Développements méthodologiques pour l'exploration spatio-temporelle des mécanismes de transduction du signal

Rouger, Vincent

02 October 2013

La membrane plasmique constitue la première entité séparant la cellule de son environnement. A ce rôle de barrière s'ajoute celui de réguler la. Par conséquent, la membrane plasmique est une zone privilégiée pour le passage d'information. Cependant, son étude reste difficile, ne serait-ce que par l'extraordinaire complexité d'organisation de cet assemblage supramoléculaire.Mon projet de thèse vise à développer de nouvelles approches expérimentales pour explorer plus spécifiquement l'organisation et le rôle de la membrane plasmique d'une cellule dans les mécanismes de transduction de l'information. Deux axes ont été privilégiés : le premier, concerne la description de la dynamique d'organisation de la membrane ; le deuxième concerne l'inter-connectivité et la transmission du signal d'une cellule avec d'autres partenaires.Ce manuscrit se compose de plusieurs parties. Le premier chapitre introduira succinctement les questions biologiques. Dans le second chapitre, je présenterai des méthodes utilisées pour l'étude de la membrane. J'y présenterai aussi une série d'observation que j'ai réalisée sur la diffusion de l'EGFR. Le troisième chapitre sera consacré à la technique de corrélation croisée de fluorescence depuis le montage jusqu'à l'étude du modèle EGFR. Dans la quatrième partie, nous verrons comment les collaborations à l'interface biophysique ont permis des développements innovants sur un système de pinces optiques holographiques. J'y présenterai les applications de ce système à différent modèles d'intérêt biologique. Enfin, je conclurai ce document par une brève discussion autour des résultats obtenus aussi bien d'un point de vue méthodologique que biologique. / The plasma membrane separates the cell from its environment. But it is more than a barrier any cell has to communicate with the outside world. Therefore the plasma membrane plays a prime role in transferring and exchanging information. However, the biological study of the plasma membrane remains difficult due to the extraordinary complexity of it organization.My thesis is a part of an effort to develop new experimental approaches to explore more specifically the organization and the role of the plasma membrane in the signal transduction mechanisms. Two major aspects were followed: the first one concerns the description of the dynamics of membrane organization and of molecular interactions, the second concerns the inter-connectivity and signal transduction between a cell and other biological partners.This manuscript is composed of several parts. The first chapter briefly introduces the biological questions that I tried to answer. In the second chapter, I present the methods commonly used to study the membrane with a dynamic perspective. Additionally, I include a series of observations that I made on the EGF receptor diffusion. The third chapter is devoted to the fluorescence cross-correlation technique to study the assembly of the EGFR. In the fourth part, I demonstrate how scientific collaborations at the interface between biology and physics have led to the development of innovative solutions on a holographic optical tweezers system. I present applications of this system in different biological models. Finally, I conclude this thesis with a brief discussion about my technological and biological results.

Membrane plasmique

Récepteur

Diffusion moléculaire

Microscopie photonique

Pinces optiques holographiques

Plasma membrane

Receptor

Molecular diffusion

Photonic microscopy

Fluorescence correlation spectroscopy

Holographic optical tweezers

571

Optical techniques for the investigation of a mechanical role for FRMD6/Willin in the Hippo signalling pathway

