Abstract:The spatial resolution of images of living samples obtained by fluorescence microscopes is physically limited due to the diffraction of visible light, which makes the study of entities of size less than the diffraction barrier (around 200 nm in the x-y plane) very challenging. To overcome this limitation, several deconvolution and super-resolution techniques have been proposed. Within the framework of inverse problems, modern approaches in fluorescence microscopy reconstruct a superresolved image from a tempor… Show more
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