Publikation: A Luminal Loop of Wilson Disease Protein Binds Copper and Is Required for Protein Activity
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The copper-transporting ATPase ATP7B is essential for loading of copper ions to copper-dependent enzymes in the secretory pathway; its inactivation results in Wilson disease. In contrast to copper-ion uptake by the cytoplasmic domains, ATP7B-mediated copper-ion release in the Golgi has not been explored yet. We demonstrate here that a luminal loop in ATP7B, rich in histidine/methionine residues, binds reduced copper (Cu(I)) ions, and identified copper-binding residues play an essential role in ATP7B-mediated metal ion release. NMR experiments on short-peptide models demonstrate that three methionine and two histidine residues are specifically involved in Cu(I) ion binding; with these residues replaced by alanines, no Cu(I) ion interaction is detected. Although more than one Cu(I) ion can interact with the wild-type peptide, removing either all histidine or all methionine residues reduces the stoichiometry to one Cu(I) ion binding per peptide. Using a yeast complementation assay, we show that for efficient copper transport by full-length ATP7B, the complete set of histidine and methionine residues in the lumen loop are required. The replacement of histidine/methionine residues by alanines does not perturb overall ATP7B structure, as the localization of ATP7B variants in yeast cells matches that of the wild-type protein. Thus, in similarity to ATP7A, ATP7B also appears to have a luminal "exit" copper ion site.
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KÖHN, Birgit, Kumaravel PONNANDAI SHANMUGAVEL, Min WU, Michael KOVERMANN, Pernilla WITTUNG-STAFSHEDE, 2018. A Luminal Loop of Wilson Disease Protein Binds Copper and Is Required for Protein Activity. In: Biophysical journal. 2018, 115(6), pp. 1007-1018. ISSN 0006-3495. eISSN 1542-0086. Available under: doi: 10.1016/j.bpj.2018.07.040BibTex
@article{Kohn2018-09-18Lumin-44419,
year={2018},
doi={10.1016/j.bpj.2018.07.040},
title={A Luminal Loop of Wilson Disease Protein Binds Copper and Is Required for Protein Activity},
number={6},
volume={115},
issn={0006-3495},
journal={Biophysical journal},
pages={1007--1018},
author={Köhn, Birgit and Ponnandai Shanmugavel, Kumaravel and Wu, Min and Kovermann, Michael and Wittung-Stafshede, Pernilla}
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<dcterms:abstract xml:lang="eng">The copper-transporting ATPase ATP7B is essential for loading of copper ions to copper-dependent enzymes in the secretory pathway; its inactivation results in Wilson disease. In contrast to copper-ion uptake by the cytoplasmic domains, ATP7B-mediated copper-ion release in the Golgi has not been explored yet. We demonstrate here that a luminal loop in ATP7B, rich in histidine/methionine residues, binds reduced copper (Cu(I)) ions, and identified copper-binding residues play an essential role in ATP7B-mediated metal ion release. NMR experiments on short-peptide models demonstrate that three methionine and two histidine residues are specifically involved in Cu(I) ion binding; with these residues replaced by alanines, no Cu(I) ion interaction is detected. Although more than one Cu(I) ion can interact with the wild-type peptide, removing either all histidine or all methionine residues reduces the stoichiometry to one Cu(I) ion binding per peptide. Using a yeast complementation assay, we show that for efficient copper transport by full-length ATP7B, the complete set of histidine and methionine residues in the lumen loop are required. The replacement of histidine/methionine residues by alanines does not perturb overall ATP7B structure, as the localization of ATP7B variants in yeast cells matches that of the wild-type protein. Thus, in similarity to ATP7A, ATP7B also appears to have a luminal "exit" copper ion site.</dcterms:abstract>
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