A review of select minerals influencing the haematopoietic process

Dalila Cunha Oliveira; Amanda Nogueira-Pedro; Ed Wilson Santos; Araceli Hastreiter; Graziela Batista Silva; Primavera Borelli; Ricardo Ambrósio Fock

doi:10.1017/S0954422418000112

A review of select minerals influencing the haematopoietic process

Published online by Cambridge University Press: 09 July 2018

Dalila Cunha Oliveira ,

Amanda Nogueira-Pedro ,

Ed Wilson Santos ,

Araceli Hastreiter ,

Graziela Batista Silva ,

Primavera Borelli and

Ricardo Ambrósio Fock

Show author details

Dalila Cunha Oliveira: Affiliation:
Experimental Hematology Laboratory, Department of Clinical and Toxicological Analyses, School of Pharmaceutical Sciences, University of Sao Paulo, University City, Sao Paulo, SP 05508-900, Brazil
Amanda Nogueira-Pedro: Affiliation:
Experimental Hematology Laboratory, Department of Clinical and Toxicological Analyses, School of Pharmaceutical Sciences, University of Sao Paulo, University City, Sao Paulo, SP 05508-900, Brazil
Ed Wilson Santos: Affiliation:
Experimental Hematology Laboratory, Department of Clinical and Toxicological Analyses, School of Pharmaceutical Sciences, University of Sao Paulo, University City, Sao Paulo, SP 05508-900, Brazil
Araceli Hastreiter: Affiliation:
Experimental Hematology Laboratory, Department of Clinical and Toxicological Analyses, School of Pharmaceutical Sciences, University of Sao Paulo, University City, Sao Paulo, SP 05508-900, Brazil
Graziela Batista Silva: Affiliation:
Experimental Hematology Laboratory, Department of Clinical and Toxicological Analyses, School of Pharmaceutical Sciences, University of Sao Paulo, University City, Sao Paulo, SP 05508-900, Brazil
Primavera Borelli: Affiliation:
Experimental Hematology Laboratory, Department of Clinical and Toxicological Analyses, School of Pharmaceutical Sciences, University of Sao Paulo, University City, Sao Paulo, SP 05508-900, Brazil
Ricardo Ambrósio Fock*: Affiliation:
Experimental Hematology Laboratory, Department of Clinical and Toxicological Analyses, School of Pharmaceutical Sciences, University of Sao Paulo, University City, Sao Paulo, SP 05508-900, Brazil
*: *Corresponding author: Ricardo Ambrósio Fock, email [email protected]

Article contents

Abstract
Introduction
Iron
Manganese
Calcium
Magnesium
Sodium and potassium
Cobalt
Iodine
Phosphorus
Selenium
Copper
Lithium
Zinc
Conclusion
References

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Abstract

Micronutrients are indispensable for adequate metabolism, such as biochemical function and cell production. The production of blood cells is named haematopoiesis and this process is highly consuming due to the rapid turnover of the haematopoietic system and consequent demand for nutrients. It is well established that micronutrients are relevant to blood cell production, although some of the mechanisms of how micronutrients modulate haematopoiesis remain unknown. The aim of the present review is to summarise the effect of Fe, Mn, Ca, Mg, Na, K, Co, iodine, P, Se, Cu, Li and Zn on haematopoiesis. This review deals specifically with the physiological requirements of selected micronutrients to haematopoiesis, showing various studies related to the physiological requirements, deficiency or excess of these minerals on haematopoiesis. The literature selected includes studies in animal models and human subjects. In circumstances where these minerals have not been studied for a given condition, no information was used. All the selected minerals have an important role in haematopoiesis by influencing the quality and quantity of blood cell production. In addition, it is highly recommended that the established nutrition recommendations for these minerals be followed, because cases of excess or deficient mineral intake can affect the haematopoiesis process.

Keywords

Minerals Trace elements Haematopoiesis Blood cells

Type: Review Article
Information: Nutrition Research Reviews , Volume 31 , Issue 2 , December 2018 , pp. 267 - 280

DOI: https://doi.org/10.1017/S0954422418000112 [Opens in a new window]
Copyright: © The Authors 2018

Introduction

Haematopoiesis is the process of blood cell production. Blood is a tissue with a high renewal rate due to the physiologically short life span of cells in the circulation. The production of these cells is dependent on a highly specialised bone marrow microenvironment, which regulates the quiescence, differentiation and self-renewal of haematopoietic stem cells (HSC)⁽ Reference Nogueira-Pedro, Dos Santos and Oliveira ¹ ^– Reference Borelli, Barros and Nakajima ³ ⁾. HSC have the ability to proliferate and differentiate to produce progenitor lineage cells and consequently mature to form the following cells: leucocytes (which include neutrophils, eosinophils, basophils, lymphocytes and monocytes), erythrocytes and platelets⁽ Reference Mendelson and Frenette ² ⁾. This process has a rapid turnover rate and is highly consuming due to the high demand for nutrients needed for constant blood cell production. Specific nutrients are required in each production phase, from the maintenance of HSC self-renewal until the release of mature cells of each lineage into the bloodstream⁽ Reference Nogueira-Pedro, Dos Santos and Oliveira ¹ ^– Reference Borelli, Barros and Nakajima ³ ⁾.

It is well established that macronutrients such as protein, carbohydrates and lipids are required for successful haematopoiesis as blood cells begin forming in the embryo and continue until the end of life. Nutrient requirements are maintained throughout life due to continual blood cell formation and replacement⁽ Reference Borelli, Barros and Nakajima ³ ^– Reference Xavier, Favero and Vinolo ⁵ ⁾. Micronutrients are also relevant to blood cell production: each mineral will be required in distinct production stages of each blood cell lineage. Micronutrients fulfill roles in the differentiation and proliferation processes intrinsic to the complex haematopoietic process, although some of the mechanisms of how micronutrients modulate haematopoiesis are still poorly known.

Furthermore, intake recommendations⁽ Reference Dennehy and Tsourounis ⁶ ⁾ as well as clinical manifestations, especially with respect to haematopoiesis, in cases of mineral deficiency are usually known. However, in situations where there is increased mineral intake or bioavailability, the effects on haematopoiesis are poorly understood.

The aim of the present review is to highlight the role of the minerals Fe, Ca, Mn, Na, K, Co, iodine, P, Se, Cu, Li and Zn in haematopoiesis, based on data available in the literature and focusing on the effects of these minerals in modulating the haematopoietic process, either positively or negatively. Understanding how micronutrients influence the haematopoietic process is relevant to highlighting the importance of each nutrient in the complex physiology of blood cell production, providing insights regarding the roles of minerals in physiological process such as cell proliferation or in pathologies such as anaemia and leukaemia. The main findings of the present review are compiled in Table 1.

Table 1 Main findings of the effects of minerals on haematopoiesis

ROS, reactive oxygen species; SOD, superoxide dismutase; MEK, MAPK/ERK kinase; MAPK, mitogen-activated protein kinase; ERK, extracellular signal-regulated kinase; TR, thyroid hormone receptor; T₃, triiodothyronine; RXR, retinoid X receptor; RAR, retinoic acid receptor; T₄, tetraiodothyronine; STAT, signal transducer and activator of transcription; CFU, colony-forming unit.

Iron

The first recordings in the literature concerning the presence of Fe in the blood are dated more than one century ago and report the existence of Fe in the liver⁽ Reference Brückmann and Zondek ⁷ ⁾. From the mid-1920s, scientists were engaged in developing a method of measuring the Fe content of different tissues: blood⁽ Reference Schultze and Elvehjem ⁸ ⁾, plasma⁽ Reference Kitzes, Elvehjem and Schuette ⁹ ⁾ and organs⁽ Reference Brückmann and Zondek ⁷ ⁾; in addition, the determination of the Fe content of food was also in progress⁽ Reference Ruegamer, Michaud and Elvehjem ¹⁰ ^, Reference Wrightson ¹¹ ⁾. These decades of studies gave rise to the standards of reference values for Fe and many other inorganic compounds, as well as cellular blood parameters, which are used nowadays in clinical laboratories worldwide⁽ Reference Grotto ¹² ^, ¹³ ⁾. On this basis, the deficiency parameter of Fe characterised by the reduction of total corporeal Fe and the exhaustion of tissue-level stores can be addressed⁽ Reference Cook ¹⁴ ⁾. Fe deficiency leads to the best-known common micronutrient-derived blood disorder: Fe-deficiency anaemia, which affects nearly two billion individuals, of whom children as well as pregnant women and women of child-bearing age are the most affected populations⁽ ¹³ ^, Reference Weiss and Goodnough ¹⁵ ⁾.

Fe is provided by food, and its absorption occurs in the superior jejunum and duodenum via the enterocytes, which can retain Fe bound to ferritin protein in the cytoplasm or deliver it to the plasma for distribution to different tissues in the body in a process mediated by the ferroportin transporter⁽ Reference Shayeghi, Latunde-Dada and Oakhill ¹⁶ ⁾. Macrophages also act as a reservoir of Fe but do so differently from the duodenal mucosal cells: they store Fe from phagocytised senescent erythrocytes⁽ Reference Canavesi, Alfieri and Pelusi ¹⁷ ^, Reference De Domenico, Ward and Musci ¹⁸ ⁾. The placenta is also an important organ for Fe storage during fetal life, when Fe is retained by transferrin receptor 1 (TfR1) present on the apical membrane of syncytiotrophoblasts (and in many other cell types), internalised, and then dissociated and released into the cytoplasm, becoming available for transfer to the fetal circulation⁽ Reference Balesaria, Hanif and Salama ¹⁹ ⁾. Lastly, the hepatocytes represent the major storage site for Fe, displaying high uptake rates for the non-transferrin-bound Fe present when the Fe exceeds the Fe total binding capacity of transferrin⁽ Reference Ganz ²⁰ ^, Reference Takami and Sakaida ²¹ ⁾ (Fig. 1).

Fig. 1 Iron absorption and metabolism. Most of the iron content is incorporated in erythrocyte Hb, and the hepatocytes represent the main site for iron storage.

Erythropoietic tissue is the major user of Fe, as Fe is essential for haeme as well as Hb synthesis by the reticulocytes (maturing erythroblasts); the haeme Fe content of erythrocytes is approximately 1 mg Fe per ml of erythrocytes⁽ Reference Nogueira-Pedro, Dos Santos and Oliveira ¹ ⁾. The reticulocyte Hb content provides an indirect measure of the functional Fe available for new erythrocyte production, and its measurement in peripheral blood is useful for the diagnosis of Fe deficiency in both adults and children⁽ Reference Mast, Blinder and Dietzen ²² ⁾. An imbalance between Hb synthesis and erythroid proliferation results in the production of hypochromic microcytic cells⁽ Reference Srinoun, Svasti and Chumworathayee ²³ ⁾. On the other hand, a lack of the haeme exporter feline leukaemia virus, subgroup C, receptor 1 (FLVCR1) leads to severe macrocytic anaemia⁽ Reference Keel, Doty and Yang ²⁴ ⁾, which is mechanistically determined by the up-regulation of the TfR1⁽ Reference Doty, Phelps and Shadle ²⁵ ⁾.

