a synthetic peptide with the putative iron binding motif of amyloid precursor protein (app) does not catalytically oxidize iron合成肽与假定的铁结合淀粉样前体蛋白(app)的主题并不催化地氧化铁.pdfVIP
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a synthetic peptide with the putative iron binding motif of amyloid precursor protein (app) does not catalytically oxidize iron合成肽与假定的铁结合淀粉样前体蛋白(app)的主题并不催化地氧化铁
A Synthetic Peptide with the Putative Iron Binding Motif
of Amyloid Precursor Protein (APP) Does Not
Catalytically Oxidize Iron
Kourosh Honarmand Ebrahimi, Peter-Leon Hagedoorn, Wilfred R. Hagen*
Department of Biotechnology, Delft University of Technology, Delft, The Netherlands
Abstract
The b-amyloid precursor protein (APP), which is a key player in Alzheimer’s disease, was recently reported to possess an
Fe(II) binding site within its E2 domain which exhibits ferroxidase activity [Duce et al. 2010, Cell 142: 857]. The putative
ligands of this site were compared to those in the ferroxidase site of ferritin. The activity was indirectly measured using
transferrin, which scavenges the Fe(III) product of the reaction. A 22-residue synthetic peptide, named FD1, with the
putative ferroxidase site of APP, and the E2 domain of APP were each reported to exhibit 40% of the ferroxidase activity of
APP and of ceruloplasmin. It was also claimed that the ferroxidase activity of APP is inhibited by Zn(II) just as in ferritin. We
measured the ferroxidase activity indirectly (i) by the incorporation of the Fe(III) product of the ferroxidase reaction into
transferrin and directly (ii) by monitoring consumption of the substrate molecular oxygen. The results with the FD1 peptide
were compared to the established ferroxidase activities of human H-chain ferritin and of ceruloplasmin. For FD1 we
observed no activity above the background of non-enzymatic Fe(II) oxidation by molecular oxygen. Zn(II) binds to
transferrin and diminishes its Fe(III) incorporation capacity and rate but it does not specifically bind to a putative ferroxidase
site of FD1. Based on these results, and on comparison of the putative ligands of the ferroxidase site of APP with those of
ferritin, we conclude that the previously reported results for ferr
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