Absolute versus functional iron deficiency

Hye Lim Jung

doi:10.3345/cep.2023.01732

Iron deficiency (ID), the most common cause of anemia, leads to iron-deficiency anemia (IDA), followed by inflammation leading to anemia of inflammation, better known as anemia of chronic disease [1]. IDA remains the most prevalent type of anemia globally, affecting children, pregnant and nonpregnant premenopausal women, and people in low- and middle-income countries [2,3]. ID is twice as prevalent as IDA, affecting more than 2 billion people globally [4,5]. As iron is necessary for erythropoiesis, myoglobin synthesis, and numerous cellular processes, ID can cause various physiological and cellular impairments, even without anemia [3,4]. In children and adolescents, it can cause failure to thrive, cognitive impairment, decreased school performance, breath-holding spells, restless leg syndrome, attention-deficit hyperactivity disorder, immune system dysregulation, and cardiac problems [4,5]. Therefore, controlling ID and IDA is a global health priority [2-4].

Total body iron is distributed in the erythrocytes, muscles, and iron-dependent enzymes for cellular metabolism and stored in the liver, spleen, and bone marrow [2,3,6]. Total body iron is sourced predominantly from recycled iron scavenged from senescent erythrocytes by macrophages in the reticuloendothelial system (RES), while a smaller amount (1–2 mg/day) is sourced from dietary iron absorbed in the duodenum [2,3,7]. Hepcidin, a protein produced by hepatocytes, regulates systemic iron homeostasis by degrading ferroportin, the key iron exporter expressed on macrophages and duodenal enterocytes [1-4]. Ferroportin exports iron from macrophages, duodenal enterocytes, and hepatocytes to the plasma. Hepcidin production is suppressed by erythropoiesis, hypoxia, and absolute ID, decreasing ferroportin degradation and increasing plasma iron levels [2,3]. Hepcidin production is increased by high iron levels and inflammation [2,3].

ID can be absolute or functional [2,3]. Absolute ID is due to low or depleted total body iron stores that causes iron deficient erythropoiesis. Its etiologies include inadequate iron uptake (poor dietary iron nutrition, reduced iron absorption), increased iron requirements, increased iron loss, and exercise (Table 1) [2,3]. Absolute ID suppresses hepcidin production and ferroportin degradation, upregulating iron absorption at the gastroduodenal junction using divalent meta-transporter 1 and iron export from macrophages and hepatocytes into the circulation [2,3,6]. Absolute ID is diagnosed as low serum ferritin (≤30 μg/L) and low serum transferrin saturation (TSAT; <20%) (Table 1) [2-5]. The diagnostic threshold of serum ferritin (≤30 μg/L) has 92% sensitivity and 98% specificity for diagnosing ID, but inflammation and age-related factors should be considered since its levels increase with age [2,4]. Hepcidin is an emerging indicator of ID that can distinguish between types [3]. IDA is diagnosed at a hemoglobin (Hb) <13 g/dL in men, Hb <12 g/dL in women, and Hb <11 g/dL in pregnant women [2]. Indications for iron therapy in absolute ID include anemia, symptoms, premature birth, pregnancy, before surgery, uncorrected underlying factors (e.g., growth) in children, poor iron intake, and blood loss. Absolute ID can be treated with oral or intravenous (IV) iron therapy (Table 1) [2,5,8]. Orally, 2–3 mg/kg of elemental Fe²⁺ iron in 1 or 2 doses/day taken 30 minutes before or after a meal or 3–5 mg/kg of elemental Fe³⁺ iron in 1 or 2 doses/day with meals (and juice or water since polymaltose is a sugar complex that must be dissolved in the gastric fluid) is recommended [5]. IV iron therapy improves Hb and serum ferritin levels in iron-resistant IDA with the TMPRSS6 mutation [5,8].

