Biol Res 39: 79-85, 2006

DMT1: Which metals does it transport?

MICHAEL D GARRICK^1,2, STEVEN T SINGLETON¹, FARIDA VARGAS¹, H-C KUO^*1, LIN ZHAO¹, MARTIN KNÖPFEL³, TODD DAVIDSON⁴, MAX COSTA⁴, PRASAD PARADKAR⁵, JEROME A ROTH⁵ and LAURA M GARRICK^1,6

Departments of ¹Biochemistry, ²Pediatrics, ⁵Pharmacology & Toxicology and ⁶Medicine, SUNY at Buffalo, Buffalo, NY, USA
³Tracechem, Berne, Switzerland
⁴Nelson Institute of Environmental Medicine, New York University, Tuxedo, NY, USA

Dirección para Correspondencia

ABSTRACT

DMT1 _ Divalent Metal (Ion) Transporter 1 or SLC11A2/DCT1/Nramp2 _ transports Fe²⁺ into the duodenum and out of the endosome during the transferrin cycle. DMT1 also is important in non-transferrin bound iron uptake. It plays similar roles in Mn²⁺ trafficking. Voltage clamping showed that six other metals evoked currents, but it is unclear if these metals are substrates for DMT1. This report summarizes progress on which metals DMT1 transports, focusing on results from the authors' labs. We recently cloned 1A/+IRE and 2/-IRE DMT1 isoforms to generate HEK293 cell lines that express them in a tetracycline-inducible fashion, then compared induced expression to uninduced expression and to endogenous DMT1 expression. Induced expression increases ~50x over endogenous expression and ~10x over uninduced levels. Fe²⁺, Mn²⁺, Ni²⁺ and Cu¹⁺ or Cu²⁺ are transported. We also explored competition between metal ions using this system because incorporation essentially represents DMT1 transport and find this order for transport affinity: Mn>?Cd>?Fe>Pb~Co~Ni>Zn. The effects of decreased DMT1 also could be examined. The Belgrade rat has diminished DMT1 function and thus provides ways of testing. A series of DNA constructs that generate siRNAs specific for DMT1 or certain DMT1 isoforms yield another way to test DMT1-based transport.

Key terms: Metal ion transport; DCT1, Nramp2 or SLC11A2; expression assay: competition between metal ions

INTRODUCTION

DMT1 _ Divalent Metal (Ion) Transporter 1 or SLC11A2 (OMIM's designation for solute carrier family 11 member 2) / DCT1 (Divalent Cation Transporter 1) / Nramp2 (Natural resistance associated macrophage protein 2) _ definitely transports Fe²⁺ as part of both nutritional acquisition in the duodenum and exit from the endosome during the transferrin cycle (for reviews, see Garrick et al., 2003, and Garrick and Garrick, 2004). In addition to these two functions, DMT1 is likely to be important in non-transferrin bound iron uptake. The transporter probably plays similar roles in Mn²⁺ trafficking (for a review, see Roth and Garrick, 2003). Data from two-electrode voltage clamping studies (Gunshin et al., 1997) showed that six other metals evoked currents, but it is not clear if these metals are substrates for DMT1.

METHODS

Most of the methods were described recently (Kuo et al., 2004). The competition assays relied on incubating HEK293 cells containing one of the following two constructs: mouse 2/-IRE or rat 1A/+IRE (each with a strong cytomegalovirus promoter under tetracycline control and a tetracycline response element) in the presence or absence of 50 nM doxycycline for 24 hr. DMT1 expression (detected by uptake of Fe²⁺ or Mn²⁺) was ~50x endogenous levels after such induction or ~5x endogenous levels without such induction; hence uptake represented ≥98% or ≥80% DMT1 expression, respectively. When ⁵⁹Fe²⁺ was the substrate, its concentration was 100 nM; for ⁵⁴Mn²⁺ the concentration was 10 nM. Incubations were for 10 or 15 min in the presence of selected concentrations of competing metal ion, so that the initial velocity for uptake was measured. Statistical treatment of the data relied on linear regression analyses using Stata (StataCorp, College Station, TX). Additional details of the data reduction are described in the results to allow the reader to visualize how this was accomplished.

RESULTS

Competition between known substrates and candidates does not inform us as to whether the candidate is actually a substrate, but does reveal whether the candidate metal ion interacts with the transporter. An example is shown in figure 1, where Pb²⁺ (from lead acetate) inhibits Mn²⁺ uptake. Although there were four conditions for the incubations, the results could be combined to calculate an IC₅₀ (Inhibitor Concentration that yields 50% of control) of 7.3 μM. It was desirable to have a quicker and less subjective method to get this value, so we relied on the observation that there appears to be a linear relation for the three series of percents over the concentration range 1-100 μM and calculated the IC₅₀ by linear regression analysis, obtaining an estimate of 8.5 μM with R² = 0.88. Similar calculations for an analysis of FeSO₄ inhibition of Mn²⁺ uptake gave an estimate of 2.0 μM for that IC₅₀ with R² = 0.90 while the graphical estimate was 2.1 μM for the IC₅₀. Linear regression analysis over the log/linear range therefore was applied to a series of analyses like figure 1 to get the data shown in table 1. The R² ranged from 0.77 to 0.95 indicating that ~77 to ~95 % of the variation in the scatter is due to the linear relationship.

Figure 1. Inhibition of Mn uptake by Pb. Cells were incubated with 54Mn2+ and selected concentrations of lead acetate [Pb(CH3COO)2] with () and without () doxycycline for the 2/-IRE () and 1A/+IRE () lines. Although induced incorporation in the presence of doxycycline was ~10x that without induction, the incubations without Pb were treated as 100% uptake for each series to allow comparison. We fitted the concentration response with a single cubic spline because the 4 series of competitions were indistinguishable. Dropping a line from the 50 % level yielded an IC50 at 7.3 μM.

