Open Access
Multi-label in vivo STED microscopy by parallelized switching of reversibly switchable fluorescent proteins
Katrin I. Willig
1, 2
,
Waja Wegner
2, 3
,
Antonia M.S. Müller
1, 2
,
Valérie Clavet Fournier
1, 2, 4
,
H. Steffens
2, 3
4
Göttingen Graduate Center for Neurosciences, Biophysics, und Molecular Biosciences (GGNB), Göttingen, Germany
|
Publication type: Journal Article
Publication date: 2021-06-01
scimago Q1
wos Q1
SJR: 3.796
CiteScore: 12.9
Impact factor: 6.9
ISSN: 22111247, 26391856
PubMed ID:
34077731
General Biochemistry, Genetics and Molecular Biology
Abstract
Despite the tremendous success of super-resolution microscopy, multi-color in vivo applications are still rare. Here we present live-cell multi-label STED microscopy in vivo and in vitro by combining spectrally separated excitation and detection with temporal sequential imaging of reversibly switchable fluorescent proteins (RSFPs). Triple-label STED microscopy resolves pre- and postsynaptic nano-organizations in vivo in mouse visual cortex employing EGFP, Citrine, and the RSFP rsEGP2. Combining the positive and negative switching RSFPs Padron and Dronpa-M159T enables dual-label STED microscopy. All labels are recorded quasi-simultaneously by parallelized on- and off-switching of the RSFPs within the fast-scanning axis. Depletion is performed by a single STED beam so that all channels automatically co-align. Such an addition of a second or third marker merely requires a switching laser, minimizing setup complexity. Our technique enhances in vivo STED microscopy, making it a powerful tool for studying multiple synaptic nano-organizations or the tripartite synapse in vivo.
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Total citations:
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Citations from 2025:
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GOST
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Willig K. I. et al. Multi-label in vivo STED microscopy by parallelized switching of reversibly switchable fluorescent proteins // Cell Reports. 2021. Vol. 35. No. 9. p. 109192.
GOST all authors (up to 50)
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Willig K. I., Wegner W., Müller A. M., Clavet Fournier V., Steffens H. Multi-label in vivo STED microscopy by parallelized switching of reversibly switchable fluorescent proteins // Cell Reports. 2021. Vol. 35. No. 9. p. 109192.
Cite this
RIS
Copy
TY - JOUR
DO - 10.1016/j.celrep.2021.109192
UR - https://doi.org/10.1016/j.celrep.2021.109192
TI - Multi-label in vivo STED microscopy by parallelized switching of reversibly switchable fluorescent proteins
T2 - Cell Reports
AU - Willig, Katrin I.
AU - Wegner, Waja
AU - Müller, Antonia M.S.
AU - Clavet Fournier, Valérie
AU - Steffens, H.
PY - 2021
DA - 2021/06/01
PB - Elsevier
SP - 109192
IS - 9
VL - 35
PMID - 34077731
SN - 2211-1247
SN - 2639-1856
ER -
Cite this
BibTex (up to 50 authors)
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@article{2021_Willig,
author = {Katrin I. Willig and Waja Wegner and Antonia M.S. Müller and Valérie Clavet Fournier and H. Steffens},
title = {Multi-label in vivo STED microscopy by parallelized switching of reversibly switchable fluorescent proteins},
journal = {Cell Reports},
year = {2021},
volume = {35},
publisher = {Elsevier},
month = {jun},
url = {https://doi.org/10.1016/j.celrep.2021.109192},
number = {9},
pages = {109192},
doi = {10.1016/j.celrep.2021.109192}
}
Cite this
MLA
Copy
Willig, Katrin I., et al. “Multi-label in vivo STED microscopy by parallelized switching of reversibly switchable fluorescent proteins.” Cell Reports, vol. 35, no. 9, Jun. 2021, p. 109192. https://doi.org/10.1016/j.celrep.2021.109192.