SPECTROSCOPIC STUDY OF THE INTERACTION OF ALUMINUM IONS WITH HUMAN TRANSFERRIN

被引:32
作者
TANG, S
MACCOLL, R
PARSONS, PJ
机构
[1] NEW YORK STATE DEPT HLTH,WADSWORTH CTR,ALBANY,NY 12201
[2] SUNY ALBANY,SCH PUBL HLTH,DEPT ENVIRONM HLTH & TOXICOL,ALBANY,NY
关键词
D O I
10.1016/0162-0134(95)00018-J
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Transferrin is the plasma protein responsible for transporting Fe3+ from the absorption to the utilization site. Interactions of apo- and holo-transferrin with Al3+ were studied by circular dichroism (CD), UV-visible, and fluorescence spectrometry. Binding of Al3+ to both metal-ion binding sites of apo-transferrin was confirmed by fluorescence studies. No interaction of Al3+ with holo-transferrin was observed, indicating that Al3+ cannot displace Fe3+ under the experimental conditions employed. An increase in tryptophan fluorescence (lambda(max) at 330 nm) by excitation at either 280 or 295 nm was observed after Al3+ interaction with apo-transferrin. There was no shift in wavelength of the fluorescence band of apo-transferrin after interaction with Al3+, but the intensity did increase. Since excitation at 295 nm is specific for tryptophan residues, tryptophan but not tyrosine must be responsible for the change in fluorescence intensity. Decreased fluorescence is the result of Fe3+ binding to apo-transferrin. The CD spectrum of apo-transferrin was slightly affected in the far UV by Al3+ binding, but a salient change was noted in the near UV at similar to 288 nm where tyrosine and tryptophan absorb. It is concluded that a small conformational change in the protein was induced by Al3+ binding to apo-transferrin.
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页码:175 / 185
页数:11
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