Litcius/Paper detail

Analysis of super-resolution single molecule localization microscopy data: A tutorial

Mohamadreza Fazel, Michael J. Wester

2022AIP Advances27 citationsDOIOpen Access PDF

Abstract

The diffraction of light imposes a fundamental limit on the resolution of light microscopes. This limit can be circumvented by creating and exploiting independent behaviors of the sample at length scales below the diffraction limit. In super-resolution single molecule localization microscopy (SMLM), the independence arises from individual fluorescent labels stochastically switching between dark and fluorescent states, which in turn allows the pinpointing of fluorophores post experimentally using a sequence of acquired sparse image frames. Finally, the resulting list of fluorophore coordinates is utilized to produce high resolution images or to gain quantitative insight into the underlying biological structures. Therefore, image processing and post-processing are essential stages of SMLM. Here, we review the latest progress on SMLM data processing and post-processing.

Topics & Concepts

MicroscopyFluorophoreDiffractionResolution (logic)OpticsImage resolutionImage processingLimit (mathematics)MicroscopeSuper-resolution microscopyLight sheet fluorescence microscopyPhotoactivated localization microscopyComputer sciencePhysicsComputer visionFluorescenceArtificial intelligenceImage (mathematics)Scanning confocal electron microscopyMathematicsMathematical analysisAdvanced Fluorescence Microscopy TechniquesAdvanced Electron Microscopy Techniques and ApplicationsNear-Field Optical Microscopy