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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
41

Développement de stratégies de biofonctionnalisation de surface de nano-objets pour des applications biologiques / Development of nano-objects surface biofunctionalization strategies for biological applications

Adumeau, Laurent 09 December 2015 (has links)
Cette étude porte sur le développement de nanoparticules pour différentes applicationsbiologiques. Trois systèmes de nanoparticules ont été mis au point : des clusters de nanoparticulesmagnétiques pour l’extraction par magnétophorèse d’objets biologiques, des agents de contrastemultimodaux (IRM, fluorescence dans le proche infrarouge) pour le diagnostic de l’athérosclérose etdes nanoparticules de silice fluorescentes doublement marquées pour la détection de tumeurs in vivo.Au cours de cette étude, une stratégie de greffage de surface de silice par des macromolécules depoly(oxyde d’éthylène) (PEG) permettant d’atteindre de hautes densités de greffage. Cette PEGylationpermet, d’annuler les interactions non spécifiques dans le cadre de l’extraction magnétique rendantainsi ce système plus efficace, et de conférer aux nanoparticules des propriétés de furtivité vis-à-vis dusystème immunitaire dans le cadre du marquage de tumeurs. Le contrôle du nombre de biomoléculesgreffées régiosélectivement sur les nanoparticules (Annexine A5, ou fragments d’anticorps) ainsi quel’étude des interactions biomoléculaires par des techniques de biophysique (SPR, QCM-D) ont permisd’optimiser la propriété de reconnaissance des nano-objets pour leurs cible respective. Enfin, les nanoobjetsont été évalués dans le cadre de leur application. / The aim of this study was the design of nanoparticles for three different biologicalapplications: magnetic nanoparticles cluster for magnetic extraction of biological materials,multimodal contrast agents (MRI and near infrared fluorescence imaging) for atherosclerosisdiagnosis, and fluorescent silica nanoparticles with two different dyes for in vitro and in vivo tumorlabeling. One part of the project dealt with the developement of a new grafting method ofpoly(ethylene oxide) macromolecules onto nanoparticle’s silica surfaces (PEGylation) in order toobtain a high grafting densities. The obtained results have shown that this PEGylation reduces the nonspecificprotein adsorption allowing a better extraction and sorting efficiency, and also permitsnanoparticles to escape the surveillance of the immune system for in vivo tumor labeling. Therefore,the biomolecular recognition of the nanoparticles has been optimized by controlling the number ofconjugated biomolecules and by studying this biomolecular recognition using biophysical methods(SPR, QCM-D). Finally, the different nano-objects were evaluated in the context of their respectiveapplication.
42

Super-resolution STED and two-photon microscopy of dendritic spine and microglial dynamics / Imagerie de la dynamique des microglies et des épines dendritiques par microscopie super-résolutive STED et bi-photonique

Pfeiffer, Thomas 21 November 2017 (has links)
Les changements des connections neuronales interviendraient dans la formation de la mémoire. J’ai développé de nouvelles approches basées sur l’imagerie photonique pour étudier (i) les interactions entre les microglies et les épines dendritiques, et (ii) le renouvellement des épines dans l’hippocampe in vivo. Ces deux phénomènes contribueraient au remodelage des circuits synaptiques intervenant dans la mémoire. (i) Les microglies sont impliquées dans de nouvelles fonctions en condition saine. J’ai examiné l’effet de la plasticité synaptique sur la dynamique morphologique des microglies, et sur leur interaction avec les épines. En combinant l’électrophysiologie et l’imagerie bi-photonique dans des tranches aigües de souris transgéniques, je démontre que la microglie intensifie son interaction physique avec les épines. Ainsi pour continuer l’étude de ces interactions et leur impact fonctionnel plus précisément, j’ai optimisé l’imagerie STED dans des tranches aigües. (ii) La plasticité structurale des épines est cruciale pour la mémoire, mais les connaissances à ce sujet dans l’hippocampe in vivo restent limitées. J’ai donc établi une technique d’imagerie chronique STED in vivo pour visualiser les épines dans l’hippocampe. Cette approche a révélé une densité double de celle reportée précédemment à l’aide de la microscopie bi-photonique. De plus j’ai observé un renouvellement des épines de 40% en 5 jours, représentant un taux important de remodelage synaptique dans l’hippocampe. Les approches d’imagerie super-résolutive permettent l’étude des interactions microglie-épine, et du renouvellement des épines hippocampiques avec une résolution inédite chez la souris vivante. / Activity-dependent changes in neuronal connectivity are thought to underlie learning and memory. I developed and applied novel high-resolution imaging-based approaches to study (i) microglia-spine interactions and (ii) the turnover of dendritic spines in the mouse hippocampus, which are both thought to contribute to the remodeling of synaptic circuits underlying memory formation. (i) Microglia have been implicated in a variety of novel tasks beyond their classic immune defensive roles. I examined the effect of synaptic plasticity on microglial morphological dynamics and interactions with spines, using a combination of electrophysiology and two-photon microscopy in acute brain slices. I demonstrated that microglia intensify their physical interactions with spines after the induction of hippocampal synaptic plasticity. To study these interactions and their functional impact in greater detail, I optimized and applied time-lapse STED imaging in acute brain slices. (ii) Spine structural plasticity is thought to underpin memory formation. Yet, we know very little about it in the hippocampus in vivo, which is the archetypical memory center of the mammalian brain. I established chronic in vivo STED imaging of hippocampal spines in the living mouse using a modified cranial window technique. The super-resolution approach revealed a spine density that was two times higher than reported in the two-photon literature, and a spine turnover of 40% over 5 days, indicating a high level of structural remodeling of hippocampal synaptic circuits. The developed super-resolution imaging approaches enable the examination of microglia-synapse interactions and dendritic spines with unprecedented resolution in the living brain (tissue).
43

