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Mössbauer studies of electrophoretically purified monoferric and diferric human transferrin
Authors:Suzanne A Kretchmar  Miguel Teixeira  Boi-Hank Huynh  Kenneth N Raymond
Institution:(1) Department of Chemistry, University of California, 94720 Berkeley, CA, USA;(2) Physics Department, Emory University, 30322 Atlanta, GA, USA;(3) Present address: Centro de Quimica Estrutural, I.S.T., Universidade Nova de Lisboa, P-1000 Lisboa, Portugal
Abstract:Summary Electrophoretically purified57Fe-enriched monoferric and diferric human transferrins and selectively labeled complexes (C-56Fe,N-57Fe]transferrin and C-57Fe,N-56Fe]transferrin) were studied by Mössbauer spectroscopy. The data were recorded at 4.2 K over a wide range of applied magnetic fields (0.05–6 T) and were analyzed by a spin-Hamiltonian formalism. Characteristic hyperfine parameters were found and the obtained zero-field splitting parameters (D=0.25±0.05 cm–1 andE/D = 0.30 ± 0.02) agree with previous electron paramagnetic resonance (EPR) findings. The weak-field spectra of the N-57Fe]transferrin are slightly broader than those of the C-57Fe]transferrin, indicating that the N-terminal iron site may be more heterogeneous. However, the absorption line positions and the relative intensities of the subspectra originating from the three Kramers doublets of each Fe3+ site are identical. Thus the electronic structures of the two iron sites can be described by the same set of spin- Hamiltonian parameters, indicating that the ligand environments for the two sites are the same, as suggested by the recent X-ray crystallographic studies. This suggestion is further supported by the observation that the strong-field spectra of the two monoferric transferrins are indistinguishable. The selectively labeled mixed-isotope transferrins exhibit spectra that are identical to those of the corresponding monoferric57Fe-enriched transferrins, implying that the occupation of one iron site has little or no effect on the immediate envirnoment of the other site, a finding that is not surprising since the two sites are separated by approximately 4.2 nm.
Keywords:  ssbauer spectroscopy  Transferrin  Electron paramagnetic resonance  Ironbinding sites
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