Hemochromatosis mutations in the general population: iron overload progression rate

doi:10.1182/blood-2003-10-3564

Blood online

SEARCH:

Advanced

Blood, 15 April 2004, Vol. 103, No. 8, pp. 2914-2919.
Prepublished online as a Blood First Edition Paper on December 4, 2003; DOI 10.1182/blood-2003-10-3564.

This Article

Abstract

Full Text (PDF)

All Versions of this Article:
2003-10-3564v1
103/8/2914    most recent

Alert me when this article is cited

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Rights and Permissions

Citing Articles

Citing Articles via HighWire

Citing Articles via CrossRef

Citing Articles via Google Scholar

Google Scholar

Articles by Andersen, R. V.

Articles by Nordestgaard, B. G.

Search for Related Content

PubMed

PubMed Citation

Articles by Andersen, R. V.

Articles by Nordestgaard, B. G.

Related Collections

Red Cells

Clinical Trials and Observations

Social Bookmarking


What's this?

Previous Article  |  Table of Contents  |  Next Article
CLINICAL OBSERVATIONS, INTERVENTIONS, AND THERAPEUTIC TRIALS
Hemochromatosis mutations in the general population: iron overload progression rate
Rolf Værn Andersen, Anne Tybjærg-Hansen, Merete Appleyard, Henrik Birgens, and Børge Grønne Nordestgaard
From the Department of Clinical Biochemistry and Department of Hematology, Herlev University Hospital, Copenhagen, Denmark; Department of Clinical Biochemistry, Rigshospitalet, Copenhagen University Hospital, Copenhagen, Denmark; and The Copenhagen City Heart Study, Bispebjerg University Hospital, University of Copenhagen, Copenhagen, Denmark..

   Abstract

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

The progression rate of iron overload in hereditary hemochromatosisin individuals in the general population is unknown. We thereforeexamined in the general population iron overload progressionrate in C282Y homozygotes. Using a cohort study of the Danishgeneral population, The Copenhagen City Heart Study, we genotyped9174 individuals. The 23 C282Y homozygotes identified were matchedto 2 subjects each of 5 other HFE genotypes with respect tosex, age, and alcohol consumption. As a function of biologicage, transferrin saturation increased from 50% to 70% from 25to 85 years of age and from 70% to 80% from 35 to 80 years ofage in female and male C282Y homozygotes, respectively. Equivalently,ferritin levels increased from 100 to 500 µg/L and decreasedfrom 800 to 400 µg/L in female and male C282Y homozygotes.As a function of 25 years follow-up irrespective of age, transferrinsaturation and ferritin levels increased slightly in male andfemale C282Y homozygotes. None of the C282Y homozygotes developedclinically overt hemochromatosis. In conclusion, individualsin the general population with C282Y homozygosity at most demonstratemodest increases in transferrin saturation and ferritin levels,and clinically overt hemochromatosis is rare. Therefore, C282Yhomozygotes identified during population screening, and notbecause of clinically overt hemochromatosis, at most need tobe screened for manifestations of hemochromatosis every 10 to20 years. (Blood. 2004;103: 2914-2919)

   Introduction

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Hereditary hemochromatosis is a disease caused by iron accumulationin the body due to excess iron absorption from the intestinaltract.¹ This leads to increased transferrin saturation and ferritinlevels, and may cause progressive organ damage such as livercirrhosis, type 1 diabetes mellitus, hypogonadotropic hypogonadism,cardiomyopathy, arthritis, and bronze coloring of the skin.Most hereditary hemochromatosis patients are homozygous forC282Y (Cys282Tyr) of the HFE gene.²
Hereditary hemochromatosis may be one of the most common geneticdisorders among people of Northern European descent.^3,4 Therefore,hereditary hemochromatosis could be an ideal condition for populationscreening^5,6; however, penetrance of C282Y homozygosity remainscontroversial.^7-19 Accordingly, before such screening procedurescan be recommended we need to know the iron overload progressionrate among healthy C282Y homozygotes in individuals from thegeneral population.
We genotyped 9174 individuals from the Danish general population,The Copenhagen City Heart Study.²⁰ Measured as increases intransferrin saturation and ferritin levels, we studied ironoverload progression rate in C282Y homozygotes during 25 yearsfollow-up. In addition, we assessed all symptoms, signs, hospitalizations,and deaths of C282Y homozygotes.