Goff, Frances

January 2019

The mammalian hippo signalling pathway controls cell proliferation and apoptosis via transcriptional co-activators YAP and TAZ, and as such is a key regulator of organ and tissue growth. Multiple cellular components converge in this pathway, including the actin cytoskeleton, which is required for YAP/TAZ activity. The precise mechanism by which the mechanical actomyosin network regulates Hippo signalling, however, is unknown. Optical methods provide a non-invasive way to image and study the biomechanics of cells. In the past two decades, super-resolution fluorescence microscopy techniques that break the diffraction limit of light have come to the fore, enabling visualisation of intracellular detail at the nanoscale level. Optical trapping, on the other hand, allows precise control of micron-sized objects such as cells. Here, super resolution structured illumination microscopy (SIM) and elastic resonator interference stress microscopy (ERISM) were used to investigate a potential role for the FERM-domain protein FRMD6, or Willin, in the mechanical control of the Hippo pathway in a neuronal cell model. A double optical trap was also integrated with the Nikon-SIM with the aim of cell stretching. Willin expression was shown to modify the morphology, neuronal differentiation, actin cytoskeleton and forces of SH-SY5Y cells. Optical trapping from above the SIM objective, however, was demonstrated to be ineffective for manipulation of adherent cells. The results presented here indicate a function for Willin in the assembly of actin stress fibres that may be the result of an interaction with the Hippo pathway regulator AMOT. Further investigation, for example by direct cell stretching, is required to elucidate the exact role of Willin in the mechanical control of YAP/TAZ.

Diffusion de la lumière dans les nuages denses mésoscopiques d'atomes froids / Light scattering in dense mesoscopic cold atomic clouds

Bourgain, Ronan

13 March 2014

Lorsque l’on place des atomes suffisamment proches les uns des autres, l’interaction dipôle-dipôle résonante entre les atomes modifie leurs propriétés. Les atomes se comportent alors de manière collective. Ces effets collectifs se produisent lorsque les distances interparticulaires sont de l’ordre de l/(2Pi), où l est la longueur d’onde de la transition atomique. La densité atomique est alors de l’ordre de 10^14 at/cm^3. Afin de créer des échantillons d’atomes froids présentant des densités aussi élevées, nous avons mis en place plusieurs méthodes de chargement de nos pinces optiques de taille micrométrique. L’une d’elles utilise un processus d’évaporation forcée qui amène les atomes proches de la dégénérescence quantique. En utilisant des nuages denses contenant quelques centaines d’atomes à des densités spatiales élevées, et en étudiant les modifications de la diffusion de la lumière qui en résultent, nous avons pu mettre en évidence des effets collectifs entre les atomes. Nous avons par ailleurs mesuré le retard de Wigner associé à la diffusion élastique de la lumière par un atome unique de rubidium. Nous avons mesuré un retard proche de la valeur théorique, c’est-à-dire deux fois la durée de vie de la transition atomique (52 ns). / When several atoms are placed close to each other, the resonant dipole-dipole interactionbetween atoms modifies the atomic properties and atoms behave collectively. These collective effects occur for interatomic distances on the order of l/(2Pi) where l is the wavelength of the atomic transition. The atomic density is then on the order of 10^14 at/cm^3. To create such cold atomic samples, we load optical tweezers with a microscopic size according to several loading schemes. One of them uses forced evaporative cooling and brings the atoms close to quantum degeneracy. We have used dense clouds containing a few hundred atoms with a high spatial density to demonstrate collective effects between the atoms. In particular, we have studied how these effects modify the scattering of light by the cloud. Besides, we have also measured for the first time the time-delay associated to the elastic scattering of light by a single rubidium atom, the so-called Wigner delay. We have shown that this delay is close to the theoretical prediction of twice the lifetime of the atomic transition (52 ns).

Systèmes mésoscopiques

Nuages denses

Atomes froids

Pinces optiques

Interaction dipôle-dipôle

Effets collectifs

Mesoscopic systems

Dense clouds

Cold atoms

Optical tweezers

Dipole-dipole interaction

Collective effects

530.12

Enhanced transport through confined channels by stationary and fluctuating potentials