Příprava nanočástic a jejich využití jako kontrastních látek pro in vivo zobrazování. / Preparation of nanoparticles and their use as contrast agents for in vivo imaging.

Odehnalová, Nikola January 2020 (has links)
This diploma thesis deals with the optimalization of synthesis of gold nanoparticles and their surface modification allowing their use as contrast agents for in vivo imaging by CT. Gold nanoparticles were prepared by the Turkevich method and characterized by TEM, DLS, MADLS and UV -Vis. Their surface was functionalized with polyethylene glycol containing a thiol group forming a bond with the Au atoms in the surface of gold nanoparticles. The terminal end of the polymer was methylated or containing an aminooxy group forming an orthogonal bond with hyaluronic acid using click-chemistry. The eligibility for in vivo application of the prepared nanoparticles was verified with stability and cytotoxicity tests. The nanoparticles modified by methylated polyethyleneglycol were injected intravenously into a mouse and their application potential as contrast agents were verified by CT.
44

Synthèse de sondes chémiluminescentes et profluorescentes pour des applications en imagerie in vivo / Synthesis of chemiluminescent and profluorogenic probes for in vivo imaging

Grandclaude, Virgile 23 September 2011 (has links)
L’imagerie moléculaire optique joue maintenant un rôle essentiel dans le diagnostic pré-clinique et le développement de médicaments. En effet, c’est un outil précieux dans la détection et le suivi de cellules vivantes que ce soit en utilisant de simples agents de marquage ou des sondes plus développées, dites « intelligentes » et activées uniquement par une interaction spécifique avec le bio-analyte ciblé. Ce travail de thèse a consisté à développer des outils synthétiques innovants afin d’optimiser les paramètres physico-chimiques et les propriétés optiques des sondes luminescentes. Ceci dans le but de répondre à la problématique complexe de l’imagerie dans le contexte in vivo. Nous avons notamment travaillé sur des aspects de pro-fluorescence et de chémiluminescence. De nouveaux pro-fluorophores à phénol basés sur une architecture originale de type bis-coumarinique ont été développés. De plus, nous avons mis en place une méthode d’hydrosolubilisation généralisable aux fluorophores à phénol de type coumarine et xanthène. Nos recherches en chémiluminescence ont permis la synthèse de nouveaux chémiluminophores couplés à des fluorophores organiques afin d‘augmenter l’efficacité d’émission de chémiluminescence dans le rouge. Enfin, nos travaux ont permis de mettre en place les premières « cassettes » chémiluminescentes basées sur une architecture de type 1,2-dioxétane. / Optical molecular imaging is now playing a pivotal role both in pre-clinical diagnosis and drug development. Indeed, this is a valuable tool for the real time detection and monitoring of living cells either through the use of structurally simple labels or more recently by means of sophisticated fluorescent probes, called “smart” probes and only activatable upon specific interaction with the targeted bio-analyte. The aim of this PhD work was the design of new synthetic tools aimed at optimizing physico-chemical and optical properties of fluorescent probes intended for challenging in vivo imaging applications. We have focused on the pro-fluorescence and chemiluminescence approaches. New phenol-based pro-fluorophores have been developed by using an original bis-coumarinic scaffold. In the context of the chemistry of fluorophores, we have also investigated a general method for the water-solubilisation of phenol-based fluorophore belonging to the coumarin and xanthene families. Our research in chemiluminescence has led the synthesis of new chemiluminophores covalently linked to fluorescent organic dyes aimed at increasing the emission efficiency in the red region of such chemiluminophores. Thus, the first chemiluminescent “energy transfer cassettes” based on a 1,2-dioxetane scaffold have been obtained.
45

