Super-resolution fluorescence imaging with single molecules.

IF: 7.786

Cited by: 117

Abstract

The ability to detect, image and localize single molecules optically with high spatial precision by their fluorescence enables an emergent class of super-resolution microscopy methods which have overcome the longstanding diffraction barrier for far-field light-focusing optics. Achieving spatial resolutions of 20-40nm or better in both fixed and living cells, these methods are currently being established as powerful tools for minimally-invasive spatiotemporal analysis of structural details in cellular processes which benefit from enhanced resolution. Briefly covering the basic principles, this short review then summarizes key recent developments and application examples of two-dimensional and three-dimensional (3D) multi-color techniques and faster time-lapse schemes. The prospects for quantitative imaging - in terms of improved ability to correct for dipole-emission-induced systematic localization errors and to provide accurate counts of molecular copy numbers within nanoscale cellular domains - are discussed.

MeSH terms

Imaging, Three-Dimensional

Microscopy, Fluorescence

Molecular Imaging

Multiprotein Complexes

Organelles

Time-Lapse Imaging

Authors

Sahl, Steffen J

Moerner, W E

Recommend literature

1. Light sheet approaches for improved precision in 3D localization-based super-resolution imaging in mammalian cells [Invited].

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

3. Spectrally Resolved and Functional Super-resolution Microscopy via Ultrahigh-Throughput Single-Molecule Spectroscopy.

4. High-speed super-resolution imaging of rotationally symmetric structures using SPEED microscopy and 2D-to-3D transformation.

5. Systematic, spatial imaging of large multimolecular assemblies and the emerging principles of supramolecular order in biological systems.