   Patients, materials, and methods

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Subjects
The basis for this study was 9174 subjects from The CopenhagenCity Heart Study (third examination, 1991-1994).^20,21 Theseindividuals were selected after age and sex stratification basedon the Danish Central Population Register code to representthe Danish general population.
More than 99% were of white Danish descent. The study protocolconformed to the ethical guidelines of the Declaration of Helsinki:the study was approved by the Steering Committee of The CopenhagenCity Heart Study, Herlev University Hospital, and the Danishethics committee for Copenhagen and Frederiksberg (No.100.2039/91).All participants gave written informed consent in accordancewith the Helsinki protocol.
Design
In a cross-sectional design, each subject homozygous for C282Ywas matched to 2 subjects each of wild type/wild type, H63D/wildtype, H63D/H63D, C282Y/wild type, and C282Y/H63D genotypes withrespect to sex, age (in 10-year groups), and alcohol consumption(in sex-specific tertiles).
To study iron overload progression rate, the matched individualsof wild type/wild type, C282Y/H63D, and C282Y/C282Y genotypeswere used to follow the development of iron status from 25 to85 years of age; we followed each individual for up to 25 yearscomprising 4 investigations between 1976 and 2001. Plasma samplesfrom 1976 to 1978 and 1981 to 1983 stored at -20°C, serumsamples from 1991 to 1994 stored at -80°C, as well as newlydrawn serum samples from 2001 were used.
To study lifetime penetrance, we conducted a fourth examinationin 2001 comprising the 20 C282Y homozygotes still alive. Duringthis examination, blood samples were obtained and in additionpatients were questioned about possible illnesses and examinedphysically by a hemochromatosis specialist (H.B.). Previousdisease was also assessed by reviewing the Danish National HospitalDischarge Register and the Danish National Register of Causesof Deaths; these registers cover all citizens of Denmark andall Danish hospitals from 1976 through 1999.
Measurements
Hemochromatosis genotyping was as described.²⁰ Transferrin wasmeasured on a Nephelometer Analyzer II (Behring, Düdingen,Switzerland), while follicle-stimulating hormone levels, luteinizinghormone levels, and ferritin levels were determined on a TechniconImmuno 1 System (Bayer, Leverkusen, Germany). Ferritin levelhigher than 250 µg/L in men and higher than 200 µg/Lin women was chosen as indication of iron overload. Aspartateaminotransferase was measured on a Hitachi 705 autoanalyzer(Hitachi, Tokyo, Japan). Albumin levels, alkaline phosphataselevels, bilirubin levels, and iron levels (except for the 1976-1978and 1981-1983 samples) were measured on a Vitros 950 autoanalyzer(Johnson & Johnson, Rochester, NY). Because plasma samplesfrom the 1976-1978 and 1981-1983 investigations contained EDTA(ethylenediaminetetraacetic acid), iron contents of these sampleswere measured by atomic absorption photometry on a Perkin-Elmer403 photometer (Shelton, CT).
Statistical analyses
Statistical analyses were performed using SPSS.²² A P valueless than .05 on a 2-sided test was significant. Correctionfor multiple comparisons was not performed. A priori we stratifiedby sex. We used Mann-Whitney U test for 2-genotype comparisons.The smoothed relation between age and transferrin saturationand ferritin levels (log transformed) in different genotypegroups was investigated using local linear regression (smootherfunction, normal kernel, bandwidth multiplier value = 5 years);ferritin levels were log transformed to approach normal distribution.

   Results

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Of 9174 subjects from the Danish general population, 6135 werewild type/wild type (66.9%; 95% CI, 65.9%-67.8%), 1881 wereH63D/wild type (20.5%; 95% CI, 19.7%-21.3%), 158 were H63D/H63D(1.7%; 95% CI, 1.5%-2.0%), 846 were C282Y/wild type (9.2%; 95%CI, 8.6%-9.9%), 131 were C282Y/H63D compound heterozygous (1.4%;95% CI, 1.2%-1.7%), and 23 were homozygous for C282Y (0.25%;95% CI, 0.16%-0.38%).²⁰
Iron status cross-sectionally
Transferrin saturation levels were increased in C282Y homozygotes(P < .001), C282Y/H63D compound heterozygotes (P < .001),C282Y/wild type (P < .05), and H63D/H63D (P < 0.01) whencompared with wild type/wild type (Figure 1). These differencesin C282Y homozygotes and C282Y/H63D compound heterozygotes versuswild type/wild type were similar when men and women were examinedseparately. Only C282Y homozygotes had average transferrin saturationlevels above 50%.

