Correlative 3D microscopy of single cells using super-resolution and scanning ion-conductance microscopy

High-resolution live-cell imaging is necessary to study complex biological phenomena. Modern fluorescence microscopy methods are increasingly combined with complementary, label-free techniques to put the fluorescence information into the cellular context. The most common high-resolution imaging appr...

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Main Authors: Navikas, Vytautas (Author) , Leitao, Samuel M. (Author) , Grußmayer, Kristin Stefanie (Author) , Descloux, Adrien (Author) , Drake, Barney (Author) , Yserentant, Klaus (Author) , Werther, Philipp (Author) , Herten, Dirk-Peter (Author) , Wombacher, Richard (Author) , Radenovic, Aleksandra (Author) , Fantner, Georg E. (Author)
Format: Article (Journal)
Language:English
Published: JUL 27 2021
In: Nature Communications
Year: 2021, Volume: 12, Pages: 1-9
ISSN:2041-1723
DOI:10.1038/s41467-021-24901-3
Online Access:Verlag, lizenzpflichtig, Volltext: https://doi.org/10.1038/s41467-021-24901-3
Verlag, lizenzpflichtig, Volltext: https://www.nature.com/articles/s41467-021-24901-3
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Author Notes:Vytautas Navikas, Samuel M. Leitao, Kristin S. Grussmayer, Adrien Descloux, Barney Drake, Klaus Yserentant, Philipp Werther, Dirk-Peter Herten, Richard Wombacher, Aleksandra Radenovic & Georg E. Fantner

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520 |a High-resolution live-cell imaging is necessary to study complex biological phenomena. Modern fluorescence microscopy methods are increasingly combined with complementary, label-free techniques to put the fluorescence information into the cellular context. The most common high-resolution imaging approaches used in combination with fluorescence imaging are electron microscopy and atomic-force microscopy (AFM), originally developed for solid-state material characterization. AFM routinely resolves atomic steps, however on soft biological samples, the forces between the tip and the sample deform the fragile membrane, thereby distorting the otherwise high axial resolution of the technique. Here we present scanning ion-conductance microscopy (SICM) as an alternative approach for topographical imaging of soft biological samples, preserving high axial resolution on cells. SICM is complemented with live-cell compatible super-resolution optical fluctuation imaging (SOFI). To demonstrate the capabilities of our method we show correlative 3D cellular maps with SOFI implementation in both 2D and 3D with self-blinking dyes for two-color high-order SOFI imaging. Finally, we employ correlative SICM/SOFI microscopy for visualizing actin dynamics in live COS-7 cells with subdiffraction-resolution. 
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