Fe is also important for the proliferation and differentiation of haematopoietic cells. Upon Fe deprivation, HL-60 (human leukaemia cell line) promonocytes bypass differentiation into macrophages/monocytes and increase apoptosis by a process involving greater than 50 % inhibition of the cyclins A, D3 and E1, cdk2, c-myc, Rb, p21 (WAF1/Cip1), bad, egr-1, FasL and iNOS genes⁽ Reference Alcantara, Kalidas and Baltathakis ²⁶ ⁾. In AML3 promyelocytic leukaemia cells, Fe-chelating therapy induces differentiation in a manner involving modulation of reactive oxygen species and the mitogen-activated protein kinase (MAPK) pathway activation; a similar effect was obtained in an AML patient refractory to chemotherapy, by using Fe-chelating agents and vitamin D₃, resulting in blast differentiation and reversal of pancytopenia⁽ Reference Callens, Coulon and Naudin ²⁷ ⁾. Osteoclast development and Fe homeostasis are also correlated and Fe can act in the proliferation of osteoclast progenitor cells. This involves increasing the levels of transcripts encoding TfR1 and divalent metal transporter 1 and decreasing the levels of transcripts encoding ferroportin⁽ Reference Xie, Lorenz and Dolder ²⁸ ⁾.

A correlation between Fe and lymphocyte proliferation is widely reported in the literature⁽ Reference Djeha, Pérez-Arellano and Brock ²⁹ ^– Reference Seligman, Kovar and Gelfand ³¹ ⁾. Intra- and extra-cellular Fe differentially support the proliferation of lymphocytes, dependent on TfR1 mRNA expression rather than on extracellular Fe availability⁽ Reference Golding and Young ³² ⁾. In addition to TfR1, ferritin is an important component of immune cell function, being involved in binding to T cells, suppression of the delayed-type hypersensitivity to induce allergy, suppression of the production of antibodies by B cells, reduction of the phagocytosis of granulocytes, and regulation of granulomonocytopoiesis. Cytokines (especially TNF-α and IL-1α) induce ferritin gene expression, which in turns requires Fe⁽ Reference Zandman-Goddard and Shoenfeld ³³ ⁾, evidencing the relationship of Fe deficiency with the triggering of several defects in both the humoral and cellular immune response⁽ Reference Bowlus ³⁴ ⁾. However, the pro-proliferative effects of Fe on lymphocytes may be analysed and explored distinctly according to the status of the immune system (for example, homeostasis v. disease/inflammation), taking into consideration, beyond other factors, the poor ability of lymphocytes to sequester excess Fe in ferritin in Fe-overloaded patients⁽ Reference Walker and Walker ³⁵ ⁾.

Much has been described in terms of Fe overload in patients who have received bone marrow transplantation⁽ Reference Ali, Pimentel and Munoz ³⁶ ^– Reference Kim, Kim and Cheong ⁴⁰ ⁾. Fe overload results from multiple erythrocyte transfusions due to the lack of an efficient Fe export system⁽ Reference Kanda, Kawabata and Chao ⁴¹ ⁾. Fe overload may contribute to post-transplant liver toxicity, veno-occlusive disease, infection susceptibility, and graft v. host disease and negatively affect cell survival. In this sense, Fe chelators may represent an alternative option for patients with an inadequate haematological recovery⁽ Reference Pullarkat ⁴² ⁾. It has been shown that Fe overload affects HSC, decreasing both the erythroid and granulocytic colony-forming units (CFU) and the femoral absolute number of HSC LSK⁺ cells, in addition to a diminished long-term and multilineage engraftment capability after transplantation in a process involving the enhancement of oxidative stress, mainly in the HSC LSK⁺ cells, erythroid cells and granulocytic cells⁽ Reference Chai, Li and Cao ⁴³ ⁾. Corroborating this finding, several reports are available in the literature evidencing the detrimental effects of oxidative stress on HSC and the components involved in haematopoiesis⁽ Reference Lu, Zhao and Rajbhandary ³⁸ ^, Reference Tataranni, Agriesti and Mazzoccoli ⁴⁴ ^, Reference Zhang, Zhai and Zhao ⁴⁵ ⁾.

Nitrosative stress is also implicated in this effect. Absence of the antioxidant enzyme haeme oxygenase-1 (HO-1), which catalyses stereospecific degradation of haeme to biliverdin, with release of ferrous Fe and carbon monoxide, disrupts HSC maintenance, reducing its reconstitution capacity⁽ Reference Suda, Takubo and Semenza ⁴⁶ ⁾. However, although oxidative stress triggered by Fe overload results in damage to the normal haematopoietic cells/environment, it can have positive effects on tumoral HSC and progenitor cells of the same origin; this may not be restricted to HSC, as modulation of the haematopoietic system at the level of Fe metabolism also occurs in mature cell populations. The challenge is to achieve an ideal outcome by using Fe chelators or otherwise inducing Fe overload, improving the haematopoietic system and/or haematological disorders without disturbing the homeostasis of the whole organism⁽ Reference Lu, Zhao and Rajbhandary ³⁸ ^, Reference Tataranni, Agriesti and Mazzoccoli ⁴⁴ ^– Reference Suda, Takubo and Semenza ⁴⁶ ⁾.

Manganese

Mn is a mineral with both nutritional relevance and potential toxicity; this ambiguous feature has prompted studies for decades attempting to understand the effects of Mn deficiency and Mn toxicity⁽ Reference Keen, Ensunsa and Watson ⁴⁷ ⁾. Mn functions as a cofactor of multiple enzymes, playing a role in many physiological processes⁽ Reference Furst ⁴⁸ ⁾. Mn is a required cofactor for arginase, superoxide dismutase (Mn-dependent superoxide dismutase (MnSOD; also called SOD2) is critical to preventing cellular oxidative stress), as well as pyruvate carboxylase⁽ Reference Carl and Gallagher ⁴⁹ ^, Reference Keen, Ensunsa and Clegg ⁵⁰ ⁾. Although its toxicity in many different tissues and organs has been described⁽ Reference Crossgrove and Zheng ⁵¹ ⁾, there is no evidence in the literature concerning damage to the haematopoietic system from direct sources, for example, occupational overexposure, dietary supplementation, or intracorporeal administration. However, an indirect effect of Mn through MnSOD has been reported, as the MnSOD enzyme is dependent on Mn availability⁽ Reference Finley and Davis ⁵² ⁾.

In myeloid leukaemic cells from the HL-60 and K562 lineages, MnSOD provides a protective effect against the cytotoxicity driven by TNF stimuli⁽ Reference Kizaki, Sakashita and Karmakar ⁵³ ⁾. MnSOD (SOD2) knockout mice show hypocellular bone marrow associate with a severe anaemia⁽ Reference Lebovitz, Zhang and Vogel ⁵⁴ ⁾. Loss of SOD2 in erythroid progenitor cells leads to increased oxidative damage, change in the membrane deformation capacity and induction of reticulocytosis⁽ Reference Friedman, Rebel and Derby ⁵⁵ ⁾. The same study showed that SOD2 reduction affects the bone marrow stem cells’ ability to reconstitute haematopoiesis in an irradiated recipient mouse and the long-term cell survival of the animal. More recently, Case et al. ⁽ Reference Case, Madsen and Motto ⁵⁶ ⁾ showed that the loss of SOD2 in HSC causes defects in erythrocyte maturation leading to a compensatory extramedullary haematopoiesis involving disrupted Fe homeostasis and increased mitochondrial oxidative stress, which in turns lead to global epigenetic dysregulation, suggesting a link between mitochondrial redox and epigenetic control of nuclear gene regulation.

Calcium

Since 1883 when studies in London with frogs demonstrated that cardiac contraction was dependent on Ca⁽ Reference Moore ⁵⁷ ⁾, many later works have shown the importance of this ion for/in cellular functions. It is fully established that Ca controls various cellular functions, due to the great versatility of responses to this ion. Several proteins are modulated directly or indirectly by the action of Ca, such as kinases, phosphatases and transcription factors⁽ Reference Bootman ⁵⁸ ⁾. Ca acts as a second messenger because of its high concentration in the extracellular medium and organelles and low concentration in the intracellular environment. Responses may be short-lived like cytokine secretion and muscle motility or contraction but may also be long-lasting like gene transcription, division and cell death⁽ Reference Berridge, Bootman and Roderick ⁵⁹ ⁾. The signs of intracellular Ca are always oscillating. Cells utilise various mechanisms to control cytoplasmic Ca levels⁽ Reference Dupont, Combettes and Bird ⁶⁰ ⁾.

Ca is a signalling ion that regulates various systems, such as haematopoiesis. Even though the participation of Ca in haematopoiesis is still not fully understood, it is known that intracellular Ca acts on the signalling of several processes, such as proliferation, differentiation and cell death⁽ Reference Paredes-Gamero, Barbosa and Ferreira ⁶¹ ⁾ (Fig. 2). Cytokine receptors, such as stem cell factor (SCF), erythropoietin (EPO), IL-3, granulocyte macrophage colony-stimulating factor (GM-CSF) and granulocyte colony-stimulating factor (G-CSF) can also be activated by Ca signalling. The binding of GM-CSF and IL-3 to their receptors promotes the dimerisation of these cytokine receptors and elicits the Janus kinase/signal transducer and activator of transcription (JAK/STAT) as well as RAS/RAF/ERK pathways⁽ Reference Paredes-Gamero, Barbosa and Ferreira ⁶¹ ⁾.

Fig. 2 Main effects of calcium deficiency on the haematopoietic system.

Intracellular Ca can also be released by the activation of phospholipase C (PLC) γ2 through cytokines or PLCβ by ATP and analogues, producing inositol 1,4,5-trisphosphate (IP₃) and diacylglycerol (DAG). These second messengers (IP₃ and DAG) act synergistically to cause the phosphorylation of proteins necessary for the processes of proliferation and differentiation of haematopoietic cells. In addition, DAG appears to act by increasing the affinity of protein kinase C for Ca and Ca²⁺/calmodulin-dependent protein kinase II (CaMKII), proteins involved with the proliferation and differentiation of primitive haematopoietic cells⁽ Reference Leon, Barbosa and Justo ⁶² ⁾. The Ca-sensing receptor (CaSR) is critical for retaining HSC near the endosteal region, possibly mediating the association of HSC with collagen type I. It was also observed that HSC detect relatively high levels of Ca (up to 40 mmol/l) through CaSR⁽ Reference Adams, Chabner and Alley ⁶³ ⁾. Upon detecting changes in Ca concentrations, cells promote the release of Ca from the stocks in the endoplasmic reticulum and mitochondria through specific channels to the cytosol or extracellular medium, in order to maintain cellular homeostasis⁽ Reference Pozzan, Rizzuto and Volpe ⁶⁴ ⁾.

