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CLINICAL OBSERVATIONS, INTERVENTIONS, AND THERAPEUTIC TRIALS
From Dipartimento di Medicina Interna, Università
di Milano, Ospedale Maggiore IRCCS, Milan, Italy; and Unità di
Epidemiologia, Ospedale Maggiore IRCCS, Milan, Italy.
Severe iron overload usually develops in patients with hereditary
hemochromatosis (HHC), but variability in the phenotypic expression of
the disease has been reported. This study assessed whether tumor
necrosis factor Hereditary hemochromatosis (HHC) is
characterized by progressive iron overload in parenchymal tissue that
may lead to hepatic cirrhosis. The disease is associated with a high
risk of development of hepatocellular carcinoma, cardiomyopathy,
diabetes, hypogonadotropic hypogonadism, skin hyperpigmentation, and
arthritis. In most patients (more than 80% of patients of Northern
European descent and 64% of patients in Italy), HHC is due to
homozygosity for the point mutation C282Y in the HFE gene. The role of
the second mutation, H63D, in the pathogenesis of the disease is still
uncertain.1,2 Half of the subjects homozygous for the
C282Y mutation identified in epidemiological studies did not have
clinical features of HHC, and about one third did not have evidence of
iron overload.3 This suggests the existence of various
acquired and genetic factors that can modify the phenotype of HHC.
Involvement of genetic factors was also suggested by the greater
concordance between clinical manifestations and biochemical markers of
iron within families than between families.4
Tumor necrosis factor Macrophages from patients with HHC have repeatedly been reported to
have a defect in iron metabolism, since a low iron content is usually
found in circulating monocytes, their precursors, and Kupffer cells. In
addition, monocytes from patients with HHC release an increased amount
of ferritin after erythrophagocytosis because they are unable to store
iron.23-25 A possible link between TNF- The aim of this study was to establish whether TNF- Patients
All patients were tested for HFE gene mutations; examined for liver and
spleen enlargement with use of abdominal ultrasonography; and assessed
for skin hyperpigmentation, diabetes (World Health Organization
criteria), cardiomyopathy (electrocardiographic and echocardiographic
examinations), hypogonadism (clinical and hormonal evaluations), and
arthropathy (clinical and radiographic evaluations). All patients were
screened for hepatitis B virus (HBV) surface antigen, anti-hepatitis C
virus (HCV) antibodies, and HCV RNA, and assessed for alcohol abuse,
which was defined as a daily intake of more than 60 g in men and
more than 40 g in women.
Liver biopsy specimens, which were obtained from all patients, were
processed routinely. Tissue sections were stained with hematoxylin and
eosin, impregnated with silver to examine the reticulin framework, and
stained with periodic acid-Schiff for glycogen, periodic Schiff
diastase for nonglycogen proteins, Perls stain for iron, and trichrome
for collagen. Liver iron concentration (LIC) was determined by atomic
absorption spectrophotometry as described previously,30
and the HII, ratio of LIC (µM/g dry weight) to age (years), was
calculated. The amount of iron removed was determined as
reported previously.31
Controls
Isolation of peripheral blood monocytes Peripheral blood monocytes were obtained from patients with iron overload and controls by using the Lymphoprep-Percoll method (Nycomed Amersham, Little Chalfont, United Kingdom)32; a few patients were also tested after iron depletion. Briefly, 30 mL venous blood (plus EDTA) was obtained from each patient and control and diluted with Hanks balanced salts. Blood was then stratified in Lymphoprep solution (ratio of blood to Lymphoprep, 2:1) and centrifuged at 1680 revolutions per minute (rpm) for 30 minutes. The mononuclear cell layer was aspirated and washed 3 times in saline solution. Monocytes were isolated by another separation in Percoll solution by using centrifugation at 2100 rpm for 30 minutes at 4°C and then washed 3 times. Finally, cells were plated (500 000 cells/mL) in 30-mm wells in RPMI 1640 medium supplemented with 10% fetal calf serum, 1% -mercaptoethanol, and 1% streptomycin in the presence or absence of
LPS (5 µg/mL; Sigma Chemical, St Louis, MO). After 24 hours, the
supernatants were collected, centrifuged at 2000 rpm for 10 minutes,
and assayed for TNF- concentration.
