To the editor:
In their recent article, Waalen et al1 address an important question connected to screening programs for hemochromatosis: How to find the individuals that would benefit from treatment. Based on their own results and those of others,1,2 including ours,3,4 they recommend serum ferritin as a better screening test than transferrin saturation (TS) for detecting clinically significant hemochromatosis (defined as C282Y homozygotes at risk for liver cirrhosis, that is, serum ferritin above 1000 μg/L). According to Waalen et al1 our phenotypic screening of 65 238 unselected individuals in a geographically stable Norwegian population, using TS as the primary test,3 “would only have detected approximately one-half of the C282Y homozygotes.” This statement may be true for women, but is definitely not correct for men. By genotyping subjects with confirmed high TS, we estimated a C282Y homozygous prevalence of 0.68% in the male population,3 a figure virtually identical to a prevalence estimate of 0.67% (allele frequency 0.081) based on genotyping 3050 randomly selected subjects from the same general population.5 Thus, our screening with TS picked up very close to 100% of homozygous men.
In the Norwegian study, 70% (32 of 46 individuals) of those with ferritin above 1000 μg/L were C282Y homozygotes (Table 1), compared with the 34% (20 of 59 individuals) in the material of Waalen et al.1 Thus, if the primary goal of the screening is to detect C282Y homozygotes with serum ferritin above 1000 μg/L, a prescreening with TS or the equivalent test unsaturated iron binding capacity (UIBC) obviously increases the positive predictive value compared with serum ferritin alone. Reserving serum ferritin testing for men and women with TS above 45% would detect all C282Y homozygous subjects with high serum ferritin in the Waalen et al material.1 This procedure would also be less expensive, as TS and UIBC tests are cheaper than serum ferritin.6 However, the serum ferritin limit of 1000 μg/L may not be optimal. Among 12 C282Y homozygous subjects with liver fibrosis and/or cirrhosis we detected 4 subjects (including 1 with possible cirrhosis) with serum ferritin well below 1000 μg/L (range 311-629 μg/L).3
Findings in 46 subjects with serum ferritin above 1000 μg/L
| HFE genotype . | n . | Age, y* . | Serum ferritin, μg/L† . | Clinical diagnosis‡ . |
|---|---|---|---|---|
| C282Y/C282Y | ||||
| Men | 28 | 48.6 (10.9) | 1612 (1383-1879) | Hemochromatosis: 28 |
| Women | 4 | 54.8 (17.3) | 1164 (912-1484) | Hemochromatosis: 4 |
| Other HFE mutations | ||||
| Men | 1 | 55.0 | 1473 | Alcohol overuse: 1 |
| Women | 4 | 76.8 (8.3) | 1989 (1084-3651) | Hemochromatosis: 1; chronic iron overdose: 2; uncertain: 1 |
| No HFE mutation or HFE genotype unknown | ||||
| Men | 5 | 51.0 (14.6) | 1766 (1072-2908) | Hemochromatosis: 2; lymphoma: 1§;leukemia: 1§; chronic iron overdose: 1 |
| Women | 4 | 75.5 (12.4) | 1489 (1077-2059) | Chronic iron overdose: 4¶ |
| HFE genotype . | n . | Age, y* . | Serum ferritin, μg/L† . | Clinical diagnosis‡ . |
|---|---|---|---|---|
| C282Y/C282Y | ||||
| Men | 28 | 48.6 (10.9) | 1612 (1383-1879) | Hemochromatosis: 28 |
| Women | 4 | 54.8 (17.3) | 1164 (912-1484) | Hemochromatosis: 4 |
| Other HFE mutations | ||||
| Men | 1 | 55.0 | 1473 | Alcohol overuse: 1 |
| Women | 4 | 76.8 (8.3) | 1989 (1084-3651) | Hemochromatosis: 1; chronic iron overdose: 2; uncertain: 1 |
| No HFE mutation or HFE genotype unknown | ||||
| Men | 5 | 51.0 (14.6) | 1766 (1072-2908) | Hemochromatosis: 2; lymphoma: 1§;leukemia: 1§; chronic iron overdose: 1 |
| Women | 4 | 75.5 (12.4) | 1489 (1077-2059) | Chronic iron overdose: 4¶ |
Subjects were detected among 609 individuals with confirmed high transferrin saturation and hemochromatosis not previously known, from a population of 65 238 screened individuals.3 Only the HFE mutations C282Y and H63D were studied.
Mean (SD).
Geometric mean (95% CI).
Given without knowledge of HFE genotype.
Unknown HFE genotype.
Including 2 with unknown HFE genotype.
On the other hand, if the primary goal is to find all subjects with serum ferritin levels above 1000 μg/L and treatable diseases, then measuring serum ferritin would be the right thing to do. However, the utility of screening for all causes of serum ferritin above 1000 μg/L is unknown. And then again, it would not be screening for hemochromatosis.
Lastly, Waalen et al argue that using serum ferritin as the screening test may reduce the anxiety of screening.1 The opposite may also be true: Knowing that you screened negative but your serum ferritin level was 900 μg/L might not be very reassuring.
In our opinion, the present knowledge does not support the statement of Waalen et al1 that “the use of serum ferritin as a screening tool for hemochromatosis seems well worth implementing.”
Authorship
Conflict-of-interest disclosure: The authors declare no competing financial interests.
Correspondence: Arne Åsberg, Department of Clinical Chemistry, Trondheim University Hospital, N-7006 Trondheim, Norway; e-mail: arne.aasberg@stolav.no.
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