Studies in zebrafish have shown that cytokinesis requires intracellular Ca signalling and signal transduction via the calmodulin pathway (CaM)⁽ Reference Webb, Li and Miller ⁶⁵ ⁾. In addition, erythropoiesis requires Ca signalling for nuclear extrusion. The uptake of extracellular Ca is fundamental for the enucleation in the orthochromatic erythroblasts⁽ Reference Wölwer, Pase and Russell ⁶⁶ ⁾. The maturation of erythrocytes is highly impaired with intracellular Ca deficiency. This evidence leads us to believe that a lack of Ca can lead to nutrient-deficiency anaemia⁽ Reference Wölwer, Pase and Russell ⁶⁶ ⁾. Although calcimimetic drugs imitate the action of Ca on the tissues by allosteric activation of the Ca receptor, no direct or indirect beneficial effects of these drugs on anaemia due to chronic disease have been observed⁽ Reference Drueke ⁶⁷ ⁾.

Barbosa et al. ⁽ Reference Barbosa, Bincoletto and Barros ⁶⁸ ⁾ also demonstrated the role of the Ca signalling pathway without myeloid involvement, relating an action of protein kinase C and PLCγ2 with M-CSF and G-CSF-mediated differentiation activated by cytokines. In addition, PLCβ2 is activated by ATP. Both PLCγ and PLCβ induce release of intracellular Ca via IP₃ formation. Increased intracellular Ca induced by G-protein (P2Y)-coupled receptors and ATP-activated ion channels (P2X) is also related to myeloid differentiation⁽ Reference Paredes-Gamero, Leon and Borojevic ⁶⁹ ⁾. ATP induces differentiation of HSC in the myeloid lineage, and this effect is modulated by cytokines such as SCF, IL-3 and GM-CSF⁽ Reference Barbosa, Leon and Nogueira-Pedro ⁷⁰ ⁾.

Understanding the role of Ca in haematopoiesis is fundamental to perceiving the mechanisms of cell proliferation and differentiation as well as changes resulting from deficiencies in this process. Mechanisms of the haematopoietic system are complex, and Ca-dependent mechanisms are still under investigation.

Magnesium

Since 1975, Mg has been considered a key factor in the so-called ‘coordinated growth and metabolism response’, i.e. the up-regulation of energy metabolism and the synthesis of proteins and DNA that precedes cell division⁽ Reference Rubin ⁷¹ ⁾. The large amount of Mg in the intracellular medium reflects its involvement with phospholipids, proteins, nucleic acids and a wide range of biological functions and enzymic reactions⁽ Reference Birch ⁷² ^, Reference Cowan ⁷³ ⁾. Mg is important for cell cycle regulation, particularly at the beginning of DNA synthesis and mitosis, in both micro-organisms and mammals. In addition, it has been reported that cell transformation can cause selective loss of this regulatory function for Mg, implying that Mg is important in oncogenesis⁽ Reference Walker ⁷⁴ ⁾. Mg concentration has a significant positive correlation with the protein synthesis rate, suggesting a key role of Mg in the regulation of protein synthesis and in the cell proliferation rate in normal tissue cell populations⁽ Reference Cameron and Smith ⁷⁵ ⁾.

Studies with interferon-α and ATP stimuli demonstrate a correlation with Ca metabolism, promoting signalling that activates phospholipase A (PLA) by inducing arachidonic acid release from the cell membrane. The prostaglandins produced by arachidonic acid through cyclo-oxygenase stimulate adenyl cyclase, which synthesises cAMP. Intracellular Mg may influence adenyl cyclase, down-regulating the same efflux of Mg. Modulation of cellular Mg homeostasis parallels the molecular control of cell proliferation, differentiation and death⁽ Reference Wolf and Cittadini ⁷⁶ ⁾.

The physiological process of haematopoiesis has a characteristic high turnover, so it is expected that the demand for Mg is high. Mg deficiency may promote defects in platelet biogenesis due to changes in the cytoskeleton, promoting changes in platelet function. In addition, changes in the transient receptor potential melastatin 7 ion channels (TRPM7) may cause macrothrombocytopenia in human subjects and in mice⁽ Reference Stritt, Nurden and Favier ⁷⁷ ⁾. Rats fed with a diet deficient in Mg show decreased erythrocyte numbers in addition to reduced erythrocyte survival and erythrocyte membrane defects and become anaemic⁽ Reference Elin, Utter and Tan ⁷⁸ ⁾ (Fig. 3). Mg and K administration promotes accelerated restoration of spleen erythropoiesis in irradiated rats⁽ Reference Fedorocko, Macková and Sándorcínová ⁷⁹ ⁾. However, the pathological processes that cause these changes are unknown. Few studies have correlated Mg with haematopoiesis. Research showing this relationship should be encouraged to better understand the mechanisms involved in the regulation of important cellular functions, such as cell proliferation and differentiation.

Fig. 3 Main effects of magnesium deficiency on the haematopoietic system.

Sodium and potassium

Homeostatic regulation is critical for all cellular functions, primarily for cell viability. The electrochemical Na and K gradient is crucial for ionic homeostasis and is regulated by the trans-membrane protein Na⁺K⁺-ATPase⁽ Reference Lang ⁸⁰ ^, Reference Singh, Pandey and Rizvi ⁸¹ ⁾. Erythrocyte maturation is linked to changes in cell volume, regulated by pump Na⁺K⁺-ATPase and K⁺Cl^– co-transport. The enhanced activity of the Na/K pump is observed in reticulocytes and decreases during cell maturation⁽ Reference Blostein, Drapeau and Benderoff ⁸² ^, Reference Lauf and Mangor-Jensen ⁸³ ⁾. Reticulocytes are characterised by higher cellular volume due to enhanced K turnover, which is increased approximately 3-fold compared with that of mature cells⁽ Reference Brugnara and Tosteson ⁸⁴ ^– Reference Furukawa, Bilezikian and Loeb ⁸⁶ ⁾. During maturation and ageing, the loss of cellular K⁺ by K⁺Cl^– cotransport decreases reticulocyte and erythrocyte volume⁽ Reference Kosower ⁸⁷ ⁾. One of the reasons for increased Na/K pump activity might be a functional demand to keep pace with augmented Na leak⁽ Reference Mairbäurl, Schulz and Hoffman ⁸⁸ ⁾.

K is important for erythroid colony formation and maintenance of self-renewal of erythroid stem cells and their differentiation in vitro ⁽ Reference Gallicchio and Murphy ⁸⁹ ^, Reference Gallicchio and Murphy ⁹⁰ ⁾. In Friend erythroleukaemia cells, a widely used model of murine erythropoiesis, exposure to high K and low Na levels is capable of completing erythroid differentiation, suggesting that cell maturation involves a selective change in K permeability⁽ Reference Mager, MacDonald and Bernstein ⁹¹ ⁾. K inward rectifier channels are essential for the development of CD34⁺/CD38^– primitive haematopoietic cells⁽ Reference Shirihai, Merchav and Attali ⁹² ^, Reference Shirihai, Attali and Dagan ⁹³ ⁾. Because these channels are not detected in most mature haematopoietic cells, their transient expression in primitive cells suggests that their role is in the early stages of HSC differentiation⁽ Reference Banati, Hoppe and Gottmann ⁹⁴ ^, Reference Kettenmann, Hoppe and Gottmann ⁹⁵ ⁾. The differentiation of some leukaemic myeloid lineage cells is also correlated with K channels. Promyelocytic HL-60 cells present a slow-inactivated K channel⁽ Reference Wieland, Chou and Chen ⁹⁶ ⁾, and promonocytic U-937 cells exhibit abnormal conductance in K channels⁽ Reference McCann, Keller and Guyre ⁹⁷ ⁾. On the other hand, in myeloid ML-1 cells, K current is suppressed during cell differentiation⁽ Reference Lu, Yang and Markakis ⁹⁸ ⁾. Few studies have correlated Na and K with haematopoietic differentiation. Understanding the signals involved in this regulation can lead us to elucidate molecular mechanisms and develop novel strategies to control haematological disorders.

Cobalt

Co is a metal with chemical properties similar to Fe and Ni⁽ ⁹⁹ ⁾. Metal ions perform a wide role in natural proteins, including nucleophilic catalysis, electron transfer as well as the stabilisation of protein structure⁽ ⁹⁹ ^, Reference Kobayashi and Shimizu ¹⁰⁰ ⁾. Co is a fundamental component in the tetrapyrrole ring of hydroxocobalamin (vitamin B₁₂), which is an essential coenzyme of cell mitosis, acting on the synthesis of methionine and metabolism of folates and purines⁽ Reference Banerjee ¹⁰¹ ^– Reference Varela-Moreiras, Murphy and Scott ¹⁰⁴ ⁾. Under conditions of hydroxocobalamin deficiency, haematopoiesis is widely affected and erythropoiesis turns ineffective because erythrocytic progenitors cannot mature adequately. This has implications for the development of megaloblastic anaemia and hypofunction of erythrocytic cells⁽ Reference Andrès, Affenberger and Zimmer ¹⁰⁵ ^, Reference Koury and Ponka ¹⁰⁶ ⁾. However, Co does not only participate in haematopoiesis via hydroxocobalamin but also acts in inorganic forms (Co²⁺), usually CoCl₂ or CoSO₄. In 1929, Waltner & Waltner⁽ Reference Waltner and Waltner ¹⁰⁷ ⁾ showed that Co stimulates erythropoiesis and induces polycythaemia in animal models. Weissbecker⁽ Reference Weissbecker ¹⁰⁸ ⁾ related increases in reticulocytes, erythrocytes, and Hb, as well as bone marrow erythroid hyperplasia, in oral administration of Co salts. In addition, Co induces EPO and blocks iodine uptake by the thyroid⁽ Reference Barceloux ¹⁰² ⁾.

Co is considered one of the most reliable and potent stimulators of erythrocyte production⁽ Reference Thorling and Erslev ¹⁰⁹ ⁾. Co enhances erythropoiesis by indirect activation of EPO gene expression. Co binds to hypoxia-inducible transcription factors (HIF), and this association inhibits the proteasomal degradation of HIF by von Hippel–Lindau (pVHL) proteins. The accumulation of HIF promotes the dimerisation of HIF-2α and HIF-1β subunits in the nucleus and powerfully activates EPO expression⁽ Reference Jelkmann ¹¹⁰ ⁾.

Co has been used extensively since the late 1970s in the treatment of several types of anaemia in children and adults, as well as in anaemia of chronic renal disease⁽ Reference Berk, Burchenaj and Castlew ¹¹¹ ^, Reference Gardnerf ¹¹² ⁾. However, soluble Co salts are toxic to the human body, and because of the side effects associated with chronic Co use, Co is rarely used nowadays, since the administration of Co is shown to induce DNA damage and promote the development of carcinomas⁽ Reference Duckham and Lee ¹¹³ ^– ¹¹⁵ ⁾.

