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Biophysical Journal 86:3981-3992 (2004)
© 2004 The Biophysical Society

Cumulant Analysis in Fluorescence Fluctuation Spectroscopy

Joachim D. Müller

School of Physics and Astronomy, University of Minnesota, Minneapolis, Minnesota

Correspondence: Address reprint requests to Joachim D. Müller, University of Minnesota, School of Physics and Astronomy, 116 Church Street SE, Minneapolis, MN 55455. Tel.: 612-625-4369; Fax: 612:624-4578; E-mail: mueller{at}physics.umn.edu.

A novel technique for the analysis of fluorescence fluctuation experiments is introduced. Fluorescence cumulant analysis (FCA) exploits the factorial cumulants of the photon counts and resolves heterogeneous samples based on differences in brightness. A simple analytical model connects the cumulants of the photon counts with the brightness {varepsilon} and the number of molecules N in the optical observation volume for each fluorescent species. To provide the tools for a rigorous error analysis of FCA, expressions for the variance of factorial cumulants are developed and tested. We compare theory with experiment by analyzing dye mixtures and simple fluorophore solutions with FCA. A comparison of FCA with photon-counting histogram (PCH) analysis, a related technique, shows that both methods give identical results within experimental uncertainty. Both FCA and PCH are restricted to data sampling times that are short compared to the diffusion time of molecules through the observation volume of the instrument. But FCA theory, in contrast to PCH, can be extended to treat arbitrary sampling times. Here, we derive analytical expressions for the second factorial cumulant as a function of the sampling time and demonstrate that the theory successfully models fluorescence fluctuation data.




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