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Advances in 3D single particle localization microscopy
Author(s) -
Yongzhuang Zhou,
Michael Handley,
Guillem Carles,
Andrew R. Harvey
Publication year - 2019
Publication title -
apl photonics
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.094
H-Index - 34
ISSN - 2378-0967
DOI - 10.1063/1.5093310
Subject(s) - microscopy , resolution (logic) , photoactivated localization microscopy , super resolution microscopy , image resolution , optical microscope , optics , diffraction , focus (optics) , light sheet fluorescence microscopy , materials science , physics , computer science , scanning confocal electron microscopy , artificial intelligence , scanning electron microscope
The spatial resolution of conventional optical microscopy is limited by diffraction to transverse and axial resolutions of about 250 nm, but localization of point sources, such as single molecules or fluorescent beads, can be achieved with a precision of 10 nm or better in each direction. Traditional approaches to localization microscopy in two dimensions enable high precision only for a thin in-focus layer that is typically much less than the depth of a cell. This precludes, for example, super-resolution microscopy of extended three-dimensional biological structures or mapping of blood velocity throughout a useful depth of vasculature. Several techniques have been reported recently for localization microscopy in three dimensions over an extended depth range. We describe the principles of operation and typical applications of the most promising 3D localization microscopy techniques and provide a comparison of the attainable precision for each technique in terms of the Cramer-Rao lower bound for high-resolution imaging.

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