Tan, Yizhou

January 2019

Binding-sites which facilitate the transport of substrates across membranes are ubiquitous in membrane proteins. To understand this fundamental process in cells, we build up a synthetic membrane system consisting of microfluidic channels and colloidal particles. Holographic optical tweezers are used to modulate the potential energy landscape in those channels. We show how to extract the underlying energy potential by analysing local transition probabilities. Our method is applicable both to equilibrium systems and non-equilibrium steady states. Our method offers improved robustness when dealing with fragmented trajectories or small ensembles of data compared to other established approaches, such as probability density function and splitting probability. Meanwhile, we utilise the intensity distribution of the optical traps generated by holographic optical tweezers to estimate energy landscapes featuring high energy barriers where transitions rarely occur. We use this newly developed experimental system to mimic the functionality of membrane protein transporters that are known to alternate their substrate-binding sites between the extracellular and cytosolic side of the membrane. We study particle transport through a channel coupled with an energy well that oscillates its position between the two entrances of the channel deterministically and stochastically. Optimised particle transport across the channel is obtained by adjusting the oscillation frequency. At the optimal oscillation frequency, the translocation rate of particles through the channel is a hundred times higher with respect to free diffusion across the channel. Our findings reveal the effect of time dependent potentials on particle transport across a channel. This work adds a new tool for the investigation of highly controlled membrane transport processes at the micron scale. Our results are relevant for improving our understanding of membrane transport especially for microfluidics application.

Probing protein - Pili interactions by optical tweezers and 3D molecular modelling

Shirdel, Mariam

January 2013

No description available.

Escherichia coli

E. coli

ETEC

pili

CS20

CFA/I

optical tweezers

OT

FMOT

histatin 5

Escherichia coli

E. coli

ETEC

pili

CS20

CFA/I

optisk pincett

histatin 5

The role of 1D diffusion for directional long-range communication on DNA

Schwarz, Friedrich

18 April 2013

Many genetic processes require enzymes or enzyme complexes that interact simultaneously with distant sites along the genome. Such long-range DNA-enzyme interactions are important for example in gene regulation, DNA replication, repair and recombination. In addition many restriction enzymes depend on interactions between two recognition sites and form therefore a model system for studying long-range communications on DNA. Topic of the present work are Type III restriction enzymes. For these enzymes the communication mechanism between their distant target sites has not been resolved and conflicting models including 3D diffusion, 1D translocation and 1D diffusion have been proposed. Also the role of ATP hydrolysis by their superfamily 2 helicase domains which catalyse functions of many enzyme systems is still poorly understood. To cleave DNA, Type III restriction enzymes sense the relative orientation of their distant target sites and cleave DNA only if at least two of them are situated in an inverted repeat. This process strictly depends on ATP hydrolysis. The aim of this PhD thesis was to elucidate this long-range communication. For this a new single molecule assay was developed using a setup combining magnetic tweezers and objective-type total internal reflection fluorescence microscopy. In addition of being able to mechanically manipulate individual DNA molecules, this assay allows to directly visualize the binding and movement of fluorescently labelled enzymes along DNA. Applying this assay to quantum dot labelled Type III restriction enzymes, a 1D diffusion of the enzymes after binding at their target sites could be demonstrated. Furthermore, it was found that the diffusion depends on the nucleotide that is bound to the ATPase domains of these enzymes. This suggested that ATP hydrolysis acts as a switch to license diffusion from the target site which leads to cleavage. In addition to the direct visualization of the enzyme-DNA interaction, the cleavage site selection, the DNA end influence (open or blocked) and the DNA binding kinetics were measured in bulk solution assays (not part of this thesis). The experimental results were compared to Monte Carlo simulations of a diffusion-collision-model which is proposed as long-range communication in this thesis.

