MRI evaluation of tissue iron burden in patients with β-thalassaemia major

β-Thalassaemia major is a hereditary anaemia characterized by ineffective erythropoiesis and haemolysis [1]. The underlying mechanism is defective production of haemoglobin β-chains, resulting in excess of α-chains, which are unstable and precipitate to form intracellular inclusion bodies [2, 3]. This excessive intracellular deposition of α-chain material is responsible for accelerated apoptosis of the erythroid precursors and for peripheral haemolysis of the erythrocytes [3]. By the age of 3 months, severe anaemia develops leading to increased intestinal iron absorption. To maintain haemoglobin at a level of 10–12 g/dl, patients suffering from β-thalassaemia major need to be given repeated blood transfusions [1]. A major drawback of this treatment is transfusion siderosis, which, in association with the increased intestinal iron absorption, apoptosis of the erythroid precursors and peripheral haemolysis, leads to iron overload [1].

Iron is ubiquitous in eukaryotic organisms. It is essential for cellular survival and proliferation and for haemoglobin synthesis [4, 5]. Human demands for iron are covered partly by intestinal absorption, but mainly from the recycling of iron from old or abnormal erythrocytes phagocytized by macrophages [6]. Iron released from macrophages binds mainly to transferrin, but also to citrate and albumin to form non-transferrin-bound iron (NTBI) which is a toxic form [7‐9]. Extracellular iron bound to transferrin enters the cell via transferrin receptors by a process of endocytosis. Once iron is released into the cytoplasm, it enters a poorly defined cellular compartment termed the labile iron pool (LIP). Iron in this compartment is loosely bound and therefore is highly toxic [10]. Intracellular iron that is not needed for immediate use is stored in the form of ferritin which consists of an apoprotein storing up to 4,500 atoms of iron (loading factor 4,500) [5, 11], and is not cytotoxic. When ferritin storage capacity is exceeded the LIP increases and haemosiderin is generated from ferritin denaturation [10]. Iron in the form of haemosiderin is thought to be more cytotoxic [10]. The iron in the LIP is in both the ferrous (Fe²⁺) and ferric (Fe³⁺) forms [12]. Fe²⁺ reacts with hydrogen and lipid peroxides and generates highly toxic hydroxyl and lipid radicals (Fenton reaction) that damage cellular membranes, proteins and nucleic acids [4]. Iron overload, just as lack of cellular iron, may lead to cell death and organ dysfunction.

Iron overload is a major cause of morbidity and mortality in β-thalassaemia major [1]. Iron accumulates initially in the reticuloendothelial system (bone marrow, spleen, liver) and then in the hepatocytes, the heart (myocytes) and the endocrine glands [1, 9, 13]. In contrast to the reticuloendothelial cells, the turnover of iron in the hepatocytes, myocytes and endocrine glands is very low [9]. Chelation therapy has been used to eliminate excess iron [1, 7]. Chelatable iron is derived from the catabolism of haemoglobin in macrophages [14]. Chelators remove NTBI from the plasma, but they do not interact with ferritin and haemosiderin at clinically relevant rates [10, 15]. Desferrioxamine (DFO), which is the chelating agent most widely used over the last 30 years, requires parenteral administration. It removes mainly extracellular iron and only a fraction of the intracellular LIP iron [14, 15]. Deferiprone is an oral iron chelator that penetrates the cellular membrane and chelates intracellular species of toxic iron [16]. Cellular uptake of chelators takes place at different rates in different cells [15]. DFO is of low toxicity, mainly affecting the optic, auditory and skeletal systems [7]. Skeletal changes develop mainly due to the toxic effects of DFO on the growth cartilage and are manifested as disproportionate truncal shortening with loss of seated height [7]. Adverse effects of deferiprone are arthralgia, gastrointestinal symptoms, elevated liver enzymes and rarely agranulocytosis [7, 16].

The effective management of patients, and especially of children, with thalassaemia requires optimal monitoring of the toxic effects of both iron overload and excessive chelation therapy. Serum ferritin has been widely used as a surrogate marker and a target ferritin level of 1,000 μg/l is generally recommended [7, 17]. However, serum ferritin represents only 1% of the total iron pool, and as an acute-phase protein it is not specific because the levels can be raised in inflammation (e.g. hepatitis) and liver damage [7, 18, 19]. Chronic liver inflammation is not rare in patients with thalassaemia, since over 40% of them have positive anti-hepatitis C virus (HCV) antibodies and more than 50% have chronic (persistent or active) hepatitis [20, 21]. Liver iron concentration (LIC) measured on needle biopsy is currently considered the gold standard for the evaluation of siderosis [7, 18, 19]. However, needle biopsy is an invasive technique, it is not easily repeatable and the accuracy of the resulting LIC measurement is greatly affected by hepatic inflammation-fibrosis and uneven iron distribution [22]. Furthermore, it appears that cardiac iron overload, which is the leading cause of death in thalassaemia, cannot be predicted from the degree of liver siderosis, probably because of differences in iron kinetics between liver and heart cells [9]. The use of non-invasive techniques for monitoring iron overload in each of the affected organs would be preferable, and to this end MRI has been used increasingly over the last two decades [19, 22‐44]. Other non-invasive methodologies are too complex, too costly and not readily available (i.e. magnetic susceptometry), or lack imaging capability (i.e. magnetic resonance spectroscopy) [45, 46].