Your search keyword '"Sweetland, Emma"' showing total 5 results

1. In vitro binding of HFE to the cation-independent mannose-6 phosphate receptor.

Author

Schimanski LM, Drakesmith H, Sweetland E, Bastin J, Rezgui D, Edelmann M, Kessler B, Merryweather-Clarke AT, Robson KJ, and Townsend AR

Subjects

Animals, Cell Line, Cell Line, Tumor, Hemochromatosis Protein, Humans, Ligands, Mice, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Antigens, CD metabolism, Histocompatibility Antigens Class I metabolism, Mannosephosphates metabolism, Membrane Proteins metabolism, Receptor, IGF Type 2 metabolism, Receptors, Transferrin metabolism, Transferrin metabolism

Abstract

Hereditary hemochromatosis is most frequently associated with mutations in HFE, which encodes a class Ib histocompatibility protein. HFE binds to the transferrin receptor-1 (TfR1) in competition with iron-loaded transferrin (Fe-Tf). HFE is released from TfR1 by increasing concentrations of Fe-Tf, and free HFE may then regulate iron homeostasis by binding other ligands. To search for new HFE ligands we expressed recombinant forms of HFE in the human cell line 293T. HFE protein was purified, biotinylated and made into fluorescently labelled tetramers. HFE tetramers bound to TfR1 in competition with Tf, but in addition we detected a binding activity on some cell types that was not blocked by Fe-Tf or by mutations in HFE that prevent binding to TfR1. We identified this second HFE ligand as the cation independent mannose-6-phosphate receptor (CI-MPR, also known as the insulin-like growth factor-2 receptor, IGF2R). HFE:CI-MPR binding was mediated through phosphorylated mannose residues on HFE. Recombinant murine Hfe also bound to CI-MPR. HFE bound to TfR1 was prevented from binding CI-MPR until released by increasing concentrations of Fe-Tf, a feature consistent with an iron sensing mechanism. However, it remains to be determined whether endogenous HFE in vivo also acquires the mannose-6 phosphate modification and binds to CI-MPR.

Published

2009

2. Ferroportin: lack of evidence for multimers.

Author

Schimanski LM, Drakesmith H, Talbott C, Horne K, James JR, Davis SJ, Sweetland E, Bastin J, Cowley D, and Townsend AR

Subjects

Cation Transport Proteins chemistry, Cation Transport Proteins genetics, Cell Line, Cell Membrane metabolism, Epithelial Cells cytology, Hemochromatosis genetics, Humans, Mutant Proteins chemistry, Mutant Proteins metabolism, Mutation, Cation Transport Proteins metabolism, Epithelial Cells metabolism, Ferritins metabolism, Hemochromatosis metabolism

Abstract

Ferroportin is a multi-transmembrane glycoprotein that mediates iron export from cells. Mutations in ferroportin are linked to type IV hemochromatosis, a dominantly inherited disorder of iron metabolism. Multimers of ferroportin, whose existence may relate to the dominant inheritance pattern of disease, have been detected in some studies but not others. We looked for evidence of multimerization in several different types of experiment. We assayed the maturation of mutant and wild-type ferroportin and found that loss-of-function mutants had a reduced half-life but did not alter the stability of coexpressed wild-type. Using bioluminescence resonance energy transfer analysis, we tested how mature wild-type ferroportin behaved in intact live cell membranes. Ferroportin-ferroportin interactions gave the very low acceptor/donor ratio-independent energy transfer levels characteristic of random protein-protein interactions, consistent with ferroportin behaving as a monomer. Consistent with these experiments, we were unable to detect a dominant negative functional effect of mutant ferroportin on wild-type, even when expression of wild-type protein was titrated to low levels. These data suggest that dominantly inherited ferroportin disease does not result from the direct action of a mutated protein inhibiting a wild-type protein within multimers. We propose other possible mechanisms of disease.

Published

2008

3. Resistance to hepcidin is conferred by hemochromatosis-associated mutations of ferroportin.

Author

Drakesmith H, Schimanski LM, Ormerod E, Merryweather-Clarke AT, Viprakasit V, Edwards JP, Sweetland E, Bastin JM, Cowley D, Chinthammitr Y, Robson KJ, and Townsend AR

Subjects

Cation Transport Proteins antagonists & inhibitors, Cell Line, Gene Expression Regulation drug effects, Hemochromatosis drug therapy, Hemochromatosis etiology, Hepcidins, Humans, Iron metabolism, Iron Radioisotopes metabolism, Transferrin metabolism, Antimicrobial Cationic Peptides pharmacology, Cation Transport Proteins genetics, Drug Resistance genetics, Hemochromatosis genetics, Mutation, Missense

