Apo- and holo-transferrin differentially interact with hephaestin and ferroportin in a novel mechanism of cellular iron release regulation

Stephanie L Baringer; Kondaiah Palsa; Vladimir S Spiegelman; Ian A Simpson; James R Connor

doi:10.1186/s12929-023-00934-2

Apo- and holo-transferrin differentially interact with hephaestin and ferroportin in a novel mechanism of cellular iron release regulation

J Biomed Sci. 2023 Jun 6;30(1):36. doi: 10.1186/s12929-023-00934-2.

Authors

Stephanie L Baringer¹, Kondaiah Palsa¹, Vladimir S Spiegelman², Ian A Simpson³, James R Connor⁴

Affiliations

¹ Department of Neurosurgery, Penn State College of Medicine, 500 University Drive, Hershey, PA, 17033, USA.
² Department of Pediatrics, Penn State College of Medicine, Hershey, PA, USA.
³ Department of Neural and Behavioral Sciences, Penn State College of Medicine, Hershey, PA, USA.
⁴ Department of Neurosurgery, Penn State College of Medicine, 500 University Drive, Hershey, PA, 17033, USA. jconnor@pennstatehealth.psu.edu.

Abstract

Background: Apo- (iron free) and holo- (iron bound) transferrin (Tf) participate in precise regulation of brain iron uptake at endothelial cells of the blood-brain barrier. Apo-Tf indicates an iron-deficient environment and stimulates iron release, while holo-Tf indicates an iron sufficient environment and suppresses additional iron release. Free iron is exported through ferroportin, with hephaestin as an aid to the process. Until now, the molecular mechanisms of apo- and holo-Tf influence on iron release was largely unknown.

Methods: Here we use a variety of cell culture techniques, including co-immunoprecipitation and proximity ligation assay, in iPSC-derived endothelial cells and HEK 293 cells to investigate the mechanism by which apo- and holo-Tf influence cellular iron release. Given the established role of hepcidin in regulating cellular iron release, we further explored the relationship of hepcidin to transferrin in this model.

Results: We demonstrate that holo-Tf induces the internalization of ferroportin through the established ferroportin degradation pathway. Furthermore, holo-Tf directly interacts with ferroportin, whereas apo-Tf directly interacts with hephaestin. Only pathophysiological levels of hepcidin disrupt the interaction between holo-Tf and ferroportin, but similar hepcidin levels are unable to interfere with the interaction between apo-Tf and hephaestin. The disruption of the holo-Tf and ferroportin interaction by hepcidin is due to hepcidin's ability to more rapidly internalize ferroportin compared to holo-Tf.

Conclusions: These novel findings provide a molecular mechanism for apo- and holo-Tf regulation of iron release from endothelial cells. They further demonstrate how hepcidin impacts these protein-protein interactions, and offer a model for how holo-Tf and hepcidin cooperate to suppress iron release. These results expand on our previous reports on mechanisms mediating regulation of brain iron uptake to provide a more thorough understanding of the regulatory mechanisms mediating cellular iron release in general.

Keywords: Blood–brain barrier; Ferroportin; Hepcidin; Hephaestin; Iron; Transferrin.

MeSH terms

Endothelial Cells / metabolism
HEK293 Cells
Hepcidins* / metabolism
Humans
Transferrin* / metabolism

Substances

Transferrin
Hepcidins
metal transporting protein 1

Abstract

MeSH terms

Substances

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