View larger version (36K):
[in this window]
[in a new window]
Figure 1.. Average levels with standard error of iron status parameters as a function of HFE genotype. Twenty-three C282Y homozygotes were each matched for sex, age, and alcohol consumption with 2 persons each of the 5 other genotypes. Due to technical error, the sample from one of the 23 C282Y homozygotes was not measured, and consequently the 2 matched persons in each of the other genotypes were also excluded. Dashed lines are upper borders of reference intervals; for ferritin these borders differ between women and men. Levels in mutation carriers were tested against wild type/wild type (WT/WT) levels using Mann-Whitney U tests: ^*P = .05, ^**P = .01, ^***P = .001. Error bars indicate the standard error of the mean.

Ferritin levels were increased in C282Y homozygotes comparedwith wild type/wild type, irrespective of whether men and womenwere examined separately or together (Figure 1). However, therewas no difference in ferritin levels between C282Y/H63D compoundheterozygotes and wild type/wild type, indicating that individualswith this genotype did not show evidence of iron overload.
Iron overload progression rate
Transferrin saturation increased from 50% at 25 years of ageto 70% at 85 years of age in female C282Y homozygotes and from70% at 35 years of age to 80% at 80 years of age in male C282Yhomozygotes on local linear regression analysis, whereas transferrinsaturation did not increase with age in female or male wildtype/wild type individuals and in female or male C282Y/H63Dcompound heterozygotes (Figure 2). Transferrin saturation valuesoscillated most in C282Y homozygotes, somewhat less in C282Y/H63Dcompound heterozygotes, and least in wild type/wild type individuals.

View larger version (33K):
[in this window]
[in a new window]
Figure 2.. Levels of transferrin saturation and ferritin in selected genotypes over a follow-up period of up to 25 years, shown as a function of age at measurement. Twenty-three C282Y homozygotes were each matched for sex, age, and alcohol consumption with 2 persons each of wild type/wild type and C282Y/H63D genotypes. Data for a given individual are connected with lines. Panels to the right show local linear regression curves for women and men separately.

From 25 to 85 years of age, ferritin levels increased from 120to 500 µg/L in female C282Y homozygotes, from 30 to 150µg/L in female C282Y/H63D compound heterozygotes, andfrom 25 to 80 µg/L in female wild type/wild type individuals(Figure 2). From 35 to 80 years of age, ferritin levels declinedfrom 800 to 400 µg/L in male C282Y homozygotes, were stablearound 150 µg/L in male C282/H63D compound heterozygotes,but increased in male wild type/wild type individuals from 40to 150 µg/L. Ferritin values oscillated more in C282Yhomozygotes than in wild type/wild type individuals or in C282/H63Dcompound heterozygotes.
As a function of 25-, 15-, and 15-year follow-up in female andmale C282Y homozygotes, C282Y/H63D compound heterozygotes, andwild type/wild type individuals, respectively, transferrin saturationincreased modestly at most (Figure 3). This was also the casefor ferritin levels.

View larger version (34K):
[in this window]
[in a new window]
Figure 3.. Levels of transferrin saturation and ferritin in selected genotypes over a follow-up period of up to 25 years, shown as a function of follow-up time. Twenty-three C282Y homozygotes were each matched for sex, age, and alcohol consumption with 2 persons each of wild type/wild type and C282Y/H63D genotypes. Data for a given individual are connected with lines. Panels to the right show local linear regression curves for women and men separately.

Lifetime penetrance
Of the 23 C282Y homozygotes, 14 women and 6 men with medianages of 66 years (range, 35-85 years) and 62 years (range, 45-81years) were alive in 2001 (Table 1). Only 4 of these had beenblood donors, and only one gave more than 50 units. One patientdied from lung cancer, one patient died from atheroscleroticheart disease, and one patient died from malignant melanoma.

View this table:
[in this window]
[in a new window]
Table 1.. Characteristics of C282Y homozygotes at the 2001 investigation

Clinically overt hemochromatosis was not diagnosed in any ofthe 23 C282Y homozygotes before the study (Table 1); one wasaccidentally diagnosed with increased iron levels, which leadto measurement of transferrin saturation of 80% and ferritinlevel of 452 µg/L and the subsequent finding of C282Yhomozygosity without clinically overt hemochromatosis (no.17).Among C282Y homozygotes, 13 of 16 women and 5 of 7 men developedtransferrin saturation higher than 50%. Iron overload definedas ferritin level higher than 200 µg/L was found in 10of 16 women, and iron overload defined as ferritin level higherthan 250 µg/L was found in 6 of 7 men.
Liver disease or enlargement was not observed in any of theC282Y homozygotes (Table 1). Diabetes mellitus type 1 was onlyfound in one C282Y homozygote, a 77-year-old woman diagnosedat 72 years of age (Table 1 no.13). Lack of secondary hypogonadismwas demonstrated by normal age-adjusted values of follicle-stimulatinghormone and luteinizing hormone in all C282Y homozygotes (Table 1).Levels of aspartate aminotransferase, follicle-stimulatinghormone, and luteinizing hormone did not differ between C282Yhomozygotes and wild type/wild type (Figure 4). None of theC282Y homozygotes received treatment for heart failure, indicatinglack of hemochromatosis-associated cardiomyopathy (Table 1).Two homozygotes had acute myocardial infarction at 55 yearsof age (no. 21) and 68 years of age (no. 13). Two C282Y homozygoteshad universal arthralgias (Table 1 nos.1 and 7), but none hadclinical signs of arthritis at physical examination. None ofthe homozygotes had skin darkening.