Iodine

Iodine is a vital micronutrient required at all stages of life, promoting general growth and development within the body as well as aiding in metabolism. In addition, iodine is an essential constituent of the thyroid thyroxine hormones (tetraiodothyronine (T₄) and triiodothyronine (T₃))⁽ Reference Niwattisaiwong, Burman and Li-ng ¹¹⁶ ⁾. Iodine acts indirectly on haematopoiesis, through thyroid hormones and prohormones, which are the only known iodine-containing compounds with biological activity. The thyroid gland produces T₄ and T₃, which are largely known to control metabolism, with emphasis on renal and cardiac function. Furthermore, thyroid hormones handle carbohydrate and fat metabolism, protein synthesis and fetal neurodevelopment⁽ Reference Brent ¹¹⁷ ^, Reference Mondal, Raja and Schweizer ¹¹⁸ ⁾.

At the cellular level, thyroid hormones undergo several metabolic reactions by different cytosolic enzymes and play a role in a variety of cellular pathways and functions, comprising insulin signalling, apoptosis, the cell cycle and proliferation⁽ Reference Flores-Morales, Gullberg and Fernandez ¹¹⁹ ^– Reference Wu, Green and Huang ¹²² ⁾. Kocher⁽ Reference Kocher ¹²³ ⁾ first described the haematological findings of thyroid abnormalities, which showed that hyperthyroidism patients presented leucopenia, relative lymphocytosis and neutropenia. Since then, several studies have correlated thyroid diseases and haematopoiesis, but this relationship is complex and some studies are inconclusive or present important limitations.

Thyroid hormones classically stimulate erythropoiesis by increasing the oxygen demand on the kidneys and stimulating EPO production⁽ Reference Evans, Rosenberg and Simpson ¹²⁴ ⁾ (Fig. 4). That is why normocytic normochromic anaemia is associated with hypothyroidism, and hyperthyroidism frequently coincides with erythrocytosis and erythroid hyperplasia on bone marrow⁽ Reference Tudhope and Wilson ¹²⁵ ^, Reference Wu and Koenig ¹²⁶ ⁾. It was unclear if thyroid hormones acted exclusively by way of EPO or could also act on haematopoietic progenitor cells until Golde et al. ⁽ Reference Golde, Bersch and Chopra ¹²⁷ ⁾ demonstrated that T₃ and T₄ directly stimulate mice erythroid colony formation in vitro. Thereafter, the expression and activity of thyroid hormone receptors (TR) were reported in mature bone marrow cells in both rats and mice⁽ Reference Gruber, Czerwenka and Wolf ¹²⁸ ^, Reference Milne, Kang and Cardona ¹²⁹ ⁾.

Fig. 4 Iodine is an essential constituent of the thyroid thyroxine hormones. Thyroid hormones classically stimulate erythropoiesis by increasing the oxygen demand on the kidneys and stimulating erythropoietin production. T₃, triiodothyronine; T₄, tetraiodothyronine; TR, thyroid hormone receptor.

In humans, TRα1 and TRα2 are important for fate determination in haematopoietic progenitors. TRα1 and TRα2 receptors are expressed on CD34⁺ haematopoietic cells and regulate apoptosis and cell growth⁽ Reference Grymuła, Paczkowska and Dziedziejko ¹³⁰ ^, Reference Kawa, Grymula and Paczkowska ¹³¹ ⁾. In erythroblasts, the activation of these receptors induces proliferation and accelerates cell differentiation⁽ Reference Bauer, Mikulits and Lagger ¹³² ⁾ (Fig. 4). The mechanisms by which thyroid hormones regulate haematopoiesis in vivo are not fully understood. Novel insights into the interactions between T₃ and T₄ and the classical haematopoietic inductors are required, so we can develop ways of intervening in both haematological and thyroid disorders.

Phosphorus

P plays a major role in physiological functions, including energy production, cellular replication and bone mineral metabolism⁽ Reference Tran, Batech and Rhee ¹³³ ⁾. It is well established that rapid cell synthesis and turnover may be associated with high phosphate consumption. Low levels of phosphate leading to hypophosphataemia are associated after bone marrow transplantation⁽ Reference Raanani, Levi and Holzman ¹³⁴ ^, Reference Uçkan, Cetin and Dida ¹³⁵ ⁾. Although different research groups affirm the correlation between hypophosphataemia in bone marrow or stem cell transplantation, there are few data available in the literature offering a concise explanation of how the decreased level of phosphates can affect haematopoiesis.

Raanani et al. ⁽ Reference Raanani, Levi and Holzman ¹³⁴ ⁾ emphasised that the release of cytokines, such as IL-6 and IL-8, is commonly associated with the development of hypophosphataemia observed in HSC transplant. The explanation for the hypophosphataemia observed was that it was due to phosphate consumption by proliferating cells after bone marrow HSC transplantation in human subjects⁽ Reference Raanani, Levi and Holzman ¹³⁴ ^– Reference Crook, Swaminathan and Schey ¹³⁷ ⁾. Increased P levels can be harmful to the haematopoietic process. Recent studies state that higher P serum levels increase the likelihood of anaemia. EPO deficiency, inflammation and oxidative stress have been implicated as potential factors associating hyperphosphataemia and anaemia. The possible mechanisms linking hyperphosphataemia and anaemia were described in 2011 by Kovesdy et al. ⁽ Reference Kovesdy, Mucsi and Czira ¹³⁸ ⁾, who suggested that high serum P may lead to a higher production of polyamines, which can function as uraemic toxins inhibiting erythropoiesis⁽ Reference Kovesdy, Mucsi and Czira ¹³⁸ ^, Reference Wojcicki ¹³⁹ ⁾.

Another possible mechanism is that high serum P leads to vascular calcification within renal arteries, which may eventually result in EPO deficiency and anaemia⁽ Reference Tran, Batech and Rhee ¹³³ ^, Reference Kuroo ¹⁴⁰ ⁾. All these results highlight that increased levels of P can modulate haematopoietic functions. However, there is a lack of data in the literature clearly explaining how hyperphosphataemia affects the production of erythrocytes. Low dietary intake, decreased absorption or increased urinary phosphate excretion and shifts of phosphate from the extracellular into the intracellular fluid are conditions known to induce moderate hypophosphataemia⁽ Reference Raanani, Levi and Holzman ¹³⁴ ⁾.

Selenium

Se is a chemical element and can be determined in blood, plasma or serum, and by assaying the activity of the selenoprotein glutathione peroxidase (GPx) in whole blood or platelets⁽ Reference Navarro-Alarcon and Cabrera-Vique ¹⁴¹ ^, Reference Tinggi ¹⁴² ⁾. Se is a trace element that exerts crucial effects on erythropoiesis. The cells that exhibit higher Se consumption are those of the haematopoietic system, such as immune cells, erythrocytes and platelets⁽ Reference Navarro-Alarcon and Cabrera-Vique ¹⁴¹ ⁾ Se is an important component of GPx, which assists in intracellular defence mechanisms against oxidative damage by preventing the production of reactive oxygen species. It is known that Se is not restricted to its antioxidant function but is also involved in multiple other aspects of human metabolism⁽ Reference Tinggi ¹⁴² ^, Reference Puspitasari, Abdulah and Yamazaki ¹⁴³ ⁾.

Haematopoiesis is characterised by tight control of cell expansion, with differentiation and maintenance of progenitors. These processes expose the cells to oxidative stress, and this could possibly affect erythropoiesis because Hb is prone to oxidative damage⁽ Reference Kaushal, Hegde and Lumadue ¹⁴⁴ ⁾. Se functions as an antioxidant through selenoproteins, preventing erythrocyte lysis. Alterations in the physiological levels of Se are usually linked with numerous pathological conditions, associated with oxidative stress⁽ Reference Navarro-Alarcon and Cabrera-Vique ¹⁴¹ ^, Reference Tinggi ¹⁴² ^, Reference Kaushal, Hegde and Lumadue ¹⁴⁴ ⁾. Se deficiency is associated with increased denaturation of Hb as well as increased methaemoglobin content, protein carbonyls, lipid peroxidation, Heinz bodies and increased erythrocyte osmotic fragility⁽ Reference Kaushal, Hegde and Lumadue ¹⁴⁴ ⁾.

Forkhead transcription factor (FoxO3a) is one of the most expressed protein in erythroid cells and is essential for the maintenance of the HSC pool. Se status is important in erythrocyte homeostasis by modulating FoxO3a localisation, which is pivotal for mitigating oxidative stress in erythroid cells⁽ Reference Kaushal, Hegde and Lumadue ¹⁴⁴ ⁾. Erythrocyte Se concentration is correlated with hospital mortality in septic shock patients. In addition, erythrocyte Se concentrations can be a predictor of mortality in patients with septic shock⁽ Reference Puspitasari, Abdulah and Yamazaki ¹⁴³ ^, Reference Costa, Gut and Pimentel ¹⁴⁵ ⁾.

Gandhi et al. ⁽ Reference Gandhi, Kaushal and Hegde ¹⁴⁶ ⁾ demonstrated that Se-dependent modulation of arachidonic acid metabolism can trigger apoptosis of primary leukaemic cells. The pro-apoptotic effects of Se were, in part, related to exacerbated oxidative stress in leukaemia stem cells that involved NADPH oxidases, particularly Nox1. In contrast, Se treatment did not affect normal HSC, suggesting that leukaemic cells are uniquely sensitive to changes in intracellular reactive oxygen species⁽ Reference Gandhi, Kaushal and Hegde ¹⁴⁶ ⁾.

Although environmental toxicity of Se in humans is rare, clinical signs such as hypochromic anaemia, leukopoenia, damaged nails, and others have been found in long-term workers who manufacture Se rectifiers⁽ Reference Navarro-Alarcon and Cabrera-Vique ¹⁴¹ ^, Reference Tinggi ¹⁴² ^, Reference Rosenfeld and Beath ¹⁴⁷ ⁾. Many researchers have shown that Se supplementation provides positive effects on the general cellular condition. Se plays crucial roles in the physiology of blood formation and pathologies such as cancer; however, the mechanism of action has yet to be unveiled⁽ Reference Puspitasari, Abdulah and Yamazaki ¹⁴³ ⁾.

Copper

Cu is an important mineral in body metabolism, largely because it allows many critical enzymes, such as cytochrome C oxidase, superoxide dismutase, tyrosinase, peptidylglycine α-amidating mono-oxygenase, and lysyl oxidase, to function properly⁽ Reference Grubman and White ¹⁴⁸ ^, Reference Huang, Pierce and Cobine ¹⁴⁹ ⁾. Cu is essential for normal haematopoiesis, and common features of Cu deficiency include anaemia, leucopenia and neutropenia⁽ Reference Huang, Pierce and Cobine ¹⁴⁹ ⁾ (Fig. 5). The involvement of Cu in haematopoiesis is also inferred from inherited or acquired Cu deficiency due to genetic mutations or malnourishment, respectively, which causes neutropenia, anaemia and thrombocytopenia due to arrested differentiation at the haematopoietic progenitor cell level⁽ Reference Williams ¹⁵⁰ ⁾. However, nutritional Cu deficiency is extremely rare and occurs in newborns, usually premature, undergoing rapid growth on a diet poor in Cu or in patients receiving parenteral nutrition for long periods of time without Cu supplementation. Although it is rare, Cu deficiency causes hypochromic anaemia unresponsive to Fe supplementation⁽ Reference Choi and Kim ¹⁵¹ ^, Reference Bustos, Jensen and Ruiz ¹⁵² ⁾. Cu is essential for normal haematopoiesis; however, the effects of fine-tuning of intracellular Cu content on the regulation of self-renewal and differentiation of HSC and progenitor cells are unknown⁽ Reference Bae and Percival ¹⁵³ ^, Reference Zhou, Zhang and Ren ¹⁵⁴ ⁾.