To assess the effect of cellular iron content on TNF- Assessment of TNF- release from monocyte-macrophage cells from 50 patients
and 34 controls was measured by using a commercially available enzyme-linked immunosorbent assay (Nycomed Amersham).
Analysis of genomic TNF- DNA samples were amplified in 50 µL ammonia reaction buffer (Bioline, London, United Kingdom) containing 200 µM deoxynucleoside triphosphate, 10 µM each primer, 2 µL DNA sample, and 2 U Taq polymerase (Bioline) for one cycle at 94°C for 4 minutes, 59°C for 1 minute, and 70°C for 45 seconds, followed by 33 cycles at 94°C for 1 minute, 59°C for 1 minute, and 70°C for 45 seconds, followed by one cycle at 70°C for 10 minutes. The polymerase chain reaction (PCR) products were digested at 37°C with NcoI to detect the TNF2 allele and with MspI to detect the TNFA allele and then subjected to 4% agarose-gel electrophoresis. Each PCR batch included a "blank" to which no DNA had been added to ensure that no contamination of samples had occurred. None of the blank reactions yielded any visible product after gel electrophoresis. HFE gene mutations C282Y and H63D HFE mutations were sought in genomic DNA extracted from peripheral leukocytes as described previously.1Statistical analysis Results were expressed as mean (± SD) and considered significant when the P value was less than .05 (2-tailed test). Mean values were compared by using t tests for unequal variances. Frequencies were compared by performing 2 tests. Genotype distributions were compared with the
Fisher exact test. Multivariate analysis was done to assess the
association between TNF- polymorphism and several variables of
phenotype expression in HHC (age at diagnosis, amount of iron removed,
liver siderosis, HCV and HBV infection, HFE genotype, alanine
aminotransferase [ALT] values, and presence of liver cirrhosis).
Demographic information and HFE gene mutations in patients with HHC Thirty-eight patients (59.4%) were homozygous for the C282Y mutation (C282Y +/+) and 26 (40.6%) were nonhomozygous (non-C282Y +/+). Two were heterozygous for the C282Y mutation, 2 were homozygous and 7 heterozygous for the H63D mutation, and 15 had neither; none had compound heterozygosity. Three non-C282Y +/+ patients had a family history of HHC. Patients homozygous for the C282Y mutation were younger and had more severe iron overload (Table 1). The prevalence of exogenous hepatotoxic factors (alcohol abuse and HBV and HCV infection) was higher in non-C282Y +/+ patients than C282Y +/+ patients, as was reported previously.2 Alcohol abuse was present in 6 of 38 C282Y +/+ patients (16%) and 9 of 26 non-C282Y +/+ patients (35%), HCV infection in 4 of 38 C282Y +/+ patients (11%) and 9 of 26 non-C282Y +/+ patients (35%; P = .03), and HBV infection in 1 of 38 C282Y +/+ patients (2%) and 4 of 26 non-C282Y +/+ patients (15%).
TNF- release in both patients and controls. TNF- release from monocytes from patients with HHC who were nonhomozygous for the C282Y mutation was similar to that from monocytes from controls
(424.01 ± 244.6 ng/L versus 478.75 ± 150.7 ng/L), whereas levels of the cytokine were significantly lower in C282Y homozygous patients (363.4 ± 157.9 ng/L; P = .01; Table
2). A few patients were retested after
reaching iron depletion, and there was no evidence of any significant
difference in TNF- release.
Of the 34 healthy subjects in whom TNF- TNF- release from iron-depleted or
enriched monocytes are shown in Figure 1.
In all subject groups, iron depletion led to a significant increase in
TNF- release compared with the amount released from control cells.
Iron addition led to a decrease in TNF- release from monocytes from
all groups. TNF- release from monocytes from patients with HHC was
lower than that from cells from controls cultured under the same
experimental conditions.
TNF- polymorphism
genotype in healthy controls and patients with HHC is shown in Table 3. In patients with HHC, the prevalence
of the TNF1/TNF2 genotype was 23%, independent of HFE genotype. This
frequency was identical to that in controls. The allele frequency for
TNF1 was 0.84 in HHC patients homozygous for C282Y, 0.92 in HHC
patients with other HFE genotypes, and 0.88 in healthy
controls.