View larger version (20K):
[in this window]
[in a new window]
Figure 4.. Average levels with standard error of aspartate aminotransferase (ASAT), follicle-stimulating hormone (FSH), and luteinizing hormone (LH) as a function of HFE genotype. Twenty-three C282Y homozygotes were each matched for sex, age, and alcohol consumption with 2 persons each of the 5 other genotypes. Levels in mutation carriers were tested against wild type/wild type (WT/WT) levels using Mann-Whitney U tests, none were significant. Error bars indicate standard error of the mean.

   Discussion

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Iron overload progression rate
Transferrin saturation increased from 50% to 70% from 25 to85 years of age and from 70% to 80% from 35 to 80 years of agein female and male C282Y homozygotes, respectively, a phenomenonnot observed for other genotypes. Within the same age ranges,ferritin levels increased from 100 to 500 µg/L and decreasedfrom 800 to 400 µg/L in female and male C282Y homozygotes.Our observation of at most only modest increases in transferrinsaturation and ferritin levels with increasing age in C282Yhomozygotes are in accordance with results of previous cross-sectionalstudies.^8-15
Pathophysiologically, our data are compatible with the ideathat most C282Y homozygotes in the population at large willdevelop biochemical iron overload early in adult life. Thereafter,the rate of increase in ferritin levels and probably in accumulationof iron is not larger in C282Y homozygotes than in individualswithout C282Y homozygosity. Thus, most C282Y homozygotes willonly reach a level of modest iron overload.
Each C282Y homozygote had an oscillating course in ferritinlevels. Some even had stable or decreasing levels, indicatinglack of progressive iron loading. This is in accordance withthe study of Olynyk et al,¹⁶ where 5 of 12 C282Y homozygoteshad static or decreasing ferritin levels during a 4-year observationperiod. We have no explanation for why one patient dropped fromgreater than 1000 µg/L to less than half the initial value.He was not treated with phlebotomy or loosing blood in anothermanner.
Lifetime penetrance
Our data indicate that, although the majority of C282Y homozygotesbiochemically had iron overload, none developed clinically overthemochromatosis. The only patient known to be a C282Y homozygotebefore this study was accidentally diagnosed and did not sufferfrom hemochromatosis. Only one patient had unequivocal biochemicalsigns of hemochromatosis, since he had serum ferritin levelhigher than 2000 µg/L and aspartate aminotransferase atthe upper limit of the normal range, suggesting that he mighthave hepatic fibrosis.²³ In addition, one woman had been a blooddonor more than 50 times, and therefore these phlebotomies couldhave protected her from developing clinically overt hemochromatosis.The C282Y homozygote with type 1 diabetes mellitus had a verylate disease onset and only slightly increased ferritin levels,and therefore her diabetes mellitus might not be related tohemochromatosis. Finally, the 2 C282Y homozygotes who sufferedfrom nonspecific arthralgias had ferritin levels of only 280and 330 µg/L, indicating that hemochromatosis most likelywas not responsible for these complaints. In accordance withthis, Beutler et al⁷ did not observe differences between C282Yhomozygotes and controls with respect to joint complaints.
Therefore, among the patients still alive in 2001, at most oneC282Y homozygote had biochemical signs compatible with subclinicalhemochromatosis, indicating a penetrance of 0% to 5% at 64 yearsof age, which is supported by 3 previous studies.^7-9 Consequently,other previous studies suggesting that at least half of C282Yhomozygotes ultimately will develop clinical signs of hemochromatosis^16-19clearly is not supported by our data. In the present study,all living C282Y homozygotes were informed about their genotypestatus, the possibility of a slightly increased risk of developinghemochromatosis, and that phlebotomy could be considered nowor later on. Of the 20 C282Y homozygotes still alive in 2001,all were referred to a hospital for further control and possibletreatment for hemochromatosis (in 2001), which therefore willnot affect the results of the present study. Before the study,only 1 of 23 homozygotes was treated with phlebotomy, but thisperson did not suffer from hemochromatosis.
Potential limitations
