Phenotypic and functional data confirm causality of the recently identified hemojuvelin p.r176c missense mutation

doi:10.3324/haematol.11247

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Disorders of Iron Metabolism

Phenotypic and functional data confirm causality of the recently identified hemojuvelin p.r176c missense mutation

Chandran Ka, Gérald Le Gac, Emilie Letocart, Isabelle Gourlaouen, Brigitte Martin, Claude Férec

Inserm, U613, Brest; Universitè de Bretagne Occidentale, Brest; Etablissement Français du Sang, Brest (CK, GLG, EL, IG, CF); Etablissement Français du Sang, Niort (BM); CHU Brest, Service de Génétique Moléculaire, Brest, France (CF)

Correspondence: Gerald Le Gac, Inserm U613, EFS, Bretagne, 46, rue Félix Le Dantec, 29200 Brest, France. Phone: international +33.02.98445064. Fax: international +33.02.98430555. E-mail: gerald.legac{at}univ-brest.fr

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In the present study, we correlate homozygosity for the veryrecently identified HJV p.R176C substitution with a juvenilehemochromatosis phenotype. We also show that the p.R176C variantfails to up-regulate the hepcidin promoter activity. Altogether,our results definitively show the R176C amino-acid change tobe a novel hemojuvelin loss-of-function mutation.

Key words: juvenile haemochromatosis, HJV, hemojuveline dysfunction, hepcidin synthesis.

Juvenile hemochromatosis (JH) differs from typical HFE-relatedhemochromatosis in that it affects both sexes equally, is linkedto a faster iron deposition in parenchymal cells, causes clinicalsymptoms in the second and third decades of life, and, althoughliver dysfunction is also part of the syndrome, is associatedwith a more frequent presentation of hypogonadism and cardiomyopathy.In the absence of treatment, JH patients may succumb to heartfailure before the age of 30.¹ JH is genetically heterogeneoussince it can be associated with mutations in the HJV gene, whichencodes hemojuvelin (OMIM 608374), and in the HAMP gene, whichencodes hepcidin (OMIM 606464).² Very recently, Aguilar-Martinezand co-workers have reported the combination of the known p.G320Vpathogenic mutation together with a newly identified p.R176Csubstitution in the HJV gene of a 5-year-old girl of Europeandescent. The girl displayed elevated iron indices without presentingclinical manifestations of juvenile hemochromatosis.³ We simultaneouslydetected the p.R176C substitution at the homozygous state ina 17-year-old female of French Caucasian ancestry. At diagnosis,the teenager presented with a transferrin saturation of 97%and a serum ferritin concentration above 2,000 µg/L. Clinicalmanifestations included astheny, arthralgy, hypogonadotrophichypogonadism and hepatomegaly. A liver biopsy specimen confirmeddiagnosis of hemochromatosis and showed micronoduleous cirrhosis.It should be stressed that, consistent with their respectivegenetic states (i.e. heterozygous or negative for the p.R176Csubstitution), relatives had normal iron indices (Figure 1).On the other hand, the p.R176C amino-acid change was not detectedin 256 healthy blood donors from the same geographical area.Written informed consent was obtained from patients and controlsbefore blood samples were taken.

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Figure 1. Family Tree. The figure shows the genotype, age, and iron indices (serum iron, transferrin saturation and serum ferritin) for the proband (number II.1) and her relatives. *Data concerning the three relatives were obtained recently, while the proband was diagnosed in 1979. She is now 44 years of age.

Hepcidin is a 25 amino-acid peptide that is mainly synthesizedby hepatocytes and plays a central role in iron homeostasis.Through its ability to bind the ferroportin iron exporter andcause its degradation, hepcidin determines the amount of ironthat must be mobilized from macrophages, enterocytes and hepatocytesto meet the body’s needs.⁴ As expected from the initialobservation of reduced hepcidin levels in patients with HJVmutations,² and subsequently in HJV knock-out mice,⁵ there isa strong functional relationship between the two gene productsinvolved in JH. While some important aspects still need to beclarified, a major advance towards a better understanding ofthis relationship was recently made by Babitt and co-workers.Indeed, these authors have demonstrated that HJV is a bone morphogenicprotein (BMP) co-receptor that up-regulates hepcidin synthesisat the transcriptional level via the classical BMP cell-signalingpathway. In turn, they have shown that hepcidin induction bythe BMP pathway is significantly reduced in hepatocytes lackingHJV. Therefore, they have proposed that enhancement of BMP intracellularsignaling by HJV is an important mechanism for regulating hepcidinexpression.⁶ To demonstrate causality of p.R176C substitution,we designed a hepcidin promoter-based luciferase reporter assayin human Hep3B hepatoma cells and used either HJV or the combinationof HJV and exogenous BMP-9 as mediator. BMP-9 was chosen because,at low doses, its potency to activate hepcidin transcriptionin HepG2 cells had proved to be higher than that of other BMPligands, and especially BMP-2.⁷ We first observed that wild-typeHJV increases the hepcidin promoter activity in a dose-dependentmanner (Figure 2A) and also confirmed that it enhances the BMPmediated stimulating effect (Figure 2B). We next establishedthat, similarly to the predominant p.G320V HJV mutant, the p.R176Cvariant fails to stimulate transcription of the hepcidin gene.The failure was apparent with and without BMP-9 addition (Figures 2B),suggesting an important loss of function. HJV exists in a plasmamembrane (m-HJV) and a soluble form (s-HJV). Silvestri and co-workershave recently shed new light on the processing of these twoforms. In particular. they have shown that m-HJV differs inthat it is extensively modified by cleavage of the Asp172-Pro173bond and the formation of disulfide bonds between the two cleavedprotein fragments. They have further demonstrated that cleavageof the Asp172-Pro173 bond, which is supported by a conservedGDPH motif and probably occurs in the late secretory pathway,is necessary for export to plasma membrane. In agreement withthese findings, the p.F170S mutant was reported to be efficientlyreleased from Hela cells while it was not cleaved and anchoredonto the cell surface as an active form.⁸ HJV shares considerablesequence similarity with the Repulsive Guidance Molecules (RGMs)and is the ortholog of a mouse RGM family member (i.e. RGMc).Remarkably, orthologs (RGMc) and paralogs (RGMa and RGMb) ofhuman HJV exhibit conserved amino-acid residues surroundingthe essential GDPH cleavage sequence. These residues includephenylalanine 170 and arginine 176 (Figure 2C). Consideringboth the case of the p.F170S mutant and the proposal by Aguilar-Martinezand co-workers of a localized protein structure defect (i.e.the destabilization of a short helix forms by the R176, S177and F178 residues)³, it could be suggested that the p.R176Cmutant is not efficiently cleaved. It would not, therefore,be able to induce the hepcidin gene transcription from the cellsurface. However, as the p.R176C substitution introduces anextra cysteine into a primary amino-acid sequence that naturallycomprises 14 cysteine residues, the hypothesis of a criticalstructural change impairing the HJV folding and its proper traffickingthrough the ER/Golgi compartments cannot be ruled out. Furtherexperiments are, therefore, required to provide further insightinto the biosynthesis and maturation of the p.R176C mutant.In conclusion, our results definitively show the R176C amino-acidchange as a novel hemojuvelin loss-of-function mutation.