Abstract

Ferroportin (FPN) mediates iron export from cells; FPN mutations are associated with the iron overloading disorder hemochromatosis. Previously, we found that the A77D, V162del, and G490D mutations inhibited FPN activity, but that other disease-associated FPN variants retained full iron export capability. The peptide hormone hepcidin inhibits FPN as part of a homeostatic negative feedback loop. We measured surface expression and function of wild-type FPN and fully active FPN mutants in the presence of hepcidin. We found that the Y64N and C326Y mutants of FPN are completely resistant to hepcidin inhibition and that N144D and N144H are partially resistant. Hemochromatosis-associated FPN mutations, therefore, either reduce iron export ability or produce an FPN variant that is insensitive to hepcidin. The former mutation type is associated with Kupffer-cell iron deposition and normal transferrin saturation in vivo, whereas patients with the latter category of FPN mutation have high transferrin saturation and tend to deposit iron throughout the liver parenchyma. FPN-linked hemochromatosis may have a variable pathogenesis depending on the causative FPN mutant.

Published

2005

4. In vitro functional analysis of human ferroportin (FPN) and hemochromatosis-associated FPN mutations.

Author

Schimanski LM, Drakesmith H, Merryweather-Clarke AT, Viprakasit V, Edwards JP, Sweetland E, Bastin JM, Cowley D, Chinthammitr Y, Robson KJ, and Townsend AR

Subjects

Antigens, CD, Cell Line, Ferritins metabolism, Humans, Intracellular Space metabolism, Iron metabolism, Iron Deficiencies, Phenotype, Protein Binding, Receptors, Transferrin metabolism, Cation Transport Proteins genetics, Cation Transport Proteins metabolism, Hemochromatosis genetics, Mutation genetics

Abstract

Type IV hemochromatosis is associated with dominant mutations in the SLC40A1 gene encoding ferroportin (FPN). Known as the "ferroportin disease," this condition is typically characterized by high serum ferritin, reduced transferrin saturation, and macrophage iron loading. Previously FPN expression in vitro has been shown to cause iron deficiency in human cell lines and mediate iron export from Xenopus oocytes. We confirm these findings by showing that expression of human FPN in a human cell line results in an iron deficiency because of a 3-fold increased export of iron. We show that FPN mutations A77D, V162delta, and G490D that are associated with a typical pattern of disease in vivo cause a loss of iron export function in vitro but do not physically or functionally impede wild-type FPN. These mutants may, therefore, lead to disease by haploinsufficiency. By contrast the variants Y64N, N144D, N144H, Q248H, and C326Y, which can be associated with greater transferrin saturation and more prominent iron deposition in liver parenchyma in vivo, retained iron export function in vitro. Because FPN is a target for negative feedback in iron homeostasis, we postulate that the latter group of mutants may resist inhibition, resulting in a permanently "turned on" iron exporter.

Published

2005

5. The hemochromatosis protein HFE inhibits iron export from macrophages.

Author

Drakesmith H, Sweetland E, Schimanski L, Edwards J, Cowley D, Ashraf M, Bastin J, and Townsend AR

Subjects

Amino Acid Substitution, Binding, Competitive, Biological Transport drug effects, Ferritins metabolism, HeLa Cells, Hemochromatosis genetics, Hemochromatosis pathology, Hemochromatosis Protein, Histocompatibility Antigens Class I genetics, Histocompatibility Antigens Class I pharmacology, Humans, Macrophages metabolism, Membrane Proteins genetics, Membrane Proteins pharmacology, Models, Molecular, Monocytes drug effects, Monocytes metabolism, Mutation, Protein Conformation, Recombinant Fusion Proteins pharmacology, Transferrin metabolism, Transferrin pharmacology, Tumor Cells, Cultured drug effects, Tumor Cells, Cultured metabolism, U937 Cells drug effects, U937 Cells metabolism, Hemochromatosis metabolism, Histocompatibility Antigens Class I physiology, Iron metabolism, Macrophages drug effects, Membrane Proteins physiology

Abstract

Hereditary hemochromatosis (HH) is a disorder of iron metabolism caused by common mutations in the gene HFE. The HFE protein binds to transferrin receptor-1 (TfR1) in competition with transferrin, and in vitro, reduces cellular iron by reducing iron uptake. However, in vivo, HFE is strongly expressed by liver macrophages and intestinal crypt cells, which behave as though they are relatively iron-deficient in HH. These latter observations suggest, paradoxically, that expression of wild-type HFE may lead to iron accumulation in these specialized cell types. Here we show that wild-type HFE protein raises cellular iron by inhibiting iron efflux from the monocytemacrophage cell line THP-1, and extend these results to macrophages derived from healthy individuals and HH patients. In addition, we find that the HH-associated mutant H41D has lost the ability to inhibit iron release despite binding to TfR1 as well as wild-type HFE. Finally, we show that the ability of HFE to block iron release is not competitively inhibited by transferrin. We conclude that HFE has two mutually exclusive functions, binding to TfR1 in competition with Tf, or inhibition of iron release.

Published

2002