Abstract
BackgroundIron is essential for the maintenance of basic cellular processes. In the regulation of its cellular levels, ferritin acts as the main intracellular iron storage protein. In this work we present a mathematical model for the dynamics of iron storage in ferritin during the process of intestinal iron absorption. A set of differential equations were established considering kinetic expressions for the main reactions and mass balances for ferritin, iron and a discrete population of ferritin species defined by their respective iron content.ResultsSimulation results showing the evolution of ferritin iron content following a pulse of iron were compared with experimental data for ferritin iron distribution obtained with purified ferritin incubated in vitro with different iron levels. Distinctive features observed experimentally were successfully captured by the model, namely the distribution pattern of iron into ferritin protein nanocages with different iron content and the role of ferritin as a controller of the cytosolic labile iron pool (cLIP). Ferritin stabilizes the cLIP for a wide range of total intracellular iron concentrations, but the model predicts an exponential increment of the cLIP at an iron content > 2,500 Fe/ferritin protein cage, when the storage capacity of ferritin is exceeded.ConclusionsThe results presented support the role of ferritin as an iron buffer in a cellular system. Moreover, the model predicts desirable characteristics for a buffer protein such as effective removal of excess iron, which keeps intracellular cLIP levels approximately constant even when large perturbations are introduced, and a freely available source of iron under iron starvation. In addition, the simulated dynamics of the iron removal process are extremely fast, with ferritin acting as a first defense against dangerous iron fluctuations and providing the time required by the cell to activate slower transcriptional regulation mechanisms and adapt to iron stress conditions. In summary, the model captures the complexity of the iron-ferritin equilibrium, and can be used for further theoretical exploration of the role of ferritin in the regulation of intracellular labile iron levels and, in particular, as a relevant regulator of transepithelial iron transport during the process of intestinal iron absorption.
Highlights
Iron is essential for the maintenance of basic cellular processes
Steady states The kinetic mathematical model was initially tested for its ability to recover the experimental steady states of iron load distribution in ferritin protein cages
A mathematical model based on the structure/function of ferritin protein nanocages and purely kinetic considerations about the mineralization/dissolution of the ferritin iron mineral core was proposed to elucidate functional characteristics of the dynamic behavior of ferritin in vitro and in vivo
Summary
Iron is essential for the maintenance of basic cellular processes. In the regulation of its cellular levels, ferritin acts as the main intracellular iron storage protein. In this work we present a mathematical model for the dynamics of iron storage in ferritin during the process of intestinal iron absorption. The maintenance of body iron homeostasis is the result of a delicate balance between intestinal absorption and obligatory losses. Intestinal iron absorption is divided into three steps, named the uptake, intracellular and transfer phases. From the cLIP, iron is either transported into the blood circulation by ferroportin or distributed to mitochondria, ferritin and other iron-requiring proteins. Poly (rC)-binding protein 1 (PCBP1) was reported as a putative iron chaperone capable of delivering cytosolic iron to ferritin [11]
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