Abstract
We present a technique that records transient changes in the fluorescence lifetime of a sample with spatial resolution along a one-dimensional scan. The technique is based on scanning the sample with a high-frequency pulsed laser beam, detecting single photons of the fluorescence light, and building up a photon distribution over the distance along the scan, the arrival times of the photons after the excitation pulses and the time after a stimulation of the sample. The maximum resolution at which lifetime changes can be recorded is given by the line scan period. Transient lifetime effects can thus be resolved at a resolution of about one millisecond. We demonstrate the technique for recording photochemical and nonphotochemical chlorophyll transients in plants and transient changes in free Ca2+ in cultured neurons. Microsc. Res. Tech. 77:216-224, 2014.
| Original language | English |
|---|---|
| Pages (from-to) | 216-224 |
| Number of pages | 9 |
| Journal | Microscopy Research and Technique |
| Volume | 77 |
| Issue number | 3 |
| DOIs | |
| State | Published - Mar 2014 |
Keywords
- Chlorophyll transients
- FLIM
- FLITS
- Fluorescence lifetime
- TCSPC
All Science Journal Classification (ASJC) codes
- Anatomy
- Histology
- Instrumentation
- Medical Laboratory Technology