Similar to streptavidin, the binding of biotin by avidin does not appear to be cooperative in the traditional sense of altered binding strength, though it appears to be cooperative in terms of ligand induced structural communication across subunits in the protein as previously shown for streptavidin. In this work we provide data from intrinsic tryptophan fluorescence as evidence of a cooperative structural change. The technique involves examination of the changes in fluorescence emission corresponding to the various tryptophan populations accompanying avidin-biotin binding. We note that the 335Â nm emission population (i.e. more hydrophobic local environment) saturates prior to full ligation and the saturation of the 350Â nm emission population commonly used in standard binding activity assays. We also note that total integrated fluorescence emission and peak height during the titration of ligand into streptavidin also reach saturation prior to the 4:1 stoichiometric end point. Unique to avidin and distinct from the behavior of streptavidin described in our prior work, the wavelength of maximum emission and full width at half maximum (FWHM) data do not saturate prior to the 4:1 stoichiometric end point. Avidin also exhibited larger FWHM for both apo and holo forms suggesting greater heterogeneity in local tryptophan environments, as compared to streptavidin. Taken together, the data suggests that the binding of the first 3 biotins effect greater structural changes in the protein than the final ligand in a similar way for avidin and streptavidin.
Avidin cooperative allosterism upon binding biotin observed by differential changes in intrinsic fluorescence.
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作者:Waner Mark J, Ellis Gianna, Graeca Meghan, Ieraci Nicholas, Morell Cole, Murphy Alycia, Mascotti David P
| 期刊: | Biochemistry and Biophysics Reports | 影响因子: | 2.200 |
| 时间: | 2023 | 起止号: | 2023 Oct 11; 36:101554 |
| doi: | 10.1016/j.bbrep.2023.101554 | ||
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