Fig. 5 Main effects of copper deficiency on the haematopoietic system.

Studies with HSC and haematopoietic progenitor cells cultured with the Cu chelator tetraethylenepentamine (TEPA) have suggested that reducing the cellular Cu content with TEPA results in preferential expansion of HSC activity in contrast to arrested differentiation, directly affecting blood cell populations⁽ Reference Huang, Pierce and Cobine ¹⁴⁹ ⁾. In addition, several mechanisms have been proposed for the role of Cu in Fe metabolism and erythropoiesis. Cu is required for the formation of erythrocytes, as Cu deficiency results in anaemia, possibly due to chronic ingestion of high amounts of Zn, which impairs Cu absorption⁽ Reference Zhou, Zhang and Ren ¹⁵⁴ ⁾. The literature also shows that serum Cu concentrations have an important relationship with blood leucocyte counts and serum Fe parameters. Studies have shown that the addition of Cu increases retinoic acid-induced differentiation of the HL-60 cell line⁽ Reference Huang, Pierce and Cobine ¹⁴⁹ ^, Reference Bae and Percival ¹⁵³ ⁾.

Lithium

Li is a mineral that can modulate the haematopoietic process directly⁽ Reference Boggs and Joyce ¹⁵⁵ ⁾. Studies have shown that ingestion of Li increases the production of neutrophil granulocytes, showing that nanomolar levels of Li can stimulate clonal proliferation of granulocyte precursors⁽ Reference Boggs and Joyce ¹⁵⁵ ^– Reference McGrath, Liang and Alberico ¹⁵⁸ ⁾. The effects of Li on haematopoiesis are not cell-lineage specific. In vitro studies have shown that Li enhances colony formation (CFU) of the erythrocyte precursor (CFU-E), the megakaryocyte precursor (CFU-Meg) and the granulocyte macrophage precursor (GM-CFU)⁽ Reference McGrath, Wade and Kister ¹⁵⁷ ^, Reference McGrath, Liang and Alberico ¹⁵⁸ ⁾. Patients treated with Li for manic–depressive illnesses usually develop leucocytosis with increases in peripherical neutrophils and eosinophils and, commonly, monocytes and platelets also tend to be increased; however, lymphocytes and erythrocytes are usually unaffected⁽ Reference Hager, Dziambor and Winkler ¹⁵⁹ ^, Reference Gallicchio and Chen ¹⁶⁰ ⁾.

In addition, a CFU assay performed with bone marrow cells has shown a higher capacity for the formation of CFU⁽ Reference Gallicchio and Chen ¹⁶⁰ ⁾. Additionally, mice infected with LP-BM5 murine leukaemia virus (MuLV) and treated with Li showed increased neutrophils and eosinophils in the peripheral blood; moreover, haematopoietic progenitor cells collected from the bone marrow and spleens of these animals showed increased GM-CFU formation⁽ Reference Gallicchio, Hughes and Tse ¹⁶¹ ⁾. However, high doses of lithium carbonate (greater than 5 mm) can have opposite effects leading to a reduction of the granulocytes in peripheral blood and lower formation of CFU⁽ Reference Gallicchio and Chen ¹⁶⁰ ^, Reference Walasek, Bystrykh and van den Boom ¹⁶² ⁾.

Zinc

Zn is required in the structure and activity of more than 300 enzymes including DNA polymerase, Cu–Zn superoxide dismutase, alkaline phosphatase, alcohol dehydrogenase, carbonic anhydrase and protein chain elongation factor⁽ Reference Vallee and Falchuk ¹⁶³ ⁾. This mineral is used in nucleic acid and protein synthesis, cell differentiation and replication, non-glucose metabolism and insulin secretion. The Zn requirement of numerous proteins makes it is essential for growth, tissue maintenance and wound healing. Proper Zn intake is critical for the integration of many tissues and systems, such as gastrointestinal, muscular, immune, reproductive and behavioural, as well as involved in the wound-healing process⁽ Reference Berg ¹⁶⁴ ^– Reference Murakami, Whiteley and Routtenberg ¹⁶⁶ ⁾.

Zn can act as a signal to induce erythropoiesis in a dose-dependent manner⁽ Reference Chen, Shiu and Ho ¹⁶⁷ ⁾. In addition, serum Zn levels have a negative effect on anaemia by blocking the utilisation of Fe of anaemic patients⁽ Reference Chirulescu, Suciu and Tănăsescu ¹⁶⁸ ⁾. It should be noted that chronic Zn infusion can induce Cu deficiency and sideroblastic anaemia, decreased plasma caeruloplasmin and microcytic anaemia⁽ Reference Livingstone ¹⁶⁹ ⁾.

On the other hand, Zn deficiency occurs in a wide range of pathologies, including haemolytic anaemias such as thalassemias and sickle cell anaemia. Zn deficiency exerts its most profound effects on rapidly proliferating tissues. Severe deficiency is usually accompanied by growth arrest, teratogenicity, hypogonadism and infertility, and commonly but not exclusively with impairment of cellular immunity⁽ Reference Livingstone ¹⁶⁹ ⁾. Substantial depletion usually occurs in cells of the erythroid and lymphoid lineages, and evaluating the phenotypic distribution of cells of the B-lineage it has been shown that Zn deficiency alters the composition as well as the phenotypic distribution of the remaining cells of the B-lineage. Zn deficiency also reduces immature or IgM-bearing B-cells, whereas the earliest B-cell progenitors are somewhat resistant to the deficiency. In addition, the ratio CD4/CD8 in the thymus is affected⁽ Reference King, Osati-Ashtiani and Fraker ¹⁷⁰ ^, Reference Fraker and King ¹⁷¹ ⁾. However, myelopoiesis is not disrupted in Zn deficiency, as shown by the expansion of all myeloid populations in the bone marrow of Zn-deficient patients⁽ Reference Fraker and King ¹⁷¹ ^, Reference Cook-Mills and Fraker ¹⁷² ⁾. Zn deficiency has been reported in patients undergoing intensive therapy with desferrioxamine, an Fe chelator that aims to reduce or stabilise non-body Fe accumulation, and in patients with decreased renal reabsorption of trace minerals.

Conclusion

Minerals are mandatory for the development of effective haematopoiesis, and the absence of these elements can have a deep impact on blood cell formation and/or blood cell functions. In contrast, mineral excess can also be harmful, although the majority of the complete mechanisms that can be disrupted by an excess of minerals are poorly understood. It is crucial to assess whether minerals can interfere to correct haematopoietic functions, providing better therapeutic care in several nutritional and haematopoietic diseases. More research is required to provide data unveiling the roles of minerals in diverse aspects of haematopoiesis.

Acknowledgements

The present review was financially supported by the Fundação de Amparo a Pesquisa do Estado de São Paulo (FAPESP 2016/16463-8).

Each author participated actively in the work and gave a substantial contribution. Each author read and approved the final submitted manuscript. D. C. O. wrote the sections about P and Se and helped to conduct the bibliographic research. A. N.-P. wrote the sections about Fe and Mn and reviewed and helped draft the manuscript. E. W. S. wrote the sections about Ca and Mg; A. H. wrote the sections about Na, K, Co and iodine. G. B. S. wrote the sections about Cu, Li and Zn. P. B. helped to conduct the bibliographic research and interpret the data and helped to write the manuscript. R. A. F. supervised, helped to write the manuscript, reviewed and contributed to the drafting of the manuscript.

The authors have no conflicts of interest to declare.

References

1. Nogueira-Pedro, A, Dos Santos, GG, Oliveira, DC, et al. (2016) Erythropoiesis in vertebrates: from ontogeny to clinical relevance. Front Biosci 8, 100–112.Google Scholar

2. Mendelson, A & Frenette, PS (2014) Hematopoietic stem cell niche maintenance during homeostasis and regeneration. Nature Med 20, 833–846.Google Scholar

3. Borelli, P, Barros, FEV, Nakajima, K, et al. (2009) Protein–energy malnutrition halts hemopoietic progenitor cells in the G0/G1 cell cycle stage, thereby altering cell production rates. Braz J Med Biol Res 42, 523–530.Google Scholar

4. Cunha, MCR, Lima, FS, Vimolo, MAR, et al. (2013) Protein malnutrition induces bone marrow mesenchymal stem cells commitment to adipogenic differentiation leading to hematopoietic failure. PLOS ONE 8, e58872.Google Scholar

5. Xavier, JG, Favero, ME, Vinolo, MAR, et al. (2007) Protein–energy malnutrition alters histological and ultrastructural characteristics of the bone marrow and decreases haematopoiesis in adult mice. Histol Histopathol 22, 651–660.Google Scholar

6. Dennehy, C & Tsourounis, C (2010) A review of select vitamins and minerals used by postmenopausal women. Maturitas 66, 370–380.Google Scholar

7. Brückmann, G & Zondek, SG (1939) Iron, copper and manganese in human organs at various ages. Biochem J 33, 1845–1857.Google Scholar

8. Schultze, MO & Elvehjem, CA (1934) An improved method for the determination of hemoglobin in chicken blood. J Biol Chem 105, 253–257.Google Scholar

9. Kitzes, G, Elvehjem, CA & Schuette, HA (1944) Determination of blood plasma iron. J Biol Chem 155, 653–660.Google Scholar

10. Ruegamer, WR, Michaud, L & Elvehjem, CA (1945) A simplified method for the determination of iron in milk. J Biol Chem 158, 573–576.Google Scholar

11. Wrightson, FM (1949) Determination of traces of iron, nickel, and vanadium in petroleum oils. Anal Chem 21, 1543–1545.Google Scholar

12. Grotto, HZW (2009) Interpretação Clínica do Hemograma (Clinical Interpretation of Blood Counts), Série Clínica Médica Ciência e Arte (Medical Clinic Series Science and Arts), 1st ed. São Paulo: Atheneu.Google Scholar

13. World Health Organization (2001) Iron Deficiency Anaemia: Assessment, Prevention and Control, A Guide for Programme Managers. Geneva: WHO.Google Scholar

14. Cook, JD (2005) Diagnosis and management of iron-deficiency anaemia. Best Pract Res Clin Haematol 18, 319–332.Google Scholar

15. Weiss, G & Goodnough, LT (2005) Anemia of chronic disease. N Engl J Med 352, 1011–1023.Google Scholar

16. Shayeghi, M, Latunde-Dada, GO, Oakhill, JS, et al. (2005) Identification of an intestinal heme transporter. Cell 122, 789–801.Google Scholar

