Tracking protein dynamics with photoconvertible Dendra2 on spinning disk confocal systems

Elena Woods, Jane Courtney, Dimitri Scholz, William W. Hall, Virginie W. Gautier

    Research output: Contribution to journalArticlepeer-review

    Abstract

    Understanding the dynamic properties of cellular proteins in live cells and in real time is essential to delineate their function. In this context, we introduce the Fluorescence Recovery After Photobleaching-Photoactivation unit (Andor) combined with the Nikon Eclipse Ti E Spinning Disk (Andor) confocal microscope as an advantageous and robust platform to exploit the properties of the Dendra2 photoconvertible fluorescent protein (Evrogen) and analyse protein subcellular trafficking in living cells. A major advantage of the spinning disk confocal is the rapid acquisition speed, enabling high temporal resolution of cellular processes. Furthermore, photoconversion and imaging are less invasive on the spinning disk confocal as the cell exposition to illumination power is reduced, thereby minimizing photobleaching and increasing cell viability. We have tested this commercially available platform using experimental settings adapted to track the migration of fast trafficking proteins such as UBC9, Fibrillarin and have successfully characterized their differential motion between subnuclear structures. We describe here step-by-step procedures, with emphasis on cellular imaging parameters, to successfully perform the dynamic imaging and photoconversion of Dendra2-fused proteins at high spatial and temporal resolutions necessary to characterize the trafficking pathways of proteins.

    Original languageEnglish
    Pages (from-to)197-207
    Number of pages11
    JournalJournal of Microscopy
    Volume256
    Issue number3
    DOIs
    Publication statusPublished - 1 Dec 2014

    Keywords

    • Dendra2
    • Live cell imaging
    • Photoconversion
    • Spinning disk confocal microscopy

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