Effects and avoidance of photoconversion-induced artifacts in confocal and STED microscopy.
Anindita DasguptaAgnes KoerferBoštjan KokotIztok UrbancicChristian EggelingPablo CarravillaPublished in: Nature methods (2024)
Fluorescence microscopy is limited by photoconversion due to continuous illumination, which results in not only photobleaching but also conversion of fluorescent molecules into species of different spectral properties through photoblueing. Here, we determined different fluorescence parameters of photoconverted products for various fluorophores under standard confocal and stimulated emission depletion (STED) microscopy conditions. We observed changes in both fluorescence spectra and lifetimes that can cause artifacts in quantitative measurements, which can be avoided by using exchangeable dyes.
Keyphrases
- single molecule
- optical coherence tomography
- living cells
- high resolution
- label free
- energy transfer
- high speed
- high throughput
- quantum dots
- raman spectroscopy
- high glucose
- drug induced
- diabetic rats
- image quality
- magnetic resonance imaging
- computed tomography
- density functional theory
- mass spectrometry
- endothelial cells