3D handheld endoscope for optical coherence tomography of the human oral mucosa in vivo

Walther, Julia, Schnabel, Christian, Ebert, Nadja, Baumann, Michael, Koch, Edmund 06 September 2019 (has links)
The early non-invasive diagnosis of epithelial tissue alterations in daily clinical routine is still challenging. Since optical coherence tomography (OCT) shows the potential to differentiate between benign and malignant tissue of primal endothelium, OCT could be beneficial for the early diagnosis of malignancies in routine health checks. In this research, a new handheld endoscopic scanning unit was designed and connected to a spectral domain OCT system of our workgroup for the in vivo imaging of the human oral mucosa.
46

Deconstructing bioluminescence: from molecular detail to in vivo imaging.

Adams, Spencer T., Jr. 29 January 2020 (has links)
Bioluminescence is the chemical production of light that results when a luciferase enzyme catalyzes the luminogenic oxidation of a small-molecule luciferin substrate. The numerous luciferases and luciferins nature has evolved can be used to illuminate biological processes, from in vitro assays to imaging processes in live animals. However, we can improve the utility of bioluminescence through modification of these enzymes and substrates. My thesis work focuses on developing reporters that expand the bioluminescent toolkit and improving our understanding of how bioluminescence works on a molecular level. The first part of my thesis focuses on characterizing luciferases and luciferins that improve bioluminescence imaging in vivo. Some of our luciferins can outperform the natural D-luciferin substrate in live mouse imaging, while others are selectively utilized by mutant luciferases in live mouse brain. We also engineered luciferins that can selectively report on endogenous enzymatic activity in live mice. The second part of my thesis focuses on determining the molecular details of how enzymes related to firefly luciferase, long-chain fatty acyl-CoA synthetases (ACSLs), can function as latent luciferases. I have determined the structure for one of these enzymes and improved its bioluminescent activity with synthetic luciferins enough to image in live mouse brain. I also characterized the selectivity in chimerized enzymes that combine firefly luciferase and ACSLs. In summary, my work improves the utility of bioluminescence for in vivo use and informs us about how evolutionarily-related enzymes function as luciferases on a molecular level.
47

In Vivo Observations of Resident Microglia and Blood Derived Macrophages in the Brain and Spinal Cord

Evans, Teresa Ann 11 June 2014 (has links)
No description available.
48

Functional analysis of embryonic brain development in Tribolium castaneum / Funktionale Analyse zur embryonalen Gehirnentwicklung in Tribolium castaneum

Koniszewski, Nikolaus 22 August 2011 (has links)
No description available.
49

In vivo diffusion tensor imaging (DTI) for the human heart under free-breathing conditions / Tenseur de diffusion d'imagerie (DTI) in vivo pour le cœur de l'homme dans des conditions de libre respiration