First, the low penetrance of C282Y homozygosity in this studymost likely was not due to selection bias, since all individualswere randomly selected from the general population of Copenhagen.²¹Second, since clinical manifestations in hereditary hemochromatosiswill not appear before 40 years of age,²⁴ we could have studiedindividuals who were too young; however, median ages at investigationwere 66 and 62 years in female and male C282Y homozygotes, makingthis possibility unlikely. Third, since women develop manifestationsof hemochromatosis later in life than men and usually in a milderform,²⁴ the minority of men in our study could have influencedthe result in favor of lesser iron overload. However, this wasprobably not the case, since our results agree with 2 largepopulation-based studies and a study of blood donors evaluatingthe clinical penetrance of C282Y homozygosity.^7-9 A similarlow penetrance was also suggested by a large necropsy studyof patients with liver cirrhosis.²⁵ Fourth, as we found fewermale (7 homozygotes among 4096 participants = 0.17%; 95% CI,0.07%-0.35%) than female C282Y homozygotes (16 among 5078 participants= 0.32%; 95% CI, 0.18%-0.51%), the former could have died atan earlier age or not been able to participate in The CopenhagenCity Heart Study; however, the average age of male C282Y homozygoteswas similar to that of men with other genotypes. Furthermore,the C282Y genotype frequencies in our study did not differ fromthat predicted from the Hardy-Weinberg equilibrium (women andmen, P = .35; women, P > .9; men, P = .10). Fifth, it seemsunlikely that we underdiagnosed the 282Y allele, because C282Ygenotype frequencies did not differ from the Hardy-Weinbergequilibrium and because the 95% confidence interval for theallele frequency for 282Y in our study of 5.3% to 5.9% overlappedthat reported for 219 Danish newborns of 5.5% to 10.9%.²⁶
Regarding progression with age, the main objective of the presentstudy, the relatively small number of C282Y homozygotes, representsa limitation. Of the 23 patients only 7 were men, the most criticalsubgroup in the study, and only 3 of these men were youngerthan 50 years of age at the last analysis. This is a rathersmall group to reach firm conclusions regarding age-relatedchanges in patients ranging from 35 to 80 years of age. Therefore,to increase the statistical power, iron load progression ratewas examined according to the length of follow-up as well asa function of biologic age. Concerning transferrin saturation,the conclusion was similar from the 2 different plots, namelythat transferrin saturation increased slightly with age in bothfemale and male C282Y homozygotes. This was also the case forferritin levels in female C282Y homozygotes; both plots demonstratedmoderate increases with age. Progression in ferritin levelsin male C282Y homozygotes differed in the 2 plots. As a functionof increasing biologic age, ferritin levels seemed to decrease;however, this most likely was caused by the 2 relatively youngmales with very high ferritin levels (Figure 2). Thus, as afunction of follow-up time, ferritin levels increased slightlyeven in male C282Y homozygotes (Figure 3).
Regarding phenotype, the work up was not completely satisfactory.A rough clinical evaluation is not enough to determine conclusivelythat clinical disease is negligible. Three of the 23 homozygoteshad serum ferritin levels greater than 1000 up to 2433 µg/Land many had transferrin saturation greater than 75%. In suchpatients we cannot totally exclude liver fibrosis or cirrhosis.Therefore, initially we considered whether we should performliver biopsies on these participants; however, for ethical reasonswe abstained from performing liver biopsy because these personsappeared healthy. All C282Y homozygous individuals were referredfor further control for hemochromatosis.
In conclusion, the average individual in the general populationwith C282Y homozygosity at most demonstrates modest increasesin transferrin saturation and ferritin during 25 years follow-upand rarely develops clinically overt hemochromatosis. Therefore,C282Y homozygotes identified during population screening, andnot because of clinically overt hemochromatosis, at most needto be screened for manifestations of hemochromatosis every 10to 20 years.
The future challenge will be to identify the few C282Y homozygoteswho will develop serious progressive iron accumulation leadingto organ damage. Other genetic and environmental factors thatregulate iron absorption and thus may modulate the phenotypeof C282Y homozygotes need to be identified.

   Acknowledgements

We thank Vibeke Wohlgehagen, Hanne Damm, and Nina Kjersgaardfor excellent technical assistance and Niels Fogh-Andersen forintroduction to atomic absorption photometry.

