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Concepts for structured illumination microscopy with extended axial resolution through mirrored illumination

Permanent link
https://hdl.handle.net/10037/24888
DOI
https://doi.org/10.1364/BOE.382398
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Date
2020-03-20
Type
Journal article
Tidsskriftartikkel
Peer reviewed

Author
Manton, James D.; Ströhl, Florian; Fiolka, Reto; Kaminski, Clemens F.; Rees, Eric J.
Abstract
Wide-field fluorescence microscopy, while much faster than confocal microscopy, suffers from a lack of optical sectioning and poor axial resolution. 3D structured illumination microscopy (SIM) has been demonstrated to provide optical sectioning and to double the resolution limit both laterally and axially, but even with this the axial resolution is still worse than the lateral resolution of unmodified wide-field microscopy. Interferometric schemes using two high numerical aperture objectives, such as 4Pi confocal and I5M microscopy, have improved the axial resolution beyond that of the lateral, but at the cost of a significantly more complex optical setup. Here, we theoretically and numerically investigate a simpler dual-objective scheme which we propose can be easily added to an existing 3D-SIM microscope, providing lateral and axial resolutions in excess of 125 nm with conventional fluorophores and without the need for interferometric detection.
Publisher
Optica
Citation
Manton, Ströhl, Fiolka, Kaminski, Rees. Concepts for structured illumination microscopy with extended axial resolution through mirrored illumination. Biomedical Optics Express. 2020;11(4):2098-2108
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  • Artikler, rapporter og annet (fysikk og teknologi) [1057]
Copyright 2020 The Author(s)

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