4.2 Article

Differential effects of basolateral and apical iron supply on iron transport in Caco-2 cells

Journal

GENES AND NUTRITION
Volume 10, Issue 3, Pages -

Publisher

BMC
DOI: 10.1007/s12263-015-0463-5

Keywords

Iron uptake; Iron transport; Iron metabolism; Iron homeostasis; Gene expression; Intestinal epithelium

Funding

  1. Biotechnology and Biological Sciences Research Council (Institute core strategic grant)
  2. NuGO (The European Nutrigenomics Organization: linking genomics, nutrition and health research), a Network of Excellence - European Commission's Research Directorate General under Priority [CT-2004-505944]

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Iron homeostasis in the human body is maintained primarily through regulation of iron absorption in the duodenum. The liver peptide hepcidin plays a central role in this regulation. Additionally, expression and functional control of certain components of the cellular iron transport machinery can be influenced directly by the iron status of enterocytes. The significance of this modulation, relative to the effects of hepcidin, and the comparative effects of iron obtained directly from the diet and/or via the bloodstream are not clear. The studies described here were performed using Caco-2 cell monolayers as a model of intestinal epithelium, to compare the effects of iron supplied in physiologically relevant forms to either the apical or basolateral surfaces of the cells. Both sources of iron provoked increased cellular ferritin content, indicating iron uptake from both sides of the cells. Supply of basolateral transferrin-bound iron did not affect subsequent iron transport across the apical surface, but reduced iron transport across the basolateral membrane. In contrast, the apical iron supply led to subsequent reduction in iron transport across the apical cell membrane without altering iron export across the basolateral membrane. The apical and basolateral iron supplies also elicited distinct effects on the expression and subcellular distribution of iron transporters. These data suggest that, in addition to the effects of cellular iron status on the expression of iron transporter genes, different modes and direction of iron supply to enterocytes can elicit distinct functional effects on iron transport.

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