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© 2021 American Chemical Society.The dynamics of peptide–protein binding and unbinding of a variant of the RNase S system has been investigated. To initiate the process, a photoswitchable azobenzene moiety has been covalently linked to the S–peptide, thereby switching its binding affinity to the S–protein. Transient fluorescence quenching was measured with the help of a time–resolved fluorometer, which has been specifically designed for these experiments and is based on inexpensive light–emitting diodes and laser diodes only. One mutant shows on–off behavior with no specific binding detectable in one of the states of the photoswitch. Unbinding is faster by at least 2 orders of magnitude, compared to that of other variants of the RNase S system. We conclude that unbinding is essentially barrier–less in that case, revealing the intrinsic dynamics of the unbinding event, which occurs on a time scale of a few hundred microseconds in a strongly stretched–exponential manner.
