Nor1 ainsi que de l’expression des gènes sensibles à Nor1. Une particularité intéressante du pSuM de Nor1 est qu’il possède également une extension phosphorylable par la kinase CK2 qui est essentielle au processus de SUMOylation. Cette extension a également un effet sur la stabilité et la compétence transcriptionnelle de Nor1. En utilisant des lignées SH-SY5Y exprimant de manière stable différents mutants SUMO de Nor1, il est démontré que la SUMOylation du pSuM diminue la prolifération et la survie cellulaire en réponse au stress oxydant. Dans la seconde étude, la SUMOylation de Nor1 sur un motif de SUMOylation canonique situé sur la Lysine 89 est caractérisée. Il est démontré que ce site de SUMOylation est ciblé principalement par SUMO1 et qu’il est important afin de maintenir une compétence transcriptionnelle et une stabilité optimale du récepteur. Cette SUMOylation régule également la prolifération et la survie en réponse à un traitement au nocodazole des lignées stables ainsi que la stabilité des microtubules. En conclusion, ces études identifient de nouveaux mécanismes de SUMOylation et phosphorylation utilisés dans la régulation de l'activité du récepteur nucléaire Nor1. Elles permettent également d’approfondir nos connaissances des rôles joués par Nor1 dans la neuroprotection en réponse au stress oxydant ainsi que dans la régulation de la stabilité du réseau de microtubules, ce qui apporte une nouvelle fonction de Nor1. Puisque Nor1 et les autres NR4A sont fortement impliqués dans la formation et maintenance du système nerveux et que les modifications post-traductionnelles peuvent réguler ces fonctions, la découverte et la caractérisation de nouveaux mécanismes de régulation de ces récepteurs ont le potentiel de nous fournir des nouvelles connaissances utiles dans le cadre des maladies neurodégénératives et autres conditions pathologiques. / To answer the many changes happening every instant in its surroundings, cells require a fine-tuned array of molecular messengers to carry on proper signal transduction and homeostasis. The superfamily of nuclear receptors contains forty-eight members implicated in a wide variety of cellular and physiological functions. The nuclear receptors of the NR4A subfamily containing Nur77/NR4A1, Nurr1/NR4A2 and Nor1/NR4A3 are heavily implicated in the development and maintenance of the nervous system. In particular, Nor1/NR4A3 has been shown to be essential for axonal guidance and neuronal survival in the hippocampus. This subfamily also operates differently from other nuclear receptors as they are considered constitutively active orphan nuclear receptors without known endogenous ligand. Therefore, there is an increasing need to identify critical mechanisms that regulate NR4A nuclear receptors and to better understand the control of their activities in a neuronal context. Nuclear receptor activity can be regulated in various ways independently of their interaction with an endogenous ligand. One is through post-translational modifications which allow the regulation of protein function depending on the cellular context. SUMOylation and phosphorylation are post-translational modifications with the potential to regulate nuclear receptor activity, stability and target gene expression. In this thesis, the impact of a canonical SUMOylation site and a phosphorylation dependant SUMOylation motif on the orphan nuclear receptor Nor1 are studied. In the first study, a newly identified non-canonical SUMOylation motif on Nor1 was described. This new motif named pSuM was first identified on the nuclear estrogen receptor ERβ and farnesoid X receptor FXR. We report that this pSuM is located at Lys-137 on Nor1 and is a target of SUMO2. The pSuM differs from traditional SUMOylation motif since it requires to be phosphorylated for SUMOylation to occur. For Nor1, our evidence showed that the obligate phosphorylation of the pSuM on Ser-139 occurred through the MAPK pathway. SUMOylation of Nor1 pSuM reduced Nor1 transcriptional competence, responsive gene expression and chromatin binding. Interestingly, the pSuM of Nor1 also possesses an extension phosphorylated by the CK2 kinase, which is essential to achieve the SUMOylation process. This extension also affected Nor1 protein stability and transcriptional activity. Using stable SH-SY5Y cell lines expressing different SUMO mutants of Nor1, we also showed that Nor1 pSuM SUMOylation reduced cell proliferation and survival to oxidative stress. In the second study, the SUMOylation of Nor1 on a canonical SUMOylation site found at Lys-89 was characterized. This SUMOylation site was found to be targeted mainly by SUMO1 and to be important in maintaining optimal transcriptional competency and stability of the receptor. This SUMOylation also regulated proliferation and survival to a nocodazole treatment of stable cell lines, as well as microtubule network stability. In conclusion, these studies provide novel mechanisms in the regulation of Nor1 activity by SUMOylation and phosphorylation. They also helped to expand our knowledge on the role played by Nor1 in neuroprotection in response to oxidative stress, as well as in the regulation of microtubule stability, which identified a new function of Nor1. Since Nor1 and other NR4A receptors are implicated in the formation and maintenance of the nervous system, the identification of post-translational modifications as a regulatory mechanism uncovers novel opportunities in our understanding of these receptors and provide new insights for neurodegenerative diseases and other neuropathological conditions.

NR4A3/Nor1

NR4A2/Nurr1

NR4A1/Nur77

SUMOylation

Stress oxydant

CK2

Microtubules

Phosphorylation

Récepteurs nucléaires

Nuclear receptor

Oxidative stress