Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes

The basic research in cell biology and in medical sciences makes large use of imaging tools mainly based on confocal fluorescence and, more recently, on non-linear excitation microscopy. Substantially the aim is the recognition of selected targets in the image and their tracking in time. We have dev...

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Autores principales: Villa, Carlo E., Caccia, Michele, Sironi, Laura, D'Alfonso, Laura, Collini, Maddalena, Rivolta, Ilaria, Miserocchi, Giuseppe, Gorletta, Tatiana, Zanoni, Ivan, Granucci, Francesca, Chirico, Giuseppe
Formato: Texto
Lenguaje:English
Publicado: Public Library of Science 2010
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2923183/
https://www.ncbi.nlm.nih.gov/pubmed/20808918
http://dx.doi.org/10.1371/journal.pone.0012216
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author Villa, Carlo E.
Caccia, Michele
Sironi, Laura
D'Alfonso, Laura
Collini, Maddalena
Rivolta, Ilaria
Miserocchi, Giuseppe
Gorletta, Tatiana
Zanoni, Ivan
Granucci, Francesca
Chirico, Giuseppe
author_facet Villa, Carlo E.
Caccia, Michele
Sironi, Laura
D'Alfonso, Laura
Collini, Maddalena
Rivolta, Ilaria
Miserocchi, Giuseppe
Gorletta, Tatiana
Zanoni, Ivan
Granucci, Francesca
Chirico, Giuseppe
author_sort Villa, Carlo E.
collection PubMed
description The basic research in cell biology and in medical sciences makes large use of imaging tools mainly based on confocal fluorescence and, more recently, on non-linear excitation microscopy. Substantially the aim is the recognition of selected targets in the image and their tracking in time. We have developed a particle tracking algorithm optimized for low signal/noise images with a minimum set of requirements on the target size and with no a priori knowledge of the type of motion. The image segmentation, based on a combination of size sensitive filters, does not rely on edge detection and is tailored for targets acquired at low resolution as in most of the in-vivo studies. The particle tracking is performed by building, from a stack of Accumulative Difference Images, a single 2D image in which the motion of the whole set of the particles is coded in time by a color level. This algorithm, tested here on solid-lipid nanoparticles diffusing within cells and on lymphocytes diffusing in lymphonodes, appears to be particularly useful for the cellular and the in-vivo microscopy image processing in which few a priori assumption on the type, the extent and the variability of particle motions, can be done.
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spelling pubmed-29231832010-08-31 Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes Villa, Carlo E. Caccia, Michele Sironi, Laura D'Alfonso, Laura Collini, Maddalena Rivolta, Ilaria Miserocchi, Giuseppe Gorletta, Tatiana Zanoni, Ivan Granucci, Francesca Chirico, Giuseppe PLoS One Research Article The basic research in cell biology and in medical sciences makes large use of imaging tools mainly based on confocal fluorescence and, more recently, on non-linear excitation microscopy. Substantially the aim is the recognition of selected targets in the image and their tracking in time. We have developed a particle tracking algorithm optimized for low signal/noise images with a minimum set of requirements on the target size and with no a priori knowledge of the type of motion. The image segmentation, based on a combination of size sensitive filters, does not rely on edge detection and is tailored for targets acquired at low resolution as in most of the in-vivo studies. The particle tracking is performed by building, from a stack of Accumulative Difference Images, a single 2D image in which the motion of the whole set of the particles is coded in time by a color level. This algorithm, tested here on solid-lipid nanoparticles diffusing within cells and on lymphocytes diffusing in lymphonodes, appears to be particularly useful for the cellular and the in-vivo microscopy image processing in which few a priori assumption on the type, the extent and the variability of particle motions, can be done. Public Library of Science 2010-08-17 /pmc/articles/PMC2923183/ /pubmed/20808918 http://dx.doi.org/10.1371/journal.pone.0012216 Text en Villa et al. http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Villa, Carlo E.
Caccia, Michele
Sironi, Laura
D'Alfonso, Laura
Collini, Maddalena
Rivolta, Ilaria
Miserocchi, Giuseppe
Gorletta, Tatiana
Zanoni, Ivan
Granucci, Francesca
Chirico, Giuseppe
Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes
title Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes
title_full Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes
title_fullStr Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes
title_full_unstemmed Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes
title_short Accumulative Difference Image Protocol for Particle Tracking in Fluorescence Microscopy Tested in Mouse Lymphonodes
title_sort accumulative difference image protocol for particle tracking in fluorescence microscopy tested in mouse lymphonodes
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC2923183/
https://www.ncbi.nlm.nih.gov/pubmed/20808918
http://dx.doi.org/10.1371/journal.pone.0012216
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