The data in table 1 indicate that there is generally satisfactory agreement between separate experiments when the same uptake is blocked by the same inhibitor, but there is a discrepancy when the uptake of Mn is compared to that for Fe. For examples, CoCl₂ has similar IC₅₀s of 87.6 and 80.2 when blocking ⁵⁹Fe²⁺ uptake; but the IC₅₀s of 8.3 and 6.4 when blocking ⁵⁴Mn²⁺ uptake, although similar to each other, are more than 10x less. CdCl₂ exhibits similar behavior but at a lower concentration. We consider the likely explanation in the discussion section that follows. The only exception to this observation is that ZnSO₄ gives less reproducibility and that there is not so great a difference between its ability to block Fe and Mn uptake. These issues could relate to its being the least effective inhibitor. Although a number of metal ions remain to be studied, these data and data that show the K_m to be ~1 mM for Mn²⁺ and ~3 mM for Fe²⁺ (Garrick et al., 2005, unpublished data) permit the following rankings for transport affinity of the metal ions: Mn²⁺>?Cd²⁺>?Fe²⁺ >Pb²⁺~Co²⁺~Ni²⁺ >Zn²⁺.

DISCUSSION

Competition

It was initially puzzling that the IC₅₀ for CdCl₂ was lower when it competed with Mn than when it competed with Fe and that a similar relationship occurred for CoCl₂. One expected the K_i for DMT1 to be the same with CdCl₂, independent of the substrate transported. An IC₅₀ is not,however, a K_i. Their relationship was defined by Cheng and Prusoff (1973) as shown below in Equation 1.

where [L] is the substrate (ligand) concentration and K_D is the dissociation constant.

The arrangement in Equation 2 below aids us in viewing the influence of these variables.

Although the K_Ds for Fe and Mn are unknown, the K_ms are ~3 and ~1 μM (Garrick et al., 2005, unpublished data). If the ratios of the K_Ds is similar, and the K_D for each is < [L], then the ratio of the substrate concentrations will affect the relative IC₅₀ values. The ~10x difference that we see reflects the ratio [Fe]/[Mn] (= 10) closely, so we suspect that the weights of [L] and different K_Ds account for our observation.

The Belgrade (b/b) rat

Because G185R mutated DMT1 is clearly defective, preparations from b/b rats provide an opportunity to learn more about the role of the transporter. Knöpfel et al. (2005b) used vesicles prepared from duodenal brush border membranes (BBM) to investigate how a calcein-based fluorescence quenching assay performed when the vesicles' DMT1 was defective. The assay had been developed earlier but used only on normal rabbit BBM. The results indicated that defective b/b DMT1 in BBM failed to transport Ni²⁺, Fe²⁺ and Mn²⁺, while BBM from +/b rats transported all three divalent metal ions successfully. The data therefore provided confirmation that b/b DMT1 is defective and evidence that normal DMT1 transports the three metal ions. Their observation that vesicles from +/b basolateral membranes (BLM) also had vigorous transport, while those from b/b BLM did not, is evidence that DMT1 also may serve functions in enterocytes at other locations than the apical surface.

Current status

The issue of which metals DMT1 transports remains a topic for intensive investigation. This report suggests the following order for DMT1 transport affinities: Mn>?Cd>?Fe>Pb~Co~Ni>Zn with some uncertainty on where to place Cu. One should keep in mind, however, that binding to DMT1 is only one of many factors that will determine the ultimate physiological and toxicological effects. Other metal-binding proteins and targets will play downstream roles and each may have alternative transporters. Keeping these caveats in mind, some conclusions are outlined below.

Fe²⁺ is definitely a substrate in which there is no question that DMT1's role is physiologically significant. One would like to know what other pathways for iron entry into cells and exit from endosomes exist, their relative contributions and what species of iron they involve. The same conclusion applies to Mn²⁺, but even less is known about alternative pathways and their relative impact.

DMT1 clearly can transport Cu, but whether the ionic form is cuprous or cupric is less certain. Other transporters clearly exist for this metal's ion(s), and the physiological role for DMT1 is still uncertain. Co is clearly a substrate, but the physiological significance of this observation needs additional elaboration; Zn may be a substrate but also deserves more study. There are clearly alternative transporters for Zn which begs the question of whether DMT1 plays much of a role physiologically, given the high concentration of Zn²⁺ needed for the IC₅₀ and the total serum concentration of Zn of ~12-17 μM.

DMT1-mediated uptake of Ni is probably toxicologically relevant, but here too, more data are desirable. Cd binds tightly to DMT1 and earlier studies (reviewed in Garrick et al., 2003) leave little doubt that DMT1 actually transports this metal. Such transport also is probably relevant toxicologically. Pb may be transported by DMT1 as well (also

ACKNOWLEDGMENTS

The research results reported or described here received support from NIH grants # DK59794 (LMG), ES11127 (JAR), ES00260 (MC), ES10344 (MC), 808 T32-ES07324 (MC) and a grant FP-91641801-0 from the Environmental Protection Agency (TD) plus a grant from the National Research Initiative of the USDA Cooperative State Research, Education and Extension Service, 2001-35200-10723 (MDG).

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Corresponding author: Michael D. Garrick, Department of Biochemistry, SUNY, 140 Farber Hall, Buffalo, NY 14214, USA, Tel.: (1-716) 829-3926, Fax: (1-716) 829-2725, E-mail: mgarrick@buffalo.edu

Received: April 4, 2005. Accepted: May 3, 2005.