Energy transfer as a probe of protein dynamics in the proteins transferrin and calmodulin.

P B O'Hara, K M Gorski and M A Rosen

Department of Chemistry, Amherst College, Massachusetts 01002.

ABSTRACT

We have initiated an investigation into the usefulness of fluorescenceenergy transfer in probing protein dynamics. Our analysis involvesmeasuring the energy transfer efficiency while perturbing theprotein conformational equilibrium with heat. As the temperatureincreases, the amplitudes of vibrations increase, and fluorescenceenergy transfer should also increase if the donor and acceptorare in a flexible region of the protein. A theoretical analysisdeveloped by Somogyi and co-workers for the temperature dependenceof dipole-dipole energy transfer (Somogyi, B., J. Matko, S.Papp, J. Hevessey, G. R. Welch, and S. Damjanovich. 1984. Biochemistry.23:3403-3411) was tested by the authors in one protein system.Energy transfer from tryptophan to a pyridoxamine derivatizedside group in RNase increased 40% over 25 degrees C. Here wereport further testing of this model in two additional proteinsystems: calmodulin, a calcium activated regulatory protein,and transferrin, a blood serum iron shuttle. Our studies showa slight differential sensitivity of the transfer efficiencyto heat for the two systems. Normalized energy transfer over6.5 A in calmodulin from a tyrosine donor to a Tb(III) acceptorincreases 40% from 295 to 320 K. Normalized energy transferover 42 A in transferrin from a Tb(III) donor to an Fe(III)acceptor increases 35% over the same temperature range. Whereasthese results demonstrate that thermally induced fluctuationsdo increase energy transfer as predicted by Somogyi, they alsoappear rather insensitive to the nature of the protein hostenvironment. In contrast to the Förster processes examinedabove, energy transfer over very short distances has shown ananomalously high temperature dependence.

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