   Footnotes

Submitted October 22, 2003; accepted December 2, 2003.
Prepublished online as Blood First Edition Paper, December 4,2003; DOI 10.1182/blood-2003-10-3564.

Supported by the Danish Heart Foundation and Chief PhysicianJohan Boserup's and Lise Boserup's Fund.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Børge G. Nordestgaard, Dept Clinical Biochemistry, Herlev University Hospital, Herlev Ringvej 75, DK-2730 Herlev, Denmark; e-mail: brno{at}herlevhosp.kbhamt.dk.

   References

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Beutler E, Bothwell TH, Charlton RW, Motulsky AG. Hereditary hemochromatosis. In: Scriver CR, Beaudet AL, Sly WS, Valle D, eds. The metabolic and molecular bases of inherited disease. 8th ed. New York, NY: McGraw-Hill; 2001: 3127-3161.

Feder JN, Gnirke A, Thomas W, et al. A novel MHC class I-like gene is mutated in patients with hereditary haemochromatosis. Nat Genet. 1996;13: 399-408.[CrossRef][Medline] [Order article via Infotrieve]

Barton JC, Bertoli LF. Hemochromatosis: the genetic disorder of the twenty-first century. Nat Med. 1996;2: 394-395.[CrossRef][Medline] [Order article via Infotrieve]

Smith BN, Kantrowitz W, Grace ND, et al. Prevalence of hereditary hemochromatosis in a Massachusetts corporation: is Celtic origin a risk factor? Hepatology. 1997;25: 1439-1446.[CrossRef][Medline] [Order article via Infotrieve]

Edwards CQ, Griffen LM, Ajioka RS, Kushner JP. Screening for hemochromatosis: phenotype versus genotype. Semin Hematol. 1998;35: 72-76.[Medline] [Order article via Infotrieve]

Adams PC. Population screening for hemochromatosis. Hepatology. 1999;29: 1324-1327.[CrossRef][Medline] [Order article via Infotrieve]

Beutler E, Felitti VJ, Koziol JA, Ho NJ, Gelbart T. Penetrance of 845G $->$ A (C282Y) HFE hereditary haemochromatosis mutation in the USA. Lancet. 2002;359: 211-218.[CrossRef][Medline] [Order article via Infotrieve]

Åsberg A, Hveem K, Krüger Ø, Bjerve KS. Persons with screening-detected haemochromatosis: as healthy as the general population? Scand J Gastroenterol. 2002;37: 719-724.[CrossRef][Medline] [Order article via Infotrieve]

Jackson HA, Carter K, Darke C, et al. HFE mutations, iron deficiency and overload in 10,500 blood donors. Br J Haematol. 2001;114; 474-484.[CrossRef][Medline] [Order article via Infotrieve]

Åsberg A, Hveem K, Thorstensen K, et al. Screening for hemochromatosis: high prevalence and low morbidity in an unselected population of 65,238 persons. Scand J Gastroenterol. 2001;36: 1108-1115.[CrossRef][Medline] [Order article via Infotrieve]

Beaumont C, Simon M, Fauchet R, et al. Serum ferritin as a possible marker of the hemochromatosis allele. N Engl J Med. 1979;301: 169-174.[Abstract]

Meyer T, Baynes R, Bothwell T, et al. Phenotypic expression of the HLA linked iron-loading gene in males over the age of 40 years: a population study using serial serum ferritin estimations. J Intern Med. 1990;227: 397-406.[Medline] [Order article via Infotrieve]

Milman N, Clausen JO, Jordal R. Iron status in young Danish men and women: a population survey comprising 548 individuals. Ann Hematol. 1995;70: 215-221.[Medline] [Order article via Infotrieve]

Bassett ML, Halliday JW, Ferris RA, Powell LW. Diagnosis of hemochromatosis in young subjects: predictive accuracy of biochemical screening tests. Gastroenterology. 1984;87: 628-633.[Medline] [Order article via Infotrieve]

Beutler E, Felitti V, Gelbart T, Ho N. The effect of HFE genotypes in patients attending a health appraisal clinic. Ann Intern Med. 2000;133: 329-337.[Abstract/Free Full Text]

Olynyk JK, Cullen DJ, Aquilia S, Rossi E, Summerville L, Powell LW. A population-based study of the clinical expression of the hemochromatosis gene. N Engl J Med. 1999;341: 718-724.[Abstract/Free Full Text]

Crawford DH, Jazwinska EC, Cullen LM, Powell LW. Expression of HLA-linked hemochromatosis in subjects homozygous or heterozygous for the C282Y mutation. Gastroenterology. 1998;114: 1003-1008.[CrossRef][Medline] [Order article via Infotrieve]