17. Canavesi, E, Alfieri, C, Pelusi, S, et al. (2012) Hepcidin and HFE protein: iron metabolism as a target for the anemia of chronic kidney disease. World J Nephrol 1, 166–176.Google Scholar

18. De Domenico, I, Ward, DM, Musci, G, et al. (2007) Evidence for the multimeric structure of ferroportin. Blood 109, 2205–2209.Google Scholar

19. Balesaria, S, Hanif, R, Salama, MF, et al. (2012) Fetal iron levels are regulated by maternal and fetal Hfe genotype and dietary iron. Haematologica 97, 661–669.Google Scholar

20. Ganz, T (2007) Molecular control of iron transport. J Am Soc Nephrol 18, 394–400.Google Scholar

21. Takami, T & Sakaida, I (2011) Iron regulation by hepatocytes and free radicals. J Clin Biochem Nutr 48, 103–106.Google Scholar

22. Mast, AE, Blinder, MA & Dietzen, DJ (2008) Reticulocyte hemoglobin content. Am J Hematol 83, 307–310.Google Scholar

23. Srinoun, K, Svasti, S, Chumworathayee, W, et al. (2009) Imbalanced globin chain synthesis determines erythroid cell pathology in thalassemic mice. Haematologica 94, 1211–1219.Google Scholar

24. Keel, SB, Doty, RT, Yang, Z, et al. (2008) A heme export protein is required for red blood cell differentiation and iron homeostasis. Science 319, 825–828.Google Scholar

25. Doty, RT, Phelps, SR, Shadle, C, et al. (2015) Coordinate expression of heme and globin is essential for effective erythropoiesis. J Clin Invest 125, 4681–4691.Google Scholar

26. Alcantara, O, Kalidas, M, Baltathakis, I, et al. (2001) Expression of multiple genes regulating cell cycle and apoptosis in differentiating hematopoietic cells is dependent on iron. Exp Hematol 29, 1060–1069.Google Scholar

27. Callens, C, Coulon, S, Naudin, J, et al. (2010) Targeting iron homeostasis induces cellular differentiation and synergizes with differentiating agents in acute myeloid leukemia. J Exp Med 207, 731–750.Google Scholar

28. Xie, W, Lorenz, S, Dolder, S, et al. (2016) Extracellular iron is a modulator of the differentiation of osteoclast lineage cells. Calcif Tissue Int 98, 275–283.Google Scholar

29. Djeha, A, Pérez-Arellano, JL, Brock, JH, et al. (1993) Transferrin synthesis by mouse lymph node and peritoneal macrophages: iron content and effect on lymphocyte proliferation. Blood 81, 1046–1050.Google Scholar

30. Kinik, ST, Tuncer, AM & Altay, C (1999) Transferrin receptor on peripheral blood lymphocytes in iron deficiency anaemia. Br J Haematol 104, 494–498.Google Scholar

31. Seligman, PA, Kovar, J & Gelfand, EW (1992) Lymphocyte proliferation is controlled by both iron availability and regulation of iron uptake pathways. Pathobiology 60, 19–26.Google Scholar

32. Golding, S & Young, SP (1995) Iron requirements of human lymphocytes: relative contributions of intra- and extra-cellular iron. Scand J Immunol 41, 229–236.Google Scholar

33. Zandman-Goddard, G & Shoenfeld, Y (2008) Hyperferritinemia in autoimmunity. Isr Med Assoc J 10, 83–84.Google Scholar

34. Bowlus, CL (2003) The role of iron in T cell development and autoimmunity. Autoimmun Rev 2, 73–78.Google Scholar

35. Walker, EM Jr & Walker, SM (2000) Effects of iron overload on the immune system. Ann Clin Lab Sci 30, 354–365.Google Scholar

36. Ali, S, Pimentel, JD, Munoz, J, et al. (2012) Iron overload in allogeneic hematopoietic stem cell transplant recipients. Arch Pathol Lab Med 136, 532–538.Google Scholar

37. Trottier, BJ, Burns, LJ, DeFor, TE, et al. (2013) Association of iron overload with allogeneic hematopoietic cell transplantation outcomes: a prospective cohort study using R2-MRI-measured liver iron content. Blood 122, 1678–1684.Google Scholar

38. Lu, W, Zhao, M, Rajbhandary, S, et al. (2013) Free iron catalyzes oxidative damage to hematopoietic cells/mesenchymal stem cells in vitro and suppresses hematopoiesis in iron overload patients. Eur J Haematol 91, 249–261.Google Scholar

39. Efebera, YA, Thandi, RS, Saliba, RM, et al. (2009) The impact of pre-stem cell transplant ferritin level on late transplant complications: an analysis to determine the potential role of iron overload on late transplant outcomes. Internet J Hematol 7, 9127.Google Scholar

40. Kim, YR, Kim, JS, Cheong, JW, et al. (2008) Transfusion-associated iron overload as an adverse risk factor for transplantation outcome in patients undergoing reduced-intensity stem cell transplantation for myeloid malignancies. Acta Haematol 120, 182–189.Google Scholar

41. Kanda, J, Kawabata, H & Chao, NJ (2011) Iron overload and allogeneic hematopoietic stem-cell transplantation. Expert Rev Hematol 4, 71–80.Google Scholar

42. Pullarkat, V (2010) Iron overload in patients undergoing hematopoietic stem cell transplantation. Adv Hematol 2010, 345756.Google Scholar

43. Chai, X, Li, D, Cao, X, et al. (2015) ROS-mediated iron overload injures the hematopoiesis of bone marrow by damaging hematopoietic stem/progenitor cells in mice. Sci Rep 5, 10181.Google Scholar

44. Tataranni, T, Agriesti, F, Mazzoccoli, C, et al. (2015) The iron chelator deferasirox affects redox signalling in haematopoietic stem/progenitor cells. Br J Haematol 170, 236–246.Google Scholar

45. Zhang, Y, Zhai, W, Zhao, M, et al. (2015) Effects of iron overload on the bone marrow microenvironment in mice. PLOS ONE 10, e0120219.Google Scholar

46. Suda, T, Takubo, K & Semenza, GL (2011) Metabolic regulation of hematopoietic stem cells in the hypoxic niche. Cell Stem Cell 9, 298–310.Google Scholar

47. Keen, CL, Ensunsa, JL, Watson, MH, et al. (1999) Nutritional aspects of manganese from experimental studies. Neurotoxicology 20, 213–223.Google Scholar

48. Furst, A (1978) Tumorigenic effect of an organomanganese compound on F344 rats and Swiss albino mice: brief communication. J Natl Cancer Inst 60, 1171–1173.Google Scholar

49. Carl, GF & Gallagher, BB (1994) Manganese and epilepsey. In Manganese in Health and Disease, pp. 133–143 [DJ Klimis-Tavantzis, editor]. Boca Raton, FL: CRC Press.Google Scholar

50. Keen, CL, Ensunsa, JL & Clegg, MS (2000) Manganese metabolism in animals and humans including the toxicity of manganese. In Metal Ions in Biological Systems: Volume 37: Manganese and its Role in Biological Processes, pp. 89–121 [A Sigel and H Sigel, editors]. New York: Marcel Dekker.Google Scholar

51. Crossgrove, J & Zheng, W (2004) Manganese toxicity upon overexposure. NMR Biomed 17, 544–553.Google Scholar

52. Finley, JW & Davis, CD (1999) Manganese deficiency and toxicity: are high or low dietary amounts of manganese cause for concern? Biofactors 10, 15–24.Google Scholar

53. Kizaki, M, Sakashita, A, Karmakar, A, et al. (1993) Regulation of manganese superoxide dismutase and other antioxidant genes in normal and leukemic hematopoietic cells and their relationship to cytotoxicity by tumor necrosis factor. Blood 82, 1142–1150.Google Scholar

54. Lebovitz, RM, Zhang, H, Vogel, H, et al. (1996) Neurodegeneration, myocardial injury, and perinatal death in mitochondrial superoxide dismutase-deficient mice. Proc Natl Acad Sci U S A 93, 9782–9787.Google Scholar

55. Friedman, JS, Rebel, VI, Derby, R, et al. (2001) Absence of mitochondrial superoxide dismutase results in a murine hemolytic anemia responsive to therapy with a catalytic antioxidant. J Exp Med 193, 925–934.Google Scholar

56. Case, AJ, Madsen, JM, Motto, DG, et al. (2013) Manganese superoxide dismutase depletion in murine hematopoietic stem cells perturbs iron homeostasis, globin switching, and epigenetic control in erythrocyte precursorcells. Free Radic Biol Med 56, 17–27.Google Scholar

57. Moore, B (1911) In memory of Sidney Ringer [1835–1910]: some account of the fundamental discoveries of the great pioneer of the bio-chemistry of crystallo-colloids in living cells. Biochem J 5, i.b3–xix.Google Scholar

58. Bootman, MD (2012) Calcium signaling. Cold Spring Harb Perspect Biol 4, a011171.Google Scholar

59. Berridge, MJ, Bootman, MD & Roderick, L (2003) Calcium signalling: dynamics, homeostasis and remodeling. Nat Rev Mol Cell Biol 4, 517–529.Google Scholar

60. Dupont, G, Combettes, L, Bird, GS, et al. (2011) Calcium oscillations. Cold Spring Harb Perspect Biol 3, a004226.Google Scholar

61. Paredes-Gamero, EJ, Barbosa, CMV & Ferreira, AT (2012) Calcium signaling as a regulator of hematopoiesis. Front Biosci 4, 1375–1384.Google Scholar

62. Leon, CM, Barbosa, CM, Justo, GZ, et al. (2011) Requirement for PLCγ2 in IL-3 and GM-CSF-stimulated MEK/ERK phosphorylation in murine and human hematopoietic stem/progenitor cells. J Cell Physiol 226, 1780–1792.Google Scholar

63. Adams, GB, Chabner, KT, Alley, IR, et al. (2006) Stem cell engraftment at the endosteal niche is specified by the calcium-sensing receptor. Nature 439, 599–603.Google Scholar

64. Pozzan, T, Rizzuto, R, Volpe, P, et al. (1994) Molecular and cellular physiology of intracellular calcium stores. Physiol Rev 74, 595–636.Google Scholar

65. Webb, SE, Li, WM & Miller, AL (2008) Calcium signalling during the cleavage period of zebrafish development. Philos Trans R Soc Lond B Biol Sci 363, 1363–1369.Google Scholar

66. Wölwer, CB, Pase, LB, Russell, SM, et al. (2016) Calcium signaling is required for erythroid enucleation. PLOS ONE 11, e0146201.Google Scholar

67. Drueke, TB (2006) Haematopoietic stem cells – role of calcium-sensing receptor in bone marrow homing. Nephrol Dial Transplant 21, 2072–2074.Google Scholar

68. Barbosa, CM, Bincoletto, C, Barros, CC, et al. (2014) PLCγ2 and PKC are important to myeloid lineage commitment triggered by M-SCF and G-CSF. J Cell Biochem 115, 42–51.Google Scholar

