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3D sub-diffraction imaging in a conventional confocal configuration by exploiting super-linear emitters

journal contribution
posted on 2024-11-02, 04:21 authored by Denitza Denkova, Martin Plöschner, Minakshi Das, Lindsay Parker, Xianlin Zheng, Yiqing Lu, Antony Orth, Nicolle Packer, James Piper
Sub-diffraction microscopy enables bio-imaging with unprecedented clarity. However, most super-resolution methods require complex, costly purpose-built systems, involve image post-processing and struggle with sub-diffraction imaging in 3D. Here, we realize a conceptually different super-resolution approach which circumvents these limitations and enables 3D sub-diffraction imaging on conventional confocal microscopes. We refer to it as super-linear excitation-emission (SEE) microscopy, as it relies on markers with super-linear dependence of the emission on the excitation power. Super-linear markers proposed here are upconversion nanoparticles of NaYF4, doped with 20% Yb and unconventionally high 8% Tm, which are conveniently excited in the near-infrared biological window. We develop a computational framework calculating the 3D resolution for any viable scanning beam shape and excitation-emission probe profile. Imaging of colominic acid-coated upconversion nanoparticles endocytosed by neuronal cells, at resolutions twice better than the diffraction limit both in lateral and axial directions, illustrates the applicability of SEE microscopy for sub-cellular biology.

Funding

ARC Centre of Excellence for Nanoscale BioPhotonics

Australian Research Council

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History

Journal

Nature Communications

Volume

10

Number

3695

Issue

1

Start page

1

End page

12

Total pages

12

Publisher

Nature

Place published

United Kingdom

Language

English

Copyright

© 2019, Crown. Open Access This article is licensed under a Creative Commons Attribution 4.0 International License

Former Identifier

2006094144

Esploro creation date

2020-06-22

Fedora creation date

2020-04-09

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