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Measuring the Number of Independent Emitters in Single-Molecule Fluorescence Images and Trajectories Using Coincident Photons

A simple new approach is described and demonstrated for measuring the number of independent emitters along with the fluorescence intensity, lifetime, and emission wavelength for trajectories and images of single molecules and multichromophoric systems using a single PC plug-in card for time-correlat...

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Bibliographic Details
Published in:Analytical chemistry (Washington) 2002-10, Vol.74 (20), p.5342-5349
Main Authors: Weston, Kenneth D, Dyck, Martina, Tinnefeld, Philip, Müller, Christian, Herten, Dirk P, Sauer, Markus
Format: Article
Language:English
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Summary:A simple new approach is described and demonstrated for measuring the number of independent emitters along with the fluorescence intensity, lifetime, and emission wavelength for trajectories and images of single molecules and multichromophoric systems using a single PC plug-in card for time-correlated single-photon counting. The number of independent emitters present in the detection volume can be determined using the interphoton times in a manner similar to classical antibunching experiments. In contrast to traditional coincidence analysis based on pulsed laser excitation and direct measurement of coincident photon pairs using a time-to-amplitude converter, the interphoton distances are retrieved afterward by recording the absolute arrival time of each photon with nanosecond time resolution on two spectrally separated detectors. Intensity changes that result from fluctuations of a photophysical parameter can be distinguished from fluctuations due to changes in the number of emitters (e.g., photobleaching) in single chromophore and multichromophore intensity trajectories. This is the first report to demonstrate imaging with contrast based on the number of independently emitting species within the detection volume.
ISSN:0003-2700
1520-6882
DOI:10.1021/ac025730z