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Figure 2. Functional study of the hemojuvelin p.R176C substitution. (A) Hep3B cells, cultured in 6 well plates, were transiently co-transfected with a hepcidin promoter-luciferase reporter plasmid (0.8 µg), a pCMV-ßgalactosidase vector (0.2 µg; to control for transfection efficiency) and 0.25 to 1 µg of a pcDNA3.1 plasmid containing the full-length human HJV coding sequence (pHJV_wt). As negative control (CTL), cells were incubated with the commercial pcDNA3.1 vector (instead of the pHJV_wt plasmid construct). The hepcidin promoter-based luciferase reporter plasmid construct was generated by cloning the –1458 to +43 region of the human hepcidin promoter (+1 refers to the beginning of transcription; Genbank #AD000684) into the commercial pGL3-basic vector. B. The hepcidin promoter-based luciferase reporter plasmid (0.8 µg) was co-transfected into Hep3B cells with the pCMV-ßgalactosidase vector (0.2 µg) and either the commercial pcDNA3.1 vector (0.5 µg; CTL) or a pHJV-related plasmid construct (0.5 µg; either pHJV_wt, pHJV_G320V or pHJV_R176C). Twelve hours after transfection cells were serum-starved for 6 hours and treated (+BMP) or not (–BMP) with 0.2 ng/mL BMP-9 for 16 hours. Results are expressed as mean ± s.d., n=3 in each group. They are representative of two independent experiments. Quantitative RT-PCR analysis confirmed that similar amounts of mRNA were generated from all the pHJV plasmid contructs (data not shown). (C) Sequence comparisons of the human, mouse, rat and chicken RGM molecules deposited in the Swissprot database (http://www.ebi.ac.uk/swissprot). Selected proteins are aligned with the sequence surrounding the GDPH tetra amino-acid motif of human HJV (i.e. human RGMc). The residue numbers refer to the putative initiating methionine.

Footnotes

Funding: this work was supported by grants from the Centre HospitalierUniversitaire de Brest (Programme Hospitalier de Recherche Clinique),the conseil scientifique de l’Etablissement Françaisdu Sang (projet 2003.19) and by the Fondation pour la RéchercheMédicale.

References

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Camaschella C, Roetto A, De Gobbi M. Juvenile haemochromatosis. Semin Hematol 2002;39:242-8.[CrossRef][Web of Science][Medline]
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Aguilar-Martinez P, Lok CY, Cunat S, Cadet E, Robson K, Rochette J. Juvenile hemochromatosis caused by a novel combination of hemojuvelin G320V/R176C mutations in a 5-year old girl. Haematologica 2007;92:421-2.[Abstract/Free Full Text]
Fleming RE, Bacon BR. Orchestration of iron homeostasis. N Engl J Med 2005;352:1741-4.[Free Full Text]
Franklin W, Huang FW, Pinkus JL, Fleming MD, Andrews NC. A mouse model of juvenile haemochromatosis. J Clin Invest 2005;115:2187-91.[CrossRef][Web of Science][Medline]
Babitt JL, Huang FW, Wrighting DM, Xia Y, Sidis Y, Samad TA, et al. Bone morphogenetic protein signaling by hemojuvelin regulates hepcidin expression. Nat Genet 2006;38:531-3.[CrossRef][Web of Science][Medline]
Truksa J, Peng H, Lee P, Beutler E. Bone morphogenic proteins 2, 4 and 9 stimulate murine hepcidin 1 expression independently of Hfe, transferrin receptor 2 (Tfr2), and IL-6. Proc Natl Acad Sci USA 2006;103:10289-93.[Abstract/Free Full Text]
Silvestri L, Pagani A, Fazi C, Gerardi G, Levi S, Arosio P, et al. Defective targeting of hemojuvelin to plasma membrane is a common pathogenic mechanism in juvenile hemochromatosis. Blood 2007;109:4503-10.[Abstract/Free Full Text]

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