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Molecular resolution imaging by post-labeling expansion single-molecule localization microscopy (Ex-SMLM)
by
Reinhard, Sebastian
, Sauer, Markus
, Guichard, Paul
, Gambarotto, Davide
, Hamel, Virginie
, Zwettler, Fabian U.
, Bell, Toby D. M.
in
631/1647/328/2238
/ 631/57/2265
/ 639/624/1111/55
/ Animals
/ Biological properties
/ Biological samples
/ Buffers
/ Centrioles
/ Centrioles - metabolism
/ Chemical compounds
/ Chlamydomonas reinhardtii - metabolism
/ Chlorocebus aethiops
/ Computer Simulation
/ COS Cells
/ Denaturation
/ Electrolytes
/ Electron microscopy
/ Embedding
/ Epitopes
/ Error reduction
/ Fluorescence
/ Fluorescent Dyes - chemistry
/ Fluorophores
/ Gelation
/ Humanities and Social Sciences
/ Hydrogels
/ Hydrogels - chemistry
/ Image resolution
/ Imaging, Three-Dimensional
/ Incompatibility
/ Labeling
/ Localization
/ Microscopes
/ Microscopy
/ Microscopy, Fluorescence - methods
/ Microtubules
/ Microtubules - metabolism
/ multidisciplinary
/ Normal Distribution
/ Photochemistry
/ Polyelectrolytes
/ Proteins
/ Science
/ Science (multidisciplinary)
/ Single Molecule Imaging - methods
2020
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Molecular resolution imaging by post-labeling expansion single-molecule localization microscopy (Ex-SMLM)
by
Reinhard, Sebastian
, Sauer, Markus
, Guichard, Paul
, Gambarotto, Davide
, Hamel, Virginie
, Zwettler, Fabian U.
, Bell, Toby D. M.
in
631/1647/328/2238
/ 631/57/2265
/ 639/624/1111/55
/ Animals
/ Biological properties
/ Biological samples
/ Buffers
/ Centrioles
/ Centrioles - metabolism
/ Chemical compounds
/ Chlamydomonas reinhardtii - metabolism
/ Chlorocebus aethiops
/ Computer Simulation
/ COS Cells
/ Denaturation
/ Electrolytes
/ Electron microscopy
/ Embedding
/ Epitopes
/ Error reduction
/ Fluorescence
/ Fluorescent Dyes - chemistry
/ Fluorophores
/ Gelation
/ Humanities and Social Sciences
/ Hydrogels
/ Hydrogels - chemistry
/ Image resolution
/ Imaging, Three-Dimensional
/ Incompatibility
/ Labeling
/ Localization
/ Microscopes
/ Microscopy
/ Microscopy, Fluorescence - methods
/ Microtubules
/ Microtubules - metabolism
/ multidisciplinary
/ Normal Distribution
/ Photochemistry
/ Polyelectrolytes
/ Proteins
/ Science
/ Science (multidisciplinary)
/ Single Molecule Imaging - methods
2020
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Molecular resolution imaging by post-labeling expansion single-molecule localization microscopy (Ex-SMLM)
by
Reinhard, Sebastian
, Sauer, Markus
, Guichard, Paul
, Gambarotto, Davide
, Hamel, Virginie
, Zwettler, Fabian U.
, Bell, Toby D. M.
in
631/1647/328/2238
/ 631/57/2265
/ 639/624/1111/55
/ Animals
/ Biological properties
/ Biological samples
/ Buffers
/ Centrioles
/ Centrioles - metabolism
/ Chemical compounds
/ Chlamydomonas reinhardtii - metabolism
/ Chlorocebus aethiops
/ Computer Simulation
/ COS Cells
/ Denaturation
/ Electrolytes
/ Electron microscopy
/ Embedding
/ Epitopes
/ Error reduction
/ Fluorescence
/ Fluorescent Dyes - chemistry
/ Fluorophores
/ Gelation
/ Humanities and Social Sciences
/ Hydrogels
/ Hydrogels - chemistry
/ Image resolution
/ Imaging, Three-Dimensional
/ Incompatibility
/ Labeling
/ Localization
/ Microscopes
/ Microscopy
/ Microscopy, Fluorescence - methods
/ Microtubules
/ Microtubules - metabolism
/ multidisciplinary
/ Normal Distribution
/ Photochemistry
/ Polyelectrolytes
/ Proteins
/ Science
/ Science (multidisciplinary)
/ Single Molecule Imaging - methods
2020
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Molecular resolution imaging by post-labeling expansion single-molecule localization microscopy (Ex-SMLM)
Journal Article
Molecular resolution imaging by post-labeling expansion single-molecule localization microscopy (Ex-SMLM)
2020
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Overview
Expansion microscopy (ExM) enables super-resolution fluorescence imaging of physically expanded biological samples with conventional microscopes. By combining ExM with single-molecule localization microscopy (SMLM) it is potentially possible to approach the resolution of electron microscopy. However, current attempts to combine both methods remained challenging because of protein and fluorophore loss during digestion or denaturation, gelation, and the incompatibility of expanded polyelectrolyte hydrogels with photoswitching buffers. Here we show that re-embedding of expanded hydrogels enables
d
STORM imaging of expanded samples and demonstrate that post-labeling ExM resolves the current limitations of super-resolution microscopy. Using microtubules as a reference structure and centrioles, we demonstrate that post-labeling Ex-SMLM preserves ultrastructural details, improves the labeling efficiency and reduces the positional error arising from linking fluorophores into the gel thus paving the way for super-resolution imaging of immunolabeled endogenous proteins with true molecular resolution.
Previous attempts to combine expansion microscopy (ExM) and single molecule localisation microscopy (SMLM) have proved challenging. Here the authors show that post-labelling Ex-SMLM improves labelling efficiency, reduces linkage error, and preserves ultrastructural details.
Publisher
Nature Publishing Group UK,Nature Publishing Group,Nature Portfolio
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