69. Paredes-Gamero, EJ, Leon, CM, Borojevic, R, et al. (2008) Changes in intracellular Ca²⁺ levels induced by cytokines and P2 agonists differentially modulate proliferation or commitment with macrophage differentiation in murine hematopoietic cells. J Biol Chem 283, 31909–31919.Google Scholar

70. Barbosa, CMV, Leon, CMMP, Nogueira-Pedro, A, et al. (2011) Differentiation of hematopoietic stem cell and myeloid populations by ATP is modulated by cytokines. Cell Death Dis 2, e165.Google Scholar

71. Rubin, H (1975) Central role for magnesium in coordinate control of metabolism and growth in animal cells. Proc Natl Acad Sci U S A 72, 3551–3555.Google Scholar

72. Birch, NG (1993) Magnesium and the Cell. San Diego, CA: Academic Press.Google Scholar

73. Cowan, JA (1995) The Biological Chemistry of Magnesium. New York: VCH Publishers.Google Scholar

74. Walker, GM (1986) Magnesium and cell cycle control: an update. Magnesium 5, 9–23.Google Scholar

75. Cameron, IL & Smith, NK (1989) Cellular concentration of magnesium and other ions in relation to protein synthesis, cell proliferation and cancer. Magnesium 8, 31–44.Google Scholar

76. Wolf, FI & Cittadini, A (1999) Magnesium in cell proliferation and differentition. Front Biosci 4, 607–617.Google Scholar

77. Stritt, S, Nurden, P, Favier, R, et al. (2016) Defects in TRPM7 channel function deregulate thrombopoiesis through altered cellular Mg²⁺ homeostasis and cytoskeletal architecture. Nat Commun 7, 11097.Google Scholar

78. Elin, RJ, Utter, A, Tan, HK, et al. (1980) Effect of magnesium deficiency on erythrocyte aging in rats. Am J Pathol 100, 765–778.Google Scholar

79. Fedorocko, P, Macková, NO, Sándorcínová, Z, et al. (2000) Influence of age and K, Mg aspartate (Cardilan) on murine haemopoiesis. Mech Ageing Dev 119, 159–170.Google Scholar

80. Lang, F (2007) Mechanisms and significance of cell volume regulation. J Am Coll Nutr 26, 613S–623S.Google Scholar

81. Singh, S, Pandey, KB & Rizvi, SI (2016) Erythrocyte senescence and membrane transporters in young and old rats. Arch Physiol Biochem 122, 228–234.Google Scholar

82. Blostein, R, Drapeau, P, Benderoff, S, et al. (1983) Changes in Na⁺-ATPase and Na,K-pump during maturation of sheep reticulocytes. Can J Biochem Cell Biol 61, 23–28.Google Scholar

83. Lauf, PK & Mangor-Jensen, A (1984) Effects of A23187 and Ca²⁺ on volume- and thiol-stimulated, ouabain-resistant K⁺C1^– fluxes in low K⁺ fluxes in low K⁺ sheep erythrocytes. Biochem Biophys Res Commun 125, 790–796.Google Scholar

84. Brugnara, C & Tosteson, DC (1987) Cell volume, K⁺ transport and cell density in human erythrocytes. Am J Physiol 252, C269–C276.Google Scholar

85. Canessa, M, Fabry, ME, Blumenfeld, N, et al. (1987) Volume-stimulated, Cl^–-dependent K⁺ efflux is highly expressed in young human red cells containing normal hemoglobin or HbS. J Membr Biol 97, 97–105.Google Scholar

86. Furukawa, H, Bilezikian, JP & Loeb, JN (1981) Potassium fluxes in the rat reticulocyte. Ouabain sensitivity and changes in the maturation. Biochim Biophys Acta 649, 625–632.Google Scholar

87. Kosower, NS (1993) Altered properties of erythrocytes in the aged. Am J Hematol 42, 241–247.Google Scholar

88. Mairbäurl, H, Schulz, S & Hoffman, JF (2000) Cation transport and cell volume changes in maturing rat reticulocytes. Am J Physiol Cell Physiol 279, C1621–C1630.Google Scholar

89. Gallicchio, VS & Murphy, MJ Jr (1979) Erythropoiesis in vitro. III. The role of potassium ions in erythroid colony formation. Exp Hematol 7, 225–230.Google Scholar

90. Gallicchio, VS & Murphy, MJ Jr (1983) Cation influences on in vitro growth of erythroid stem cells (CFU-e and BFU-e). Cell Tissue Res 233, 175–181.Google Scholar

91. Mager, DL, MacDonald, ME & Bernstein, A (1979) Growth in high-K⁺ medium induces Friend cell differentiation. Dev Biol 70, 268–273.Google Scholar

92. Shirihai, O, Merchav, S, Attali, B, et al. (1996) K⁺ channel antisense oligodeoxynucleotides inhibit cytokine-induced expansion of human hemopoietic progenitors. Pflugers Arch 431, 632–638.Google Scholar

93. Shirihai, O, Attali, B, Dagan, D, et al. (1998) Expression of two inward rectifier potassium channels is essential for differentiation of primitive human hematopoietic progenitor cells. J Cell Physiol 177, 197–205.Google Scholar

94. Banati, RB, Hoppe, D, Gottmann, K, et al. (1991) A subpopulation of bone marrow-derived macrophage like cells share a unique ion channel pattern wit microglia. J Neurosci Res 30, 593–600.Google Scholar

95. Kettenmann, H, Hoppe, D, Gottmann, K, et al. (1990) Cultured microglial cells have a distinct pattern of membrane channels different from peritoneal macrophages. J Neurosci Res 26, 278–287.Google Scholar

96. Wieland, SJ, Chou, RH & Chen, TA (1987) Elevation of a potassium current in differentiating human leukemic (HL-60) cells. J Cell Physiol 132, 371–375.Google Scholar

97. McCann, FV, Keller, TM & Guyre, PM (1987) Ion channels in human macrophages compared with the U-937 cell line. J Membrane Biol 96, 57–64.Google Scholar

98. Lu, L, Yang, T, Markakis, D, et al. (1993) Alterations in a voltage-gated K⁺ current during the differentiation of ML-1 human myeloblastic leukemia cells. J Membrane Biol 132, 267–274.Google Scholar

99. Expert Group on Vitamins and Minerals (2003) Safe Upper Levels for Vitamins and Minerals. London: Food Standards Agency.Google Scholar

100. Kobayashi, M & Shimizu, S (1999) Cobalt proteins. Eur J Biochem 26, 1–9.Google Scholar

101. Banerjee, R (1997) The Yin-Yang of cobalamin biochemistry. Chem Biol 4, 175–186.Google Scholar

102. Barceloux, DG (1999) Cobalt. Clin Toxicol 37, 201–216.Google Scholar

103. Institute of Medicine (1998) Cobalt. In Dietary Reference Intakes for Thiamin, Riboflavin, Niacin, Vitamin B₆, Folate, Vitamin B₁₂, Pantothenic Acid, Biotin, and Choline, pp. 306–356. Washington, DC: National Academies Press.Google Scholar

104. Varela-Moreiras, G, Murphy, MM & Scott, JM (2009) Cobalamin, folic acid, and homocysteine. Nutr Rev 67, S69–S72.Google Scholar

105. Andrès, E, Affenberger, S, Zimmer, J, et al. (2006) Current hematological findings in cobalamin deficiency: a study of 201 consecutive patients with documented cobalamin deficiency. Clin Lab Haematol 28, 50–56.Google Scholar

106. Koury, MJ & Ponka, P (2004) New insights into erythropoiesis: the roles of folate, vitamin B₁₂, and iron. Annu Rev Nutr 24, 105–131.Google Scholar

107. Waltner, K & Waltner, K (1929) Kobalt und blut (Cobalt and blood). Klin Wochenschr 8, 313.Google Scholar

108. Weissbecker, L (1950) Die kobalttherapie (Cobalt therapy). Dtsch Med Wochenschr 75, 116–118.Google Scholar

109. Thorling, EB & Erslev, AJ (1972) The effect of some erythropoietic agents on the “tissue” tensions of oxygen. Br J Haematol 23, 483–490.Google Scholar

110. Jelkmann, W (2012) The disparate roles of cobalt in erythropoiesis, and doping relevance. Open J Hematol 3, 3–6.Google Scholar

111. Berk, L, Burchenaj, LH & Castlew, B (1949) Erythropoietic effect of cobalt in patients with or without anemia. N Engl J Med 240, 754–761.Google Scholar

112. Gardnerf, H (1953) The effect of cobaltous chloride in the anemia associated with chronic renal disease. J Lab Clin Med 41, 56–64.Google Scholar

113. Duckham, JM & Lee, HA (1976) The treatment of refractory anaemia of chronic renal failure with cobalt chloride. Q J Med 45, 277–294.Google Scholar

114. De Boeck, M, Kirsch-Volders, M & Lison, D (2003) Cobalt and antimony: genotoxicity and carcinogenicity. Mutat Res 533, 135–152.Google Scholar

115. World Health Organization International Agency for Research on Cancer (2006) IARC monographs on the evaluation of carcinogenic risks to humans: volume 86: cobalt in hard metals and cobalt sulfate, gallium arsenide, indium phosphide and vanadium pentoxide. http://monographs.iarc.fr/ENG/Monographs/vol86/mono86.pdf (accessed May 2018).Google Scholar

116. Niwattisaiwong, S, Burman, KD & Li-ng, M (2017) Iodine deficiency: clinical implications. Cleve Clin J Med 84, 236–244.Google Scholar

117. Brent, G (2012) Mechanisms of thyroid hormone action. J Clin Invest 122, 3035–3043.Google Scholar

118. Mondal, S, Raja, K, Schweizer, U, et al. (2016) Chemistry and biology in the biosynthesis and action of thyroid hormones. Angew Chem Int Ed Engl 55, 7606–7630.Google Scholar

119. Flores-Morales, A, Gullberg, H, Fernandez, L, et al. (2002) Patterns of liver gene expression governed by TRβ. Mol Endocrinol 16, 1257–1268.Google Scholar

120. Hara, M, Suzuki, S, Mori, J, et al. (2000) Thyroid hormone regulation of apoptosis induced by retinoic acid in promyeloleukemic Hl-60 cells: studies with retinoic acid receptor-specific and retinoid X receptor-specific ligands. Thyroid 10, 1023–1034.Google Scholar

121. Lin, HY, Davis, FB, Gordinier, JK, et al. (1999) Thyroid hormone induces activation of mitogen-activated protein kinase in cultured cells. Am J Physiol 276, C1014–C1024.Google Scholar

122. Wu, SY, Green, WL, Huang, WS, et al. (2005) Alternate pathways of thyroid hormone metabolism. Thyroid 15, 943–958.Google Scholar

123. Kocher, T (1908) Blutuntersuchungen bei Morbus Basedowii mit Beiträgen zur Frühdiagnose u. Theorie der Krankheit (Blood tests in Basedowii disease with contributions to early diagnosis and the theory of illness). Arch Klin Chir 87, 131.Google Scholar