DNA

Langstrecken Kommunikation

Restriktionsenzyme

Magnetische Pinzette

TIRF-Mikroskopie

magnetic tweezers

DNA

restriction enzymes

TIRF- microscopy

helicase

ddc:570

rvk:WC 2905

rvk:WD 5360

Role of Caveolae in Membrane Tension

Köster, Darius Vasco

13 December 2010

Caveolae sind charakteristische Plasmamembraneinstülpungen, die in vielen Zelltypen vorkommen und deren biologische Funktion umstritten ist. Ihre besondere Form und ihre Häu gkeit in Zellen, die stets mechanischen Belastungen ausgesetzt sind, führten zu der Annahme, dass Caveolae die Plasmamembran vor mechanischen Belastungen schützen und als Membranreservoir dienen. Dies sollte mit dieser Dissertation experimentell geprüft werden. Zunächst wurde der Ein uss der Caveolae auf die Membranspannung von Zellen im Normalzustand untersucht. Dann wurden die Zellen mechanisch belastet. Mit Fluoreszensmikroskopie wurde das Verschwinden von Caveolae nach Strecken der Zellen oder nach einem hypo-osmotischen Schock beobachtet. Messungen der Membranspannung vor und unmittelbar nach dem hypo-osmotischem Schock zeigten, dass Caveolae einen Anstieg der Membranspannung verhindern, unabhängig von ATP und dem Cytoskelett. Die Erzeugung von Membranvesikel mit Caveolae erlaubte es, diesen Effekt der Caveolae in einem vereinfachten Membransystem zu beobachten. Schliesslich wurden Muskelzellen untersucht. Zellen, die genetisch bedingt weniger Caveolae haben und mit Muskelschwundkrankheiten in Verbingung stehen, waren mechanisch weniger belastbar als gesunde Zellen. Zusammenfassend wird mit dieser Dissertation die These bestärkt, dass Caveolae einem Anstieg der Membranspannungen entgegenwirken. Dass dies in Zellen und in Vesikeln unabhängig von Energie und Cytoskelett geschieht, lässt auf einen passiven, mechanisch getriebenen Prozess schliessen. Diese Erkenntnis trägt zum Verständnis der Rolle von Caveolae in Zellen bei und kann dem besseren Verständnis von Krankheiten bedingt durch Caveolin-Mutationen, wie z.B. Muskelschwundkrankheiten, dienen. / Caveolae, the characteristic plasma membrane invaginations present in many cells, have been associated with numerous functions that still remain debated. Taking into account the particular abundance of caveolae in cells experiencing mechanical stress, it was proposed that caveolae constitute a membrane reservoir and bu er the membrane tension upon mechanical stress. The present work aimed to check this proposition experimentally. First, the in uence of caveolae on the membrane tension was studied on mouse lung endothelial cells in resting conditions using tether extraction with optically trapped beads. Second, experiments on cells upon acute mechanical stress showed that caveolae serve as a membrane reservoir bu ering surges in membrane tension in their immediate, ATP- and cytoskeleton-independent attening and disassembly. Third, caveolae incorporated in membrane vesicles also showed the tension bu ering. Finally, in a physiologically more relevant case, human muscle cells were studied, and it was shown that mutations with impaired caveolae which are described in muscular dystrophies render muscle cells less resistant to mechanical stress. In Summary the present work provides experimental evidence for the hypothesis that caveolae bu er the membrane tension upon mechanical stress. The fact that this was observed in cells and membrane vesicles in an ATP and cytoskeleton independent manner reveals a passive, mechanically driven process. This could be a leap forward in the comprehension of the role of caveolae in the cell, and in the understanding of genetic diseases like muscular dystrophies. / Cavéoles sont des invaginations caractéristiques de la membrane plas- mique présents dans beaucoup de types cellulaires. Ils sont liées à plusieurs fonctions cellulaires, ce qui sont encore débattues. Prenant compte de l importance des cavéoles dans les cellules soumises au stress mécanique, les cavéoles sont proposées de constituer un réservoir membranaire et de tamponner la tension membranaire pendant des stresses mécaniques. Cette étude a eu le but de tester cette hypothèse expérimentalement. En premier, l in uence des cavéoles sur la tension membranaire au repos a été étudiée sur des cellules endothéliales du poumon de la souris. Puis, on a montré que les cavéoles tamponnent l augmentation de la tension membranaire après l application d un stress mécanique. En suite, la réalisation des vésicules membranaires contenant des cavéoles a permit de montrer leur rôle comme réservoir membranaire dans un système simpli é. Finalement, dans un contexte physiologiquement plus relevant, l étude des cellules musculaires a montrée que les mutations du cavéolin associées aux dystrophies musculaires rendent les cellules moins résistante aux stresses mécaniques. En conclusion, cette étude supporte l\'hypothèse que les cavéoles tamponnent la tension membranaire pendant des stresses mécaniques. Le fait que cela se passe dans les cellules et les vésicules indépendamment d ATP et du cytosquelette révèlent un processus passif et mécanique. Cela pourrait servir à une meilleure compréhension du rôle des cavéoles dans la cellule et les maladies génétiques comme les dystrophies musculaires.

