Litcius/Paper detail

Transient Fluorescence Labeling: Low Affinity—High Benefits

Maxim M. Perfilov, Alexey S. Gavrikov, Konstantin A. Lukyanov, Alexander S. Mishin

2021International Journal of Molecular Sciences15 citationsDOIOpen Access PDF

Abstract

Fluorescent labeling is an established method for visualizing cellular structures and dynamics. The fundamental diffraction limit in image resolution was recently bypassed with the development of super-resolution microscopy. Notably, both localization microscopy and stimulated emission depletion (STED) microscopy impose tight restrictions on the physico-chemical properties of labels. One of them-the requirement for high photostability-can be satisfied by transiently interacting labels: a constant supply of transient labels from a medium replenishes the loss in the signal caused by photobleaching. Moreover, exchangeable tags are less likely to hinder the intrinsic dynamics and cellular functions of labeled molecules. Low-affinity labels may be used both for fixed and living cells in a range of nanoscopy modalities. Nevertheless, the design of optimal labeling and imaging protocols with these novel tags remains tricky. In this review, we highlight the pros and cons of a wide variety of transiently interacting labels. We further discuss the state of the art and future perspectives of low-affinity labeling methods.

Topics & Concepts

STED microscopyPhotobleachingFluorescence recovery after photobleachingMicroscopyFluorescenceFluorescence microscopeFluorescent labellingSuperresolutionBiophysicsTransient (computer programming)Live cell imagingNanotechnologyBiological systemComputer scienceChemistryPhysicsMaterials scienceOpticsBiologyImage (mathematics)Artificial intelligenceBiochemistryCellOperating systemAdvanced Fluorescence Microscopy TechniquesAdvanced Biosensing Techniques and ApplicationsCell Image Analysis Techniques