Macromolecular crowding is crucial for cellular homeostasis. In vivo studies of macromolecular crowding and ultimately water-dynamics are needed to understand their role in cellular fates. The macromolecular crowding in the lens is essential for understanding normal optics of the lens, and moreover for understanding and prevention of cataract and presbyopia. Here we combine the use of the water nano-environmentally sensitive sensor (6-acetyl-2-dimethylaminonaphthalene, ACDAN) with in vivo studies of Aquaporin zero zebrafish mutants to understand the lens macromolecular crowding. Spectral phasor analysis of ACDAN fluorescence reveal the extent of water dipolar relaxation and demonstrate that the mutations in the duplicated zebrafish Aquaporin 0s, Aqp0a and Aqp0b, alter the water state and macromolecular crowding in the living zebrafish lens. Our results provide in vivo evidence that Aqp0a promotes fluid influx in the deeper lens cortex, whereas Aqp0b facilitates fluid efflux. This work opens new perspectives for in vivo studies on macromolecular crowding.
Cardiac myocytes constitute a unique physiological system. They are the muscle cells that build up heart tissue and provide the force to pump blood by synchronously contracting at every beat. This contraction is regulated by calcium concentration, among other ions, which exhibits a very complex behaviour, rich in dynamical states at the molecular, cellular and tissue levels. Details of such dynamical patterns are closely related to the mechanisms responsible for cardiac function and also cardiac disease, which is the first cause of death in the modern world. The emerging field of translational cardiology focuses on the study of how such mechanisms connect and influence each other across spatial and temporal scales finally yielding to a certain clinical condition. In order to study such patterns, we benefit from the recent and very important advances in the field of experimental cell physiology. In particular, fluorescence microscopy allows us to observe the distribution of calcium in the cell with a spatial resolution below the micron and a frame rate around the millisecond, thus providing a very accurate monitoring of calcium fluxes in the cell. This thesis is the result of over five years' work on biological signal and digital image processing of cardiac cells. During this period of time the aim has been to develop computational techniques for extracting quantitative data of physiological relevance from microscopy images at different scales. The two main subjects covered in the thesis are image segmentation and classification methods applied to fluorescence microscopy imaging of cardiac myocytes. These methods are applied to a variety of problems involving different space and time scales such as the localisation of molecular receptors, the detection and characterisation of spontaneous calcium-release events and the propagation of calcium waves across a culture of cardiac cells. The experimental images and data have been provided by four internationally renowned collaborators in the field. It is thanks to them and their teams that this thesis has been possible. They are Dr. Leif Hove-Madsen from the Institut de Ciències Cardiovasculars de Catalunya in Barcelona, Prof. S. R. Wayne Chen from the Department of Physiology and Pharmacology in the Libin Cardiovascular Institute of Alberta, University of Calgary, Dr. Peter P. Jones from the Department of Physiology in the University of Otago, and Prof. Glen Tibbits from the Department of Biomedical Physiology & Kinesiology at the Simon Fraser University in Vancouver. The work belongs to the biomedical engineering discipline, focusing on the engineering perspective by applying physics and mathematics to solve biomedical problems. Specifically, we frame our contributions in the field of computational translational cardiology, attempting to connect molecular mechanisms in cardiac cells up to cardiac disease by developing signal and image-processing methods and machine-learning methods that are scalable through the different scales. This computational approach allows for a quantitative, robust and reproducible analysis of the experimental data and allows us to obtain results that otherwise would not be possible by means of traditional manual methods. The results of the thesis provide specific insight into different cell mechanisms that have a non-negligible impact at the clinical level. In particular, we gain a deeper knowledge of cell mechanisms related to cardiac arrhythmia, fibrillation phenomena, the emergence of alternans and anomalies in calcium handling due to cell ageing. Els cardiomiòcits constitueixen un sistema fisiològic únic. Són les cèl·lules muscular que formen el cor i proporcionen la força per bombar la sang fent una contracció a cada batec. La regulació d'aquesta contracció es fa mitjançant concentració de calci (entre d'altres ions) i presenta una dinàmica molt complexa