Functional ID is an imbalance between iron demand and availability despite adequate total body stores that causes iron-restricted erythropoiesis [1-4]. Its etiologies are inflammation and/or infection causing anemia of chronic disease or inflammation, including cancer, autoimmune disease, chronic kidney disease (CKD), congestive heart failure (CHF), chronic pulmonary disease, inflammatory bowel disease (IBD), and obesity (Table 1) [1]. In functional ID, inflammatory cytokines such as interleukin (IL)-6, IL-1β, and lipopolysaccharide induce hepcidin production, causing ferroportin degradation and iron retention of macrophages in RES, decreased iron absorption at the gastroduodenal junction, and decreased bioavailability of plasma iron, ultimately resulting in iron-restricted erythropoiesis (Table 1) [1,3,4,6,9]. Inflammatory cytokines such as IL-1, tumor necrosis factor-α, and interferon-γ inhibit renal erythropoietin production and activity, inhibit erythropoiesis by radical formation, and promote hepatic and splenic erythrophagocytosis, reducing erythrocyte half life (Table 1) [1,2,4,9]. Functional ID is diagnosed at a TSAT < 20% and serum ferritin level <100 μg/L, the former being more important [1,2,4,8]. In CHF, ferritin <100 μg/L, or ferritin <300 μg/L with TSAT < 20%, is used to diagnose ID (Table 1) [2]. For patients with CKD, the Kidney Disease Improving Global Outcomes Guideline recommends considering iron therapy at ferritin ≤500 μg/L and TSAT ≤30% (Table 1), but in recent clinical trials in patients with CKD receiving dialysis, a ferritin level <200 μg/L or TSAT <20% was an indication for iron therapy [2]. Functional ID is best treated with IV iron and/or erythropoiesis-stimulating agent (ESA) therapy with underlying disease correction [1-5,8-10]. IV iron with ESA therapy showed clinical and laboratory improvements in patients with malignancy and chemotherapy-induced anemia, CKD receiving dialysis, and IBD who were intolerant of oral iron therapy [1-5,8-10]. IV iron therapy-improved the exercise capacity and quality of life of patients with CHF and ID [3,8-10]. For IV iron therapy in children, ferric sucrose is authorized from 3 years of age, while ferric carboxymaltose is authorized from 18 years of age in United States and from 14 years of age in Europe [5,8,10].

Footnotes

Conflicts of interest

No potential conflict of interest relevant to this article was reported.

Funding

This study received no specific grant from any funding agency in the public, commercial, or not-forprofit sectors.

Table 1.