124. Evans, ES, Rosenberg, LL & Simpson, ME (1961) Erythropoietic response to calorigenic hormones. Endocrinology 68, 517–532.Google Scholar

125. Tudhope, GR & Wilson, GM (1960) Anemia in hypothyroidism. Q J Med 29, 513–533.Google Scholar

126. Wu, Y & Koenig, RJ (2000) Gene regulation by thyroid hormone. Trends Endocrinol Metab 11, 207–211.Google Scholar

127. Golde, DW, Bersch, N, Chopra, IJ, et al. (1977) Thyroid hormones stimulate erythropoiesis in vitro . Br J Haematol 37, 173–177.Google Scholar

128. Gruber, R, Czerwenka, K, Wolf, F, et al. (1999) Expression of the vitamin D receptor, of estrogen and thyroid hormone receptor α- and β-isoforms, and of the androgen receptor in cultures of native mouse bone marrow and stromal/osteoblastic cells. Bone 24, 465–473.Google Scholar

129. Milne, M, Kang, MI, Cardona, G, et al. (1999) Expression of multiple thyroid hormone receptor isoforms in rat femoral and vertebral bone marrow and in bone marrow osteogenic cultures. J Cell Biochem 74, 684–693.Google Scholar

130. Grymuła, K, Paczkowska, E, Dziedziejko, V, et al. (2007) The influence of 3,3’,5-triiodo-l-thyronine on human haematopoiesis. Cell Prolif 40, 302–315.Google Scholar

131. Kawa, MP, Grymula, K, Paczkowska, E, et al. (2010) Clinical relevance of thyroid dysfunction in human haematopoiesis: biochemical and molecular studies. Eur J Endocrinol 162, 295–305.Google Scholar

132. Bauer, A, Mikulits, W, Lagger, G, et al. (1998) The thyroid hormone receptor function as a ligand-operated developmental switch between proliferation and differentiation of erythroid progenitors. EMBO J 17, 4291–4303.Google Scholar

133. Tran, L, Batech, M, Rhee, CM, et al. (2016) Serum phosphorus and association with anemia among a large diverse population with and without chronic kidney disease. Nephrol Dial Transplant 31, 636–645.Google Scholar

134. Raanani, P, Levi, I, Holzman, F, et al. (2001) Engraftment-associated hypophosphatemia – the role of cytokine release and steep leukocyte rise post stem cell transplantation. Bone Marrow Transplant 27, 311–317.Google Scholar

135. Uçkan, D, Cetin, M, Dida, A, et al. (2003) Hypophosphatemia and hypouricemia in pediatric allogeneic bone marrow transplant recipients. Pediatr Transplant 7, 98–101.Google Scholar

136. Clark, RE & Lee, ES (1995) Severe hypophosphataemia during stem cell harvesting in chronic myeloid leukaemia. Br J Haematol 90, 450–452.Google Scholar

137. Crook, M, Swaminathan, R & Schey, S (1996) Hypophosphataemia in patients undergoing bone marrow transplantation. Leuk Lymphoma 22, 335–337.Google Scholar

138. Kovesdy, CP, Mucsi, I, Czira, ME, et al. (2011) Association of serum phosphorus level with anemia in kidney transplant recipients. Transplantation 91, 875–882.Google Scholar

139. Wojcicki, JM (2013) Hyperphosphatemia is associated with anemia in adults without chronic kidney disease: results from the National Health and Nutrition Examination Survey (NHANES): 2005–2010. BMC Nephrol 14, 178.Google Scholar

140. Kuroo, M (2014) New developments in CKD-MBD. Why is phosphate overload harmful? (article in Japanese). Clin Calcium 24, 1785–1792.Google Scholar

141. Navarro-Alarcon, M & Cabrera-Vique, C (2008) Selenium in food and the human body: a review. Sci Total Environ 400, 115–141.Google Scholar

142. Tinggi, U (2003) Essentiality and toxicity of selenium and its status in Australia: a review. Toxicol Lett 137, 103–110.Google Scholar

143. Puspitasari, IM, Abdulah, R, Yamazaki, C, et al. (2014) Updates on clinical studies of selenium supplementation in radiotherapy. Radiat Oncol 9, 125.Google Scholar

144. Kaushal, N, Hegde, S, Lumadue, J, et al. (2011) The regulation of erythropoiesis by selenium in mice. Antioxid Redox Signal 14, 1403–1412.Google Scholar

145. Costa, NA, Gut, AL, Pimentel, JA, et al. (2014) Erythrocyte selenium concentration predicts intensive care unit and hospital mortality in patients with septic shock: a prospective observational study. Crit Care 18, R92.Google Scholar

146. Gandhi, UH, Kaushal, N, Hegde, S, et al. (2014) Selenium suppresses leukemia through the action of endogenous eicosanoids. Cancer Res 74, 3890–3901.Google Scholar

147. Rosenfeld, I & Beath, OA (1946) The influence of protein diets on selenium poisoning. Am J Vet Res 7, 52–56.Google Scholar

148. Grubman, A & White, AR (2014) Copper as a key regulator of cell signalling pathways. Expert Rev Mol Med 16, e11.Google Scholar

149. Huang, X, Pierce, LJ, Cobine, PA, et al. (2009) Copper modulates the differentiation of mouse hematopoietic progenitor cells in culture. Cell Transplant 18, 887–897.Google Scholar

150. Williams, DM (1983) Copper deficiency in humans. Semin Hematol 20, 118–128.Google Scholar

151. Choi, JW & Kim, SK (2005) Relationships of lead, copper, zinc, and cadmium levels versus hematopoiesis and iron parameters in healthy adolescents. Ann Clin Lab Sci 35, 428–434.Google Scholar

152. Bustos, RI, Jensen, EL, Ruiz, LM, et al. (2013) Copper deficiency alters cell bioenergetics and induces mitochondrial fusion through up-regulation of MFN2 and OPA1 in erythropoietic cells. Biochem Biophys Res Commun 437, 426–432.Google Scholar

153. Bae, B & Percival, SS (1993) Retinoic acid-induced HL-60 cell differentiation is augmented by copper supplementation. J Nutr 123, 997–1002.Google Scholar

154. Zhou, XY, Zhang, T, Ren, L, et al. (2016) Copper elevated embryonic hemoglobin through reactive oxygen species during zebrafish erythrogenesis. Aquat Toxicol 175, 1–11.Google Scholar

155. Boggs, DR & Joyce, RA (1983) The hematopoietic effects of lithium. Semin Hematol 20, 129–138.Google Scholar

156. Ferensztajn-Rochowiak, E & Rybakowski, JK (2016) The effect of lithium on hematopoietic, mesenchymal and neural stem cells. Pharmacol Rep 68, 224–230.Google Scholar

157. McGrath, HE, Wade, PM, Kister, VK, et al. (1992) Lithium stimulation of HPP-CFC and stromal growth factor production in murine Dexter culture. J Cell Physiol 151, 276–286.Google Scholar

158. McGrath, HE, Liang, CM, Alberico, TA, et al. (1987) The effect of lithium on growth factor production in long-term bone marrow cultures. Blood 70, 1136–1142.Google Scholar

159. Hager, ED, Dziambor, H, Winkler, P, et al. (2002) Effects of lithium carbonate on hematopoietic cells in patients with persistent neutropenia following chemotherapy or radiotherapy. J Trace Elem Med Biol 16, 91–97.Google Scholar

160. Gallicchio, VS & Chen, MG (1980) Modulation of murine pluripotential stem cell proliferation in vivo by lithium carbonate. Blood 56, 1150–1152.Google Scholar

161. Gallicchio, VS, Hughes, NK, Tse, KF, et al. (1995) Effect of lithium in immunodeficiency: improved blood cell formation in mice with decreased hematopoiesis as the result of LP-BM5 MuLV infection. Antiviral Res 26, 189–202.Google Scholar

162. Walasek, MA, Bystrykh, L, van den Boom, V, et al. (2012) The combination of valproic acid and lithium delays hematopoietic stem/progenitor cell differentiation. Blood 119, 3050–3059.Google Scholar

163. Vallee, BL & Falchuk, KH (1993) The biochemical basis of zinc physiology. Physiol Rev 73, 79–118.Google Scholar

164. Berg, JM (1986) Potential metal-binding domains in nucleic acid binding proteins. Science 232, 485–487.Google Scholar

165. Ackland, ML & Michalczyk, AA (2016) Zinc and infant nutrition. Arch Biochem Biophys 611, 51–57.Google Scholar

166. Murakami, K, Whiteley, MK & Routtenberg, A (1987) Regulation of protein kinase C activity by cooperative interaction of Zn²⁺ and Ca² ⁺ J Biol Chem 262, 13902–13906.Google Scholar

167. Chen, YH, Shiu, JR, Ho, CL, et al. (2017) Zinc as a signal to stimulate red blood cell formation in fish. Int J Mol Sci 18, E138.Google Scholar

168. Chirulescu, Z, Suciu, A, Tănăsescu, C, et al. (1990) Possible correlation between the zinc and copper concentrations involved in the pathogenesis of various forms of anemia. Med Interne 28, 31–35.Google Scholar

169. Livingstone, C (2015) Zinc: physiology, deficiency, and parenteral nutrition. Nutr Clin Pract 30, 371–382.Google Scholar

170. King, LE, Osati-Ashtiani, F & Fraker, PJ (1995) Depletion of cells of the B lineage in the bone marrow of zinc-deficient mice. Immunology 85, 69–73.Google Scholar

171. Fraker, PJ & King, LE (2001) A distinct role for apoptosis in the changes in lymphopoiesis and myelopoiesis created by deficiencies in zinc. FASEB J 15, 2572–2578.Google Scholar

172. Cook-Mills, JM & Fraker, PJ (1993) Functional capacity of the residual lymphocytes from zinc-deficient adult mice. Br J Nutr 69, 835–848.Google Scholar

Table 1 Main findings of the effects of minerals on haematopoiesis

Fig. 1 Iron absorption and metabolism. Most of the iron content is incorporated in erythrocyte Hb, and the hepatocytes represent the main site for iron storage.

Fig. 2 Main effects of calcium deficiency on the haematopoietic system.

Fig. 3 Main effects of magnesium deficiency on the haematopoietic system.

Fig. 4 Iodine is an essential constituent of the thyroid thyroxine hormones. Thyroid hormones classically stimulate erythropoiesis by increasing the oxygen demand on the kidneys and stimulating erythropoietin production. T3, triiodothyronine; T4, tetraiodothyronine; TR, thyroid hormone receptor.

Fig. 5 Main effects of copper deficiency on the haematopoietic system.

Article contents

A review of select minerals influencing the haematopoietic process

Abstract

Keywords

Introduction

Iron

Manganese

Calcium

Magnesium

Sodium and potassium

Cobalt

Iodine

Phosphorus

Selenium

Copper

Lithium

Zinc

Conclusion

Acknowledgements

References

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