Plasmamembran

Membranspannung

Caveolae

Optische Falle

Vesikel

Caveola

plasma membrane

membrane tension

optical tweezers

osmotic shock

TIRF

vesicle

micropipette

ddc:530

Plasma Membran

Optische Pinzette

Experimental study of the kinetics of two systems : DNA complexation by the NCp7 protein and probe dynamics in a glassy colloidal suspension

Klajner, Piotr

11 May 2012

In the first part of this thesis, we study the kinetics of the complexation of a double-stranded DNA byNCp7 protein. To do this, we study the evolution of mechanical properties of DNA and its complexation by stretching the DNA/NCp7 complex with a optical trap. We observed that the persistence length of the complex decreases progressively during the complexation. Using astatistical model we describe the evolution of the flexibility of DNA complexed with NCp7. Our main result is that the fraction phi of base pairs that have reacted is not a linear function of time at low phi.We interpret our results assuming that the adsorption of NCp7 on DNA is highly cooperative. In the second chapter, we describe the dynamics of probe particles in a colloidal glassy suspension of Laponite. Laponite is a colloidal discoidal particle of 25 nm in diameter and 0.92 nm thick. We take advantage of evanescent wave microscopy, and follow the movement of fluorescent latex particles.Then we image these particles. We show that for a movement that has a single characteristic time scale, it is simply a linear function of time. We find that, what ever their size, the motion of probe particles can be described by a succession of two dynamic modes, where the fastest mode corresponds to the diffusion of particles in a viscoelastic fluid.

[CHIM:OTHE] Chemical Sciences/Other

[CHIM:OTHE] Chimie/Autre

Single molecule

Real time

Optical tweezers

Optical trap

TIRFM

From single to many atoms in a microscopic optical dipole trap

Fuhrmanek, Andreas

23 September 2011

This thesis focuses on the manipulation of rubidium 87 atoms in a microscopic optical dipole trap. The experiments are performed in various regimes where the number of atoms in the microscopic trap ranges from exactly one atom to several thousands on average.The single atom regime allows us to calibrate the experimental setup. We use it a quantum bit, which state we can prepare and read out with efficiencies of 99.97% and 98.6%, respectively. When several atoms are loaded in the microscopic trap we observe a sub-Poissonian distribution of the number of atoms due to light-assisted collisions in the presence of near-resonant light. A study of these collisions in our particular case (microscopic trap) reveals extremely high loss rates approaching the theoretical Langevin limit. Finally, we demonstrate that the loading of the microscopic trap is more efficient when we superimpose on this trap a second macroscopic trap, which we use as an atom reservoir. This reservoir allows us to load the micro trap from the macro trap in the absence of any near-resonant light, thus avoiding light-assisted collisions.The loading of the micro trap from the macro trap leads to optimal initial conditions for forced evaporation towards Bose-Einstein condensation with about ten atoms only. After evaporation we reach phase-space densities approaching the degenerate regime.