Absolute iron deficiency versus functional iron deficiency

Category	Absolute iron deficiency	Functional iron deficiency
Definition	Low or depleted total body iron stores	Imbalance between iron demand and iron availability, despite adequate total body iron stores
Etiology	Poor dietary iron nutrition: low heme iron diet such as vegan diet; poverty; prolonged breastfeeding, milk preference	Inflammation and/or infection
		Anemia of chronic disease
	Reduced iron absorption: GI diseases such as Celiac disease, atrophic gastritis, inflammatory bowel disease; bowel resection; high gastric PH due to antacid or proton pump inhibitor therapy or Helicobacter pylori infection; competition from other metals such as calcium, copper, lead or zinc; intrinsic erythrocyte defects; iron-refractory IDA due to mutation of TMPRSS6 gene	Anemia of inflammation:
		Autoimmune disease
		Cancer
	Increased iron requirements: growth, pregnancy, erythropoiesisstimulating agent therapy	Chronic kidney disease (CKD)
		Congestive heart failure (CHF)
	Blood loss: GI blood loss, genitourinary blood loss such as heavy menstrual bleeding, pulmonary blood loss, trauma, phlebotomy, large vascular malformation	Chronic pulmonary disease
		Inflammatory bowel disease
	Exercise: multifactorial	Obesity
		Elderly
		Critical illness (accelerated course)
Pathophysiology	Low total body iron stores	Increased inflammatory cytokines (IL-6, IL-1β, IL-10, TNF-α, IFN-γ)
	Iron-deficient erythropoiesis	IL-6, IL-1β, LPS induce hepatic hepcidin production
	Suppressed hepatic hepcidin production	Increased ferroportin degradation
	Decreased ferroportin degradation	Reduced GI absorption of iron
	Increased GI absorption of iron	Increased iron sequestration in macrophages of RES
	Increased iron export from macrophages and hepatocytes into plasma	Iron-restricted erythropoiesis
		IL-1β, TNF-α and IFN-γ inhibit renal production and activity of EPO; inhibit erythropoiesis through radical formation; promote hepatic and splenic erythrophagocytosis reducing erythrocyte survival
Diagnosis	Ferritin ≤30 μg/L (WHO: Ferritn <12 μg/L in children <5 years of age; Ferritin <15 μg/L in person over 5 years of age)	TSAT <20%
	TSAT <20%	Ferritin <100 μg/L
	Normal to low Hb	In CHF: ferritin <100 μg/L or ferritin <300 μg/L with TSAT <20%
	Increased sTfR	In CKD considering for iron therapy: ferritin ≤ 500 μg/L and TSAT ≤30%
	CHr low <29 pg	Mild to moderate anemia
	Normal to low MCV (<75 fL) and MCH	Normal sTfR
	RDW increased	CHr low <29 pg
	Hepcidin low	Normal to mild low MCV and MCH
	Bone marrow (not recommended for routine screening): absent iron stores	Hepcidin high relative to TSAT
Treatment	Heme iron in food	Treatment of underlying diseases
	Oral iron therapy	IV iron therapy
	IV iron therapy	Erythropoiesis-stimulating agents
		Blood transfusion
		Vitamin B9, B12, D, C
Novel therapeutics		Antagonists of hepcidin
Novel therapeutics		Agents that redistribute endogenous iron for erythropoiesis

GI, gastrointestinal; IDA, iron-deficiency anemia; IL, interleukin; TNF, tumor necrosis factor; IFN, interferon; LPS, lipopolysaccharide; RES, reticuloendothelial system; EPO, erythropoietin; WHO, World Health Oraganization; ferritin, serum ferritin; TSAT, transferrin saturation; IV, intravenous; sTfR, soluble transferrin receptor; Hb, hemoglobin; CHr, reticulate hemoglobin content; MCV, mean corpuscular volume; MCH, mean corpuscular hemoglobin; RDW, red cell distribution width.

References

1. Weiss G, Ganz T, Goodnough LT. Anemia of inflammation. Blood 2019;133:40–50.

2. Ning S, Zeller MP. Management of iron deficiency. Hematology Am Soc Hematol Educ Program 2019;2019:315–22.

3. Pasricha SR, Tye-Din J, Muckenthaler MU, Swinkels DW. Iron deficiency. Lancet 2021;397:233–48.

4. Lee NH. Iron deficiency in children with a focus on inflammatory conditions. Clin Exp Pediatr 2024;67:283–93.

5. Mattiello V, Schmugge M, Hengartner H, von der Weid N, Renella R, SPOG Pediatric Hematology Working Group. Diagnosis and management of iron deficiency in children with or without anemia: consensus recommendations of the SPOG Pediatric Hematology Working Group. Eur J Pediatr 2020;179:527–45.

6. Andrews NC. Disorders of iron metabolism. N Engl J Med 1999;341:1986–995.

7. Koleini N, Shapiro JS, Geier J, Ardehali H. Ironing out mechanisms of iron homeostasis and disorders of iron deficiency. J Clin Invest 2021;131:e148671.

8. Lee NH. Iron deficiency anemia. Clin Pediatr Hematol Oncol 2020;27:101–12.

9. Lanser L, Fuchs D, Kurz K, Weiss G. Physiology and inflammation driven pathophysiology of iron homeostasis mechanistic insights into anemia of inflammation and its treatment. Nutrients 2021;13:3732.

10. Goodnough LT, Nemeth E, Ganz T. Detection, evaluation, and management of iron-restricted erythropoiesis. Blood 2010;116:4754–61.