Literature DB >> 28847959

Adaptive-illumination STED nanoscopy.

Jörn Heine1, Matthias Reuss1, Benjamin Harke1, Elisa D'Este2, Steffen J Sahl2, Stefan W Hell3,4.   

Abstract

The concepts called STED/RESOLFT superresolve features by a light-driven transfer of closely packed molecules between two different states, typically a nonfluorescent "off" state and a fluorescent "on" state at well-defined coordinates on subdiffraction scales. For this, the applied light intensity must be sufficient to guarantee the state difference for molecules spaced at the resolution sought. Relatively high intensities have therefore been applied throughout the imaging to obtain the highest resolutions. At regions where features are far enough apart that molecules could be separated with lower intensity, the excess intensity just adds to photobleaching. Here, we introduce DyMIN (standing for Dynamic Intensity Minimum) scanning, generalizing and expanding on earlier concepts of RESCue and MINFIELD to reduce sample exposure. The principle of DyMIN is that it only uses as much on/off-switching light as needed to image at the desired resolution. Fluorescence can be recorded at those positions where fluorophores are found within a subresolution neighborhood. By tuning the intensity (and thus resolution) during the acquisition of each pixel/voxel, we match the size of this neighborhood to the structures being imaged. DyMIN is shown to lower the dose of STED light on the scanned region up to ∼20-fold under common biological imaging conditions, and >100-fold for sparser 2D and 3D samples. The bleaching reduction can be converted into accordingly brighter images at <30-nm resolution.

Keywords:  STED microscopy; adaptive illumination; fluorescence nanoscopy; photobleaching; superresolution

Year:  2017        PMID: 28847959      PMCID: PMC5604029          DOI: 10.1073/pnas.1708304114

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  20 in total

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2.  Macromolecular-scale resolution in biological fluorescence microscopy.

Authors:  Gerald Donnert; Jan Keller; Rebecca Medda; M Alexandra Andrei; Silvio O Rizzoli; Reinhard Lührmann; Reinhard Jahn; Christian Eggeling; Stefan W Hell
Journal:  Proc Natl Acad Sci U S A       Date:  2006-07-24       Impact factor: 11.205

3.  Controlled light-exposure microscopy reduces photobleaching and phototoxicity in fluorescence live-cell imaging.

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Journal:  Nat Biotechnol       Date:  2007-01-21       Impact factor: 54.908

Review 4.  Far-field optical nanoscopy.

Authors:  Stefan W Hell
Journal:  Science       Date:  2007-05-25       Impact factor: 47.728

5.  Quantitative nanoscopy of inhibitory synapses: counting gephyrin molecules and receptor binding sites.

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Journal:  Neuron       Date:  2013-07-24       Impact factor: 17.173

6.  Nanometer resolution imaging and tracking of fluorescent molecules with minimal photon fluxes.

Authors:  Francisco Balzarotti; Yvan Eilers; Klaus C Gwosch; Arvid H Gynnå; Volker Westphal; Fernando D Stefani; Johan Elf; Stefan W Hell
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7.  Nanoscale Molecular Reorganization of the Inhibitory Postsynaptic Density Is a Determinant of GABAergic Synaptic Potentiation.

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8.  DNA origami-based standards for quantitative fluorescence microscopy.

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9.  Breaking the diffraction barrier: super-resolution imaging of cells.

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  25 in total

1.  STED super-resolved microscopy.

Authors:  Giuseppe Vicidomini; Paolo Bianchini; Alberto Diaspro
Journal:  Nat Methods       Date:  2018-01-29       Impact factor: 28.547

Review 2.  Strategies to maximize performance in STimulated Emission Depletion (STED) nanoscopy of biological specimens.

Authors:  Wiebke Jahr; Philipp Velicky; Johann Georg Danzl
Journal:  Methods       Date:  2019-07-22       Impact factor: 3.608

3.  Event-driven acquisition for content-enriched microscopy.

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4.  Coherent-hybrid STED: high contrast sub-diffraction imaging using a bi-vortex depletion beam.

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Journal:  Nat Cell Biol       Date:  2019-01-02       Impact factor: 28.824

Review 6.  From Dynamics to Membrane Organization: Experimental Breakthroughs Occasion a "Modeling Manifesto".

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Review 7.  Advances in fluorescence microscopy techniques to study kidney function.

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Journal:  Nat Rev Nephrol       Date:  2020-09-18       Impact factor: 28.314

Review 8.  Between life and death: strategies to reduce phototoxicity in super-resolution microscopy.

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Journal:  J Phys D Appl Phys       Date:  2020-02-14       Impact factor: 3.207

Review 9.  Technological advances in super-resolution microscopy to study cellular processes.

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Journal:  Mol Cell       Date:  2022-01-20       Impact factor: 17.970

Review 10.  Super-resolution fluorescence microscopy studies of human immunodeficiency virus.

Authors:  Jakub Chojnacki; Christian Eggeling
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