Results regarding the 238 TNF-
Relation between TNF- polymorphism. A
trend toward a lower prevalence of cirrhosis in patients with TNF- polymorphism was observed, although the difference was not significant (4 of 15 patients [26.7%] versus 28 of 49 patients [57.1%];
P = .07). The trend was independent of HFE genotype; in
fact, cirrhosis was present in 2 of 9 C282Y +/+ patients (22%) and 2 of 6 non-C232Y +/+ patients (33%) with TNF- polymorphism and in 15 of 29 C282Y +/+ patients (52%) and 13 of 20 non-C232Y +/+ patients
(65%) without TNF- polymorphism.
Severe liver siderosis (grade IV on Perls staining), which was not
related to TNF- Serum ALT levels were significantly lower in patients with polymorphism
than in those without it (37.5 ± 25 U/L versus 77.2 ± 53 U/L;
P = .006). When the 23 patients with coexistent
hepatotoxic factors (HBV and HCV infections and alcohol abuse) were not
included in the statistical analysis, this difference increased
(P = .004). Logistic regression analysis indicated that
TNF- Relation between TNF- release was measured
had the 308 polymorphism. TNF- release in those with TNF- polymorphism did not differ from that in subjects without it (patients, 422 ± 232 ng/L and 379 ± 224 ng/L; and controls, 420 ± 145
ng/L and 500 ± 115 ng/L, respectively). The difference between
patients and controls without TNF- polymorphism was significant
(P = .01).
In this study, we found that, compared with controls, patients
with HHC had a lower prevalence of the polymorphism at position 238 of
the TNF- Our study was prompted by studies showing that TNF- Alternatively, the decreased TNF- A possible consequence of the reduced TNF- We analyzed the prevalence of 308 and 238 polymorphisms in patients
with HHC and found that the 238 polymorphism, but not the 308 polymorphism, was significantly less prevalent in patients than in
healthy controls. We did not find any relation between TNF- An alternative hypothesis is that the polymorphism makes the phenotype
of patients with HHC milder, possibly as a consequence of the increased
TNF- The milder liver involvement we observed in patients with TNF- In conclusion, our data suggest that TNF-
Submitted October 27, 2000; accepted February 14, 2001.
Supported by MURST 2000, Ricerca Finalizzata IRCCS 1998, and MURST 1999.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Silvia Fargion, Dipartimento di Medicina Interna, Ospedale Maggiore IRCCS, Pad Granelli, Via F Sforza 35, 20122 Milan, Italy; e-mail: silvia.fargion{at}unimi.it.
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© 2001 by The American Society of Hematology.
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K J H Robson, A T Merryweather-Clarke, E Cadet, V Viprakasit, M G Zaahl, J J Pointon, D J Weatherall, and J Rochette Recent advances in understanding haemochromatosis: a transition state J. Med. Genet., October 1, 2004; 41(10): 721 - 730. [Abstract] [Full Text] [PDF]
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L. Giordani, P. Bruzzi, C. Lasalandra, M. Quaranta, F. Schittulli, F. Della Ragione, and A. Iolascon Association of Breast Cancer and Polymorphisms of Interleukin-10 and Tumor Necrosis Factor-{alpha} Genes Clin. Chem., October 1, 2003; 49(10): 1664 - 1667. [Full Text] [PDF]
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F. Wieser, G. Fabjani, C. Tempfer, C. Schneeberger, R. Zeillinger, J. C. Huber, and R. Wenzl Tumor Necrosis Factor-{alpha} Promotor Polymorphisms and Endometriosis Reproductive Sciences, September 1, 2002; 9(5): 313 - 318. [Abstract] [PDF]
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| Copyright © 2001 by American Society of Hematology Online ISSN: 1528-0020 | |||||||||
promoter polymorphisms influence the
phenotypic expression of hereditary hemochromatosis
Top
Abstract
Introduction
one at position 308 (the TNF2
allele)
) and none were C282Y +/+ or had
compound heterozygosity. Monocytes from the 2 C282Y +/
-
T-cell-receptor knockout mice, in which
enteral administration of iron is not followed by the expected increase
in TNF-