Berlin 2018 – wissenschaftliches Programm

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BP: Fachverband Biologische Physik

BP 23: Bioimaging and Biopspectroscopy II

BP 23.4: Vortrag

Mittwoch, 14. März 2018, 15:45–16:00, H 2013

Characterisation of Metabolic Dynamics by Fluorescence Lifetime Imaging Microscopy of NAD(P)H — •André Weber¹, Yury Prokazov¹, Marcus Hauser², and Werner Zuschratter¹ — ¹Leibniz-Institut für Neurobiologie Magdeburg, Germany — ²Institut für Biometrie und Medizinische Informatik, Otto-von-Guericke- Universität Magdeburg, Germany

The energy metabolism of eucaryotic cells can show complex dynamics, i.e. glycolytic oscillations. Monitoring this intrinsic behaviour by fluorescence microscopy is influence the metabolism, which is sensitive to excitation light intensities, especially in UV range.

We show a low light imaging approach using a single photon counting position sensitive detector working with laser intensities below 3mW/cm² and a time resolution below 90ps. For excitation of intracellular NAD(P)H a 8 MHz pulsed frequency-tripled Nd:vanadate laser tuned at 355 nm was used. The analysis of the complex fluorescence decay of NAD(P)H in intact yeast cells revealed 4 molecular species with characteristic fluorescence lifetimes showing individual behaviour and glycolytic oscillations as response to glucose addition. Laser intensities higher 3mW/cm² did not lead to long lasting glycolytic oscillations.