Measuring protein stability in living zebrafish embryos using fluorescence 
decay after photoconversion (FDAP)

Rogers, KW; Blässle, AJ; Schier, AF; Müller, P

doi:10.3791/52266

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Measuring protein stability in living zebrafish embryos using fluorescence decay after photoconversion (FDAP)

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Blässle, AJ
Müller Group, Friedrich Miescher Laboratory, Max Planck Society;

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Müller, P
Müller Group, Friedrich Miescher Laboratory, Max Planck Society;

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Citation

Rogers, K., Blässle, A., Schier, A., & Müller, P. (2015). Measuring protein stability in living zebrafish embryos using fluorescence decay after photoconversion (FDAP). Journal of Visualized Experiments, 2015(95): 52266. doi:10.3791/52266.

Cite as: https://hdl.handle.net/21.11116/0000-000B-972E-8

Abstract

Protein stability influences many aspects of biology, and measuring the clearance kinetics of proteins can provide important insights into biological systems. In FDAP experiments, the clearance of proteins within living organisms can be measured. A protein of interest is tagged with a photoconvertible fluorescent protein, expressed in vivo and photoconverted, and the decrease in the photoconverted signal over time is monitored. The data is then fitted with an appropriate clearance model to determine the protein half-life. Importantly, the clearance kinetics of protein populations in different compartments of the organism can be examined separately by applying compartmental masks. This approach has been used to determine the intra- and extracellular half-lives of secreted signaling proteins during zebrafish development. Here, we describe a protocol for FDAP experiments in zebrafish embryos. It should be possible to use FDAP to determine the clearance kinetics of any taggable protein in any optically accessible organism.