Wei, Hongjiang 20 November 2013 (has links)
L'orientation des fibres myocardiaque est à la base du comportement électro-mécanique du cœur, et connue pour être altérée dans diverses maladies cardiaques telles que la cardiopathie ischémique et l'hypertrophie ventriculaire. Cette thèse porte principalement sur l'imagerie in vivo du tenseur de diffusion (diffusion tensor imaging—DTI) en vue d’obtenir la structure des fibres myocardiques du cœur humain dans des conditions de respiration libre. L'utilisation de DTI pour l'étude du cœur humain in vivo est un grand défi en raison du mouvement cardiaque. En particulier, l’acquisition DTI avec respiration libre sans recourir au gating respiratoire est très difficile à cause des mouvements à a fois respiratoire et cardiaque. Pour aborder ce problème, nous proposons de nouvelles approches consistant à combiner des acquisitions à retards de déclenchement multiples (trigger delay—TD) et des méthodes de post-traitement. D’abord, nous réalisons des acquisitions avec multiples TD décalés en fin de diastole. Ensuite, nous développons deux méthodes de post-traitement. La première méthode s’attaque au problème d’effets de mouvement physiologique sur DTI cardiaque in vivo en utilisant les techniques de recalage et de PCATMIP (Principal Components Analysis filtering and Temporal Maximum Intensity Projection). La deuxième méthode traite le problème de mouvement par l’utilisation d’un algorithme de fusion d’images basé sur l’ondelette (wavelet-based image fusion-WIF) et d’une technique de débruitage PCA (Principal Components Analysis). Enfin, une comparaison des mesures DTI entre la méthode PCATMIP et la méthode WIF est réalisée ; les champs de tenseurs sont calculés, à partir desquels les propriétés de l’architecture des fibres in vivo sont comparées. Les résultats montrent qu’en utilisant les approches proposées, il est possible d’étudier l’impact du mouvement cardiaque sur les paramètres de tenseur de diffusion, et d’explorer les relations sous-jacentes entre les propriétés de tenseur de diffusion mesurées et le mouvement cardiaque. Nous trouvons aussi que la combinaison des acqusiitions avec des TD multiples décalés and des post-traitements d’images peut compenser les effets de mouvement physiologique, ce qui permet d’obtenir l’architecture 3D du cœur humain dans des conditions de respiration libre. Les résultats suggèrent de nouvelles solutions au problème de perte du signal due au mouvement, qui sont prometteuses pour obtenir les propriétés de l’architecture des fibres myocardiques du cœur humain in vivo, dans des conditions cliniques. / The orientation of cardiac fibers underlies the electro-mechanical behavior of the heart, and it is known to be altered in various cardiac diseases such as ischemic heart disease and ventricular hypertrophy. This thesis mainly focuses on in vivo diffusion tensor imaging (DTI) to obtain the myocardial fiber structure of the human heart under free-breathing conditions. The use of DTI for studying the human heart in vivo is challenging due to cardiac motion. In particular, free-breathing DTI acquisition without resorting to respiratory gating is very difficult due to both respiratory and cardiac motion. To deal with this problem, we propose novel approaches that combine multiple shifted trigger delay (TD) acquisitions and post-processing methods. First, we perform multiple shifted TD acquisitions at end diastole. Then, we focus on two different post-processing methods. The first method addresses physiological motion effects on in vivo cardiac DTI using image co-registration and PCATMIP (Principal Components Analysis filtering and Temporal Maximum Intensity Projection). The second method is a wavelet-based image fusion (WIF) algorithm combined with a PCA noise removing method. Finally, a comparison of DTI measurements between the PCATMIP and WIF methods is also performed; tensor fields are calculated, from which the in vivo fiber architecture properties are compared. The results show that using the proposed approaches, we are able to study the cardiac motion effects on diffusion tensor parameters, and investigate the underlying relationship between the measured diffusion tensor properties and the cardiac motion. We also find that the combination of multiple shifted TD acquisitions and dedicated image post-processing can compensate for physiological motion effects, which allows us to obtain 3D fiber architectures of the human heart under free-breathing conditions. The findings suggest new solutions to signal loss problems associated with bulk motion, which are promising for obtaining in vivo human myocardial fiber architecture properties in clinical conditions.
50

Cerebellar Development and Neurogenesis in Zebrafish

Kaslin, Jan, Brand, Michael 19 March 2019 (has links)
Cerebellar organization and function have been studied in numerous species of fish. Fish models such as goldfish and weakly electric fish have led to important findings about the cerebellar architecture, cerebellar circuit physiology and brain evolution. However, most of the studied fish models are not well suited for developmental and genetic studies of the cerebellum. The rapid transparent ex utero development in zebrafish allows direct access and precise visualization of all the major events in cerebellar development. The superficial position of the cerebellar primordium and cerebellum further facilitates in vivo imaging of cerebellar structures and developmental events at single cell resolution. Furthermore, zebrafish is amenable to high-throughput screening techniques and forward genetics because of its fecundity and easy keeping. Forward genetics screens in zebrafish have resulted in several isolated cerebellar mutants and substantially contributed to the understanding of the genetic networks involved in hindbrain development (Bae et al. 2009; Brand et al. 1996). Recent developments in genetic tools, including the use of site specific recombinases, efficient transgenesis, inducible gene expression systems, and the targeted genome lesioning technologies TALEN and Cas9/CRISPR has opened up new avenues to manipulate and edit the genome of zebrafish (Hans et al. 2009; Scott 2009; Housden et al. 2016; Li et al. 2016)}. These tools enable the use of genome-wide genetic approaches, such as enhancer/exon traps and cell specific temporal control of gene expression in zebrafish. Several seminal papers have used these technologies to successfully elucidate mechanisms involved in the morphogenesis, neurogenesis and cell migration in the cerebellum (Bae et al. 2009; Chaplin et al. ; Hans et al. 2009; Volkmann et al. ; Volkmann et al. 2008). In addition, the use of genetically encoded sensors and probes that allows detection and manipulation of neuronal activity using optical methods have open up new means to study the physiology and function of the cerebellum (Simmich et al. 2012; Matsui et al. 2014). Taken together, these features have allowed zebrafish to emerge as a complete model for studies of molecular, cellular and physiological mechanisms involved in cerebellar development and function at both cell and circuit level.

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