Bradley LA, Haddow JE, Palomaki GE. Population screening for haemochromatosis: a unifying analysis of published intervention trials. J Med Screen. 1996;3: 178-184.[Medline] [Order article via Infotrieve]

Bulaj ZJ, Ajioka RS, Phillips JD, et al. Disease-related conditions in relatives of patients with hemochromatosis. N Engl J Med. 2000;343: 1529-1535.[Abstract/Free Full Text]

Ellervik C, Mandrup-Poulsen T, Nordestgaard BG, et al. Prevalence of hereditary haemochromatosis in late-onset type 1 diabetes mellitus: a retrospective study. Lancet. 2001;358: 1405-1409.[CrossRef][Medline] [Order article via Infotrieve]

Schnohr P, Jensen G, Lange P, Scharling H, Appleyard M. The Copenhagen City Heart Study: tables with data from the third examination 1991-1994. Eur Heart J Suppl. 2001;3: 1-83.

SPSS Base 8.0 for Windows User's Guide and SPSS Interactive Graphics 8.0. Chicago, IL: SPSS Inc; 1998.

Guyader D, Jacquelinet C, Moirand R, et al. Noninvasive prediction of fibrosis in C282Y homozygous hemochromatosis. Gastroenterology. 1998;115: 929-936.[CrossRef][Medline] [Order article via Infotrieve]

Bothwell TH, MacPhail AP. Hereditary hemochromatosis: etiologic, pathologic, and clinical aspects. Semin Hematol. 1998;35: 55-71.[Medline] [Order article via Infotrieve]

Willis G, Wimperis JZ, Lonsdale R, et al. Incidence of liver disease in people with HFE mutations. Gut. 2000;46: 401-404.[Abstract/Free Full Text]

Merryweather-Clarke AT, Simonsen H, Shearman JD, et al. A retrospective anonymous pilot study in screening newborns for HFE mutations in Scandinavian populations. Hum Mutat. 1999;13: 154-159.[CrossRef][Medline] [Order article via Infotrieve]

Add to CiteULike CiteULike    Add to Connotea Connotea    Add to Del.icio.us Del.icio.us    Add to Digg Digg    Add to Reddit Reddit    Add to Technorati Technorati    What's this?

This article has been cited by other articles:

W. H. Rogowski
The Cost-Effectiveness of Screening for Hereditary Hemochromatosis in Germany: A Remodeling Study
Med Decis Making, March 1, 2009; 29(2): 224 - 238.
[Abstract] [PDF]

J. Waalen, V. J. Felitti, T. Gelbart, and E. Beutler
Screening for hemochromatosis by measuring ferritin levels: a more effective approach
Blood, April 1, 2008; 111(7): 3373 - 3376.
[Abstract] [Full Text] [PDF]

K. J. Allen, L. C. Gurrin, C. C. Constantine, N. J. Osborne, M. B. Delatycki, A. J. Nicoll, C. E. McLaren, M. Bahlo, A. E. Nisselle, C. D. Vulpe, et al.
Iron-Overload-Related Disease in HFE Hereditary Hemochromatosis
N. Engl. J. Med., January 17, 2008; 358(3): 221 - 230.
[Abstract] [Full Text] [PDF]

A. Piperno, D. Girelli, E. Nemeth, P. Trombini, C. Bozzini, E. Poggiali, Y. Phung, T. Ganz, and C. Camaschella
Blunted hepcidin response to oral iron challenge in HFE-related hemochromatosis
Blood, December 1, 2007; 110(12): 4096 - 4100.
[Abstract] [Full Text] [PDF]

C. Ellervik, A. Tybjaerg-Hansen, M. Appleyard, H. Sillesen, G. Boysen, and B. G. Nordestgaard
Hereditary hemochromatosis genotypes and risk of ischemic stroke
Neurology, March 27, 2007; 68(13): 1025 - 1031.
[Abstract] [Full Text] [PDF]

U.S. Preventive Services Task Force*
Screening for hemochromatosis: recommendation statement.
Ann Intern Med, August 1, 2006; 145(3): 204 - 208.
[Abstract] [Full Text] [PDF]

E. P. Whitlock, B. A. Garlitz, E. L. Harris, T. L. Beil, and P. R. Smith
Screening for hereditary hemochromatosis: a systematic review for the U.S. Preventive Services Task Force.
Ann Intern Med, August 1, 2006; 145(3): 209 - 223.
[Abstract] [Full Text] [PDF]