tant a l'escala molecular, cel·lular i de teixit. Detalls d'aquesta dinàmica estan fortament relacionats amb la funció cardíaca i per sobre de tot amb patologies cardíaques. La disciplina emergent de la cardiologia translacional es centra en l'estudi de com aquests mecanismes es connecten i s'influencien entre sí a través de diferents escales temporals i espacials finalment donant lloc a condicions clíniques. Per estudiar aquests patrons ens beneficiem dels recents avenços en fisiologia i biologia cel·lular. En particular, la microscòpia de fluorescència ens permet observar la distribució de calci dins una cèl·lula amb una resolució espacial per sota de la micra i temporal per sota del mil·lisegon, permetent un monitoratge acurat dels fluxos de calci en la cèl·lula cardíaca. Aquesta tesi és el resultat de més de cinc anys de feina en processament de senyal i imatge de cardiomiòcits humans. Durant aquest període de temps l'objectiu principal ha estat desenvolupar tècniques computacionals per extraure dades d'imatges de microscòpia amb rellevància fisiològica. Els dos temes principals coberts a la tesi són segmentació d'imatges i classificadors, aplicats a imatges de microscòpia de fluorescència de cardiomiòcits. Els mètodes s'apliquen a diferents problemes involucrant diverses escales espacials i temporals, des de determinar la posició de receptors a l’escala molecular passant detectar i caracteritzar alliberament espontani de calci intracel·lular fins a la propagació d'ones de calci en un cultiu de cèl·lules cardíaques. Les dades experimentals han estat proporcionades per quatre col·laboradors de renom internacional. És gràcies a ells i els seus equips que aquesta tesi ha estat possible. Són el Dr. Leif Hove-Madsen de l'Institut de Ciències Cardiovasculars de Catalunya a Barcelona, el Dr. S.R. Wayne Chen del Department of Physiology and Pharmacology al Libin Cardiovascular Institute of Alberta, University of Calgary, el Dr. Peter P. Jones del Department of Physiology a la University of Otago, i el Dr. Glen Tibbits del Department of Biomedical Physiology & Kinesiology de la Simon Fraser University a Vancouver. El treball pertany a la disciplina de la enginyeria biomèdica, fent èmfasi a la perspectiva de l'enginyeria, aplicant física i matemàtiques per solucionar problemes de la biomedicina. Específicament, s'emmarca en la cardiologia translacional computacional, mirant de connectar mecanismes a l’escala molecular amb patologies cardíaques mitjançant tècniques de processament de dades i aprenentatge automàtic que són escalables a les diferents escales d’aplicació. Aquest enfocament computacional permet una anàlisi quantitatiu, robust i reproduïble de les dades experimentals i ens permet d'obtenir resultats que serien impossibles d'assolir mitjançant els tradicionals mètodes manuals. Els resultats que proporciona la tesi han permès aprofundir en l'enteniment de diferents mecanismes fisiològics amb impacte en l'àmbit clínic. Particularment hem permès d’assolir coneixements relacionats amb l'arítmia cardíaca, la fibril·lació, processos d'alternança i anomalies relacionades amb l’envelliment.
starved condition. The obtained super-resolution and diffusion maps exhibit differential localization and mobility of fatty acids upon cell-starvation, suggesting a link between fatty acid distribution and metabolic state of a cell. This differential localization of fatty acids upon starvation is physiologically relevant and hints towards a spatial protection mechanism against lipotoxicity. Our approach of using red-shifted states of conventional BODIPY probes for super-resolution microscopy in living cells opens up new avenues for studying cellular processes at the nanoscopic length scale. Single molecule tracking and localization has become a powerful strategy for noninvasive imaging of nanoscale structures in biology. The aim of this study is to develop a scanning astigmatism module for 3D Stochastic-Optical-Reconstruction-Microscopy (STORM). For 3D STORM imaging, a weak cylindrical lens is placed in the imaging path to induce astigmatism. The specific location of the lens in the optical path can affect the extent of correction and in our approach, the ability to scan the lens position allows for finer control and thus optimization for the reconstruction. Our design uses an Arduino-based circuit along with a stepper motor controlled by a Python interface to position the cylindrical lens. The ellipticity and orientation of fluorophores' localization are obtained using the ImageJ data analysis plugin ThunderSTORM. We demonstrate the feasibility of this approach through 3D reconstruction of the mitochondrial morphology of HeLa cells. Improvement in the visualization of cellular structures and their relationships with nanoscale resolution in all three dimensions will contribute to a better understanding of molecular processes occurring in cells.
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