RESUMEN
The resolution of fluorescence microscopy images is limited by the physical properties of light. In the last decade, numerous super-resolution microscopy (SRM) approaches have been proposed to deal with such hindrance. Here we present Mean-Shift Super Resolution (MSSR), a new SRM algorithm based on the Mean Shift theory, which extends spatial resolution of single fluorescence images beyond the diffraction limit of light. MSSR works on low and high fluorophore densities, is not limited by the architecture of the optical setup and is applicable to single images as well as temporal series. The theoretical limit of spatial resolution, based on optimized real-world imaging conditions and analysis of temporal image stacks, has been measured to be 40 nm. Furthermore, MSSR has denoising capabilities that outperform other SRM approaches. Along with its wide accessibility, MSSR is a powerful, flexible, and generic tool for multidimensional and live cell imaging applications.
Asunto(s)
Algoritmos , Medicamentos Genéricos , Sistemas de Lectura , Microscopía Fluorescente , Colorantes FluorescentesRESUMEN
Rotavirus genome replication and assembly take place in cytoplasmic electron dense inclusions termed viroplasms (VPs). Previous conventional optical microscopy studies observing the intracellular distribution of rotavirus proteins and their organization in VPs have lacked molecular-scale spatial resolution, due to inherent spatial resolution constraints. In this work we employed super-resolution microscopy to reveal the nanometric-scale organization of VPs formed during rotavirus infection, and quantitatively describe the structural organization of seven viral proteins within and around the VPs. The observed viral components are spatially organized as five concentric layers, in which NSP5 localizes at the center of the VPs, surrounded by a layer of NSP2 and NSP4 proteins, followed by an intermediate zone comprised of the VP1, VP2, VP6. In the outermost zone, we observed a ring of VP4 and finally a layer of VP7. These findings show that rotavirus VPs are highly organized organelles.
Asunto(s)
Células Epiteliales/virología , Rotavirus/crecimiento & desarrollo , Proteínas Virales/análisis , Replicación Viral , Animales , Línea Celular , Macaca mulatta , Microscopía Fluorescente , Análisis EspacialRESUMEN
Tracing tubular structures from biomedical images is important for a wide range of applications. Particularly, the spermatozoon is an essential cell whose flagella have a tubular form. Its main function is to fertilize the egg, and the flagellum is fundamental to achieve this task which depends importantly on the dynamics of intracellular calcium ([Ca2+]i). Measuring [Ca2+]i along the flagellum in 3-D is not a simple matter since it requires: 1) sophisticated fluorescence imaging techniques dealing with low intensity and signal to noise ratio (SNR) and 2) tracing the flagellum's centerline. Most of the algorithms proposed to trace tubular structures have been developed for multi-branch structures not being adequate for single tubular structures with low SNR. Taking into account the prior knowledge that the flagellum is constituted by a single tubular structure, we propose an automatic method to trace and track multiple single tubular structures from 3-D images. First, an algorithm based on one-class classification allows enhancement of the flagellum. This enhanced 3-D image permits guiding an iterative centerline algorithm toward the flagellum's centerline. Each sperm is assigned an ID to keep track of it in 3-D . Our algorithm was quantitatively evaluated using a ground truth 564 semi-manual traces (six 3-D image stacks) comparing them to those obtained from state-of-the-art tubular structure centerline extraction algorithms. The qualitative and quantitative results show that our algorithm is extracting similar traces as compared with ground truth, and it is more robust and accurate to trace the flagellum's centerline than multi-branch algorithms.
Asunto(s)
Imagenología Tridimensional/métodos , Imagen Óptica/métodos , Cola del Espermatozoide/fisiología , Algoritmos , Humanos , MasculinoRESUMEN
Viruses employ a variety of strategies to hijack cellular activities through the orchestrated recruitment of macromolecules to specific virus-induced cellular micro-environments. Adenoviruses (Ad) and other DNA viruses induce extensive reorganization of the cell nucleus and formation of nuclear Replication Compartments (RCs), where the viral genome is replicated and expressed. In this work an automatic algorithm designed for detection and segmentation of RCs using ellipses is presented. Unlike algorithms available in the literature, this approach is deterministic, automatic, and can adjust multiple RCs using ellipses. The proposed algorithm is non iterative, computationally efficient and is invariant to affine transformations. The method was validated over both synthetic images and more than 400 real images of Ad-infected cells at various timepoints of the viral replication cycle obtaining relevant information about the biogenesis of adenoviral RCs. As proof of concept the algorithm was then used to quantitatively compare RCs in cells infected with the adenovirus wild type or an adenovirus mutant that is null for expression of a viral protein that is known to affect activities associated with RCs that result in deficient viral progeny production.