[PHYS:QPHY] Physics/Quantum Physics

[PHYS:QPHY] Physique/Physique Quantique

Atomic physics

Quantum information

Single atoms

Mesoscopic systems

Optical tweezers

Bose-Einstein condensation

Light-assisted collisions

Dipole trap

Interaction of XMAP215 with a Microtubule Plus-end Studied with Optical Tweezers

Trushko, Anastasiya

23 July 2012

Microtubules are a part of the cell cytoskeleton that performs different functions, such as providing the mechanical support for the shape of a cell, acting as tracks along which the motor protein move organelles from one part of the cell to another, or the forming mitotic spindle during the cell division. The microtubules are dynamic structures, namely they can grow and shrink. The phase of microtubule growth alternates with the phase of shrinkage that results in the dynamic microtubule network in the cell. However, to form stable and spatially well-defined structures, such as a mitotic spindle, the cell needs to control this stochastic process. This is done by microtubule-associated proteins (MAPs). One class of MAPs is the proteins of XMAP216/Dis1 family, which are microtubule polymerases. The founding member of this family is X. laevis XMAP215. XMAP215 is a processive polymerase acting on the microtubule plus end. XMAP215 binds either directly or reaches the microtubule plus end by the diffusion along the microtubule lattice. Being at the microtubule plus-end XMAP215 stays there transiently and helps to incorporate up to 25 tubulin dimers into microtubule lattice before it dissociates and, therefore, it processively tracks the growing microtubule end during polymerization. There are two hypothesis of microtubule assembly promotion: (i) XMAP215 repeatedly releases an associated tubulin dimer into the microtubule growing plus end or (ii) structurally stabilizes a polymerized tubulin intermediate at the growing plus end and, therefore, preventing depolymerization events. The first way results into the increase of on-rate of tubulin dimers at the microtubule end, whereas the second way results into the decrease of off-rate of tubulin dimers at the microtubule end. Here, I show the study of the mechanism of microtubule growth acceleration by XMAP215 and the dependence of XMAP215 polymerization activity on the applied force. To answer these questions, I investigated the addition of tubulin dimers to the plus end of the microtubule by XMAP215 and how this addition depends on the applied force. XMAP215 remains at the microtubule end for several rounds of tubulin addition surfing both growing and shrinking microtubule ends. Therefore, if one could track the position of the XMAP215 molecules at the very tip of a microtubule with sufficient resolution, it would provide the information about the dynamics of the microtubule end. The technique, which can detect the position of the object of interest with high spatial and temporal resolution in addition to being able to exert a force, is an optical trap. A calibrated optical trap not only provides a good measure of displacement but also enables force measurements. To monitor the position of the molecules of interest, the molecules of interest are usually attached to a microsphere. Hence, I tethered XMAP215 to a microsphere held by an optical trap, and used XMAP215 as a handle to interact with the microtubule tip. When the microtubule grows, the XMAP215 coated microsphere will move in the optical trap and this movement can be detected with high temporal and spatial resolution. My work demonstrates that cooperatively working XMAP215 molecules can not only polymerize microtubule but also harness the energy of microtubule polymerization or depolymerization to transport some cargo. There is an evidence that orthologues of XMAP215 in budding yeasts, fission yeasts and Drosophila localize on the kinetochores. Therefore, the ability of the bearing some load during microtubule polymerization could be potentially important for the XMAP215 functioning during cell division. I also showed the influence of external force applied to the XMAP215 molecules. Pointing toward microtubule growth, a force of 0.5 pN applied to the microtubule tip-coupled XMAP215-coated microsphere increases XMAP215 polymerization activity. However, the force of the same magnitude but applied against microtubule growth does not affect XMAP215 polymerization activity. This result can be explained by the fact, that the force acting in the direction of microtubule growth constrains XMAP215 to be at the very microtubule tip. Hence, XMAP215 can not diffuse away from plus-end and there is higher chance to incorporate tubulin dimers into the microtubule plus-end. The on- and off-rate of tubulin dimers at the microtubule end are both decreased when the external force applied either in direction of microtubule growth or opposite to it. The external force affects the off-rate slightly stronger than on-rate of tubulin dimer. Taking together, my study gives new insights into the mechanism of microtubule polymerization by XMAP215 and shows some novel properties of this protein.

Mikrotubuli

XMAP215

Cytoskelett

dynamische Instabilität

Generierung der Kraft

microtubule

XMAP215

microtubule dynamic instability

microtubule force generation

XMAP215

optical tweezers

ddc:570

rvk:WE 2400