2016
DOI: 10.1007/978-3-319-46527-2_8
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Lung Imaging in Animal Models

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Cited by 2 publications
(7 citation statements)
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“…The selectivity for specific wavelengths facilitates the visualization of different fluorescent objects as a bright structure against a dark background (Lichtman and Conchello, 2005 ; Lindon et al, 2016 ). Although fluorescence microscopy has been widely used to study tissues in vivo (Lindon et al, 2016 ), its application in lung IVM is limited to superficial layers and low resolution (Witte, 1992 ; Presson et al, 2011 ; Lefrançais et al, 2017 ).…”
Section: Setupmentioning
confidence: 99%
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“…The selectivity for specific wavelengths facilitates the visualization of different fluorescent objects as a bright structure against a dark background (Lichtman and Conchello, 2005 ; Lindon et al, 2016 ). Although fluorescence microscopy has been widely used to study tissues in vivo (Lindon et al, 2016 ), its application in lung IVM is limited to superficial layers and low resolution (Witte, 1992 ; Presson et al, 2011 ; Lefrançais et al, 2017 ).…”
Section: Setupmentioning
confidence: 99%
“…Both laser scanning and spinning disk confocal microscopes pass a single beam of laser light through the pinhole. It should be noted that while confocal laser scanning microscopy focuses the light through one small pinhole in order to sequentially scan the sample point by point, confocal spinning disk microscopy exploits multiple pinholes for simultaneous confocal illumination (Masedunskas et al, 2012 ; Sanderson et al, 2014 ; Lefrançais et al, 2017 ). Therefore, either X–Y-deflection of the laser or a spinning disk with a spatial array of pinholes and automated-focus (z-axis) control enables the visualization of sequential optical sections of the specimen and three-dimensional images.…”
Section: Setupmentioning
confidence: 99%
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