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Spatiotemporal Imaging with Light-Sheet Microscopy: Having Your Cake and Eating It Too

RECORD | Already taken place Tu, 8.7.2025
Discover how FCS can be used in light-sheet microscopes—without customization—to analyze molecular behavior in biofilms, drosophila, and zebrafish at high speed and sensitivity.
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Bruker: Spatiotemporal Imaging with Light-Sheet Microscopy: Having Your Cake and Eating It Too
Bruker: Spatiotemporal Imaging with Light-Sheet Microscopy: Having Your Cake and Eating It Too

Light-sheet microscopes record whole cross‑sections of large, live biological samples in a single step. This modality is also ideal for recording molecular dynamics in each cross‑section of the same samples if the recording is performed fast enough (~1000 frames/s).

In this webinar, our guest speaker will focus on how one of these single-molecule sensitive techniques, Fluorescence Correlation Spectroscopy (FCS), can be implemented in home‑built or commercial light sheet microscopes (imaging FCS) without customization. FCS determines molecular concentrations, mobilities, transport, and interactions. Join this event to see several examples of measurements in biofilms, drosophila, and zebrafish.

Presenter: Dr. Thorsten Wohland (Professor, Departments of Biological Sciences and Chemistry, Centre for Bioimaging Sciences and Institute for Digital Molecular Analytics and Science, National University of Singapore)

Thorsten Wohland studied Physics at the Technical University of Darmstadt and the University of Heidelberg in Germany from 1989-1995. He completed his diploma thesis in physics at the European Molecular Biology Laboratory (EMBL) in Heidelberg, Germany, working on optical tweezers. From 1997-2000 he conducted his doctoral thesis at the Swiss Federal Institute of Technology in Lausanne (ETHL/EPFL), Switzerland, on fluorescence correlation spectroscopy. After two years as a postdoctoral fellow in Stanford he joined the National University of Singapore (NUS) where he is now Professor in the Departments of Biological Sciences and Chemistry, working on the integration of fluorescence microscopy and spectroscopy to yield quantitative microscopy methods that can extract information with high spatial and temporal resolution and the application of these methods to biological problems.

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