D. W. Swinkels, M. C.H. Janssen, J. Bergmans, and J. J.M. Marx
Hereditary Hemochromatosis: Genetic Complexity and New Diagnostic Approaches
Clin. Chem., June 1, 2006; 52(6): 950 - 968.
[Abstract] [Full Text] [PDF]

L. Peltonen, M. Perola, J. Naukkarinen, and A. Palotie
Lessons from studying monogenic disease for common disease.
Hum. Mol. Genet., April 15, 2006; 15(suppl_1): R67 - R74.
[Full Text] [PDF]

L. W. Powell, J. L. Dixon, G. A. Ramm, D. M. Purdie, D. J. Lincoln, G. J. Anderson, V. N. Subramaniam, D. G. Hewett, J. W. Searle, L. M. Fletcher, et al.
Screening for hemochromatosis in asymptomatic subjects with or without a family history.
Arch Intern Med, February 13, 2006; 166(3): 294 - 301.
[Abstract] [Full Text] [PDF]

S. Goland, S. D. Malnick, C. Ellervik, B. G. Nordestgaard, A. Tybjaerg-Hansen, P. Grande, A. Tybjaerg-Hansen, M. Appleyard, and B. G. Nordestgaard
Letter Regarding Article by Ellervik et al, "Hereditary Hemochromatosis and Risk of Ischemic Heart Disease: A Prospective Study and a Case-Control Study" * Response
Circulation, January 3, 2006; 113(1): e10 - e10.
[Full Text] [PDF]

A. Qaseem, M. Aronson, N. Fitterman, V. Snow, K. B. Weiss, D. K. Owens, and for the Clinical Efficacy Assessment Subcommittee
Screening for Hereditary Hemochromatosis: A Clinical Practice Guideline from the American College of Physicians
Ann Intern Med, October 4, 2005; 143(7): 517 - 521.
[Abstract] [Full Text] [PDF]

B. Schmitt, R. M. Golub, and R. Green
Screening Primary Care Patients for Hereditary Hemochromatosis with Transferrin Saturation and Serum Ferritin Level: Systematic Review for the American College of Physicians
Ann Intern Med, October 4, 2005; 143(7): 522 - 536.
[Abstract] [Full Text] [PDF]

C. Ellervik, A. Tybjaerg-Hansen, P. Grande, M. Appleyard, and B. G. Nordestgaard
Hereditary Hemochromatosis and Risk of Ischemic Heart Disease: A Prospective Study and a Case-Control Study
Circulation, July 12, 2005; 112(2): 185 - 193.
[Abstract] [Full Text] [PDF]

P. C. Adams, D. M. Reboussin, C. Leiendecker-Foster, G. C. Moses, G. D. McLaren, C. E. McLaren, F. W. Dawkins, I. Kasvosve, R. T. Acton, J. C. Barton, et al.
Comparison of the Unsaturated Iron-Binding Capacity with Transferrin Saturation as a Screening Test to Detect C282Y Homozygotes for Hemochromatosis in 101 168 Participants in the Hemochromatosis and Iron Overload Screening (HEIRS) Study
Clin. Chem., June 1, 2005; 51(6): 1048 - 1052.
[Full Text] [PDF]

P. C. Adams, D. M. Reboussin, J. C. Barton, C. E. McLaren, J. H. Eckfeldt, G. D. McLaren, F. W. Dawkins, R. T. Acton, E. L. Harris, V. R. Gordeuk, et al.
Hemochromatosis and Iron-Overload Screening in a Racially Diverse Population
N. Engl. J. Med., April 28, 2005; 352(17): 1769 - 1778.
[Abstract] [Full Text] [PDF]

K. Juul, B. G. Nordestgaard, and A. Tybjaerg-Hansen
Factor V Leiden and Venous Thromboembolism
Ann Intern Med, September 21, 2004; 141(6): 484 - 485.
[Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

All Versions of this Article:
2003-10-3564v1
103/8/2914    most recent

Alert me when this article is cited

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Rights and Permissions

Citing Articles

Citing Articles via HighWire

Citing Articles via CrossRef

Citing Articles via Google Scholar

Google Scholar

Articles by Andersen, R. V.

Articles by Nordestgaard, B. G.

Search for Related Content

PubMed

PubMed Citation

Articles by Andersen, R. V.

Articles by Nordestgaard, B. G.

Related Collections

Red Cells

Clinical Trials and Observations

Social Bookmarking


What's this?

  Copyright © 2004 by American Society of Hematology         Online ISSN: 1528-0020





	Copyright © 2004 by American Society of Hematology Online ISSN: 1528-0020