Abstract
Hinokitiol, a natural lipophilic chelator, appears capable of replacing several iron transporters after they have been genetically ablated. Divalent metal-ion transporter (DMT1) is the major iron importer in enterocytes and erythroblasts. We have compared DMT1 and hinokitiol in multiple fashions to learn if the smaller molecule is a suitable substitute using two HEK293 cell lines engineered to overexpress different isoforms of DMT1. Both the macromolecule and the lipophilic chelator enable import of ferrous ions into HEK293 cells. Hinokitiol also mediates ferric ion import but DMT1 cannot do so. While DMT1 can also import Mn2+ ions, hinokitiol lacks this ability. The Michaelis–Menten analysis for kinetics of macromolecular catalysis is also suitable for hinokitiol-supported iron import. To compare hinokitiol to DMT1 relative to other metal ions that DMT1 can transport, we employed an organic extraction procedure with which we initially matched the results obtained for Fe2+, Fe3+ and Mn2+, and then showed that multiple other cations were unlikely to enter via hinokitiol. The small chelator thus shares some functional properties with DMT1, but distinct difference were also noted.
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A recent, ingenious proposal (Grillo et al. 2017) argues that small molecule replacement is a potential therapeutic modality when genetic defects eliminate catalytic or transport activity of proteins to obstruct a step in a metabolic pathway. This proposal opens an alternative to gene therapy with the authors suggesting that a natural product that acts as an iron chelator, hinokitiol, can potentially substitute for several iron transporters.
The specific rationale (Grillo et al. 2017) for the Burke group’s use of hinokitiol was “Deficiencies of passive ion-transport proteins cause many human diseases … “(yet) “the corresponding active ion-transport proteins typically remain functional,” (so) “there may be a buildup of ion gradients upstream of the membranes that normally host these missing proteins.” They argued that a smaller molecule like hinokitiol could serve as a channel to relieve this buildup. Their paper supported this rationale by showing that hinokitiol could substitute for divalent metal-ion transporter (DMT1) and other iron transport proteins when they were deficient.
Over-expression of DMT1 in HEK293 cells (Garrick et al. 2006a) could be recast in similar terms because we had originally selected HEK293 cells for having very low iron-transport activity thus implying modest endogenous DMT1 expression. We then stably transfected the cells to create 2 cell lines representing all 4 of the N- and C-termini of DMT1 isoforms and subject to doxycycline inducible over-expression. Two major DMT1 mRNA isoforms vary by starting in exons 1A or 1B; the protein encoded by the former has its N-terminus extended to include exon 1A while the latter does not get translated so its N-terminus starts in exon 2. Two other isoform variants depend on whether poly-A attaches after exon 16 or 17; the 3′ UTR of exon 16 includes an iron responsive element (IRE) but the IRE is absent when exon 17 is present. Although IREs are stem loop structures in mRNA, the respective distinct protein C-termini receive designations: +IRE or –IRE, respectively. Having cells that would overexpress 1A/+ IRE DMT1 or 1B/− IRE DMT1 in a regulated fashion allowed us to characterize the DMT1 isoforms functionally and kinetically. In addition, this approach enabled us to learn more about other metal ions that DMT1 transports (Arredondo et al. 2014; Davidson et al. 2005; Garrick et al. 2003, 2006a, b; Jiang et al. 2013; Roth and Garrick 2003), largely confirming earlier suspicions based on induced currents (Gunshin et al. 1997). This promiscuity was also established by direct measurements subsequently (Illing et al. 2012). Some metal ions like Cu1+ remain controversial. These results also lead one to wonder about whether kinetic analyses leading to a Michaelis constant (Km) could be applied to hinokitiol and what other metal ions could rely on hinokitiol to gain entry.
If one advocates using hinokitiol to replace defective DMT1, then a direct comparison of functioning DMT1 and hinokitiol needs to be made. We set out to do so for the most physiologically relevant metal ion, Fe2+ as well as Fe3+ (the main dietary form of nonheme iron). This study asks how well hinokitiol recapitulates iron transporter(s) (here DMT1) for which it could be substituted. So issues are for which metal ion gradients can the smaller molecule allow entry into cells and how well can the Km concept apply to it.
Results
Import assay comparisons
Figure 1 compares uptake of ferrous ions by HEK293 cells for a series of situations that illustrate how DMT1 can release an external/internal concentration gradient to generate cellular uptake and that hinokitiol is effective in the same conditions whereas C2deoxyhinokitiol (C2d, an inactive control for hinokitiol) is ineffective. This effectiveness demonstrates that hinokitiol can replace DMT1 for import of ferrous iron.
Results similar to Fig. 1 were obtained with HEK293 cells capable of expressing mouse 1B/− IRE DMT1 (not shown). Our results with hinokitiol confirm and extend those obtained by Grillo et al. (2017), supporting hinokitiol as a potential treatment modality for DMT1 deficiency and the concentration gradient rationale offered. DMT1 fails to transport Fe3+ unless supported by a ferrireductase to convert it to Fe2+ (Conrad et al. 2000; Fleming et al. 1998; Mackenzie and Garrick 2005), whereas hinokitiol enables Fe3+ entry (Grillo et al. 2017). We tested Fe3+ entry in this HEK293 system (Fig. 2).
The ordinate for Fig. 1 is × 7.5 greater than that for Fig. 2 to allow coverage of the increased expression of DMT1 in the former; so one should recognize that hinokitiol actually imports Fe2+ faster than Fe3+. Similar results were obtained with HEK293 cells capable of expressing rat 1A/+ IRE DMT1. The results with hinokitiol confirm and extend those obtained by Grillo and colleagues (Grillo et al. 2017) to indicate that hinokitiol can enable the import of iron in its ferric form whereas DMT1 does not do so (Conrad et al. 2000). Nevertheless, the import is faster with ferrous ions as they had also noted after incorporating hinokitiol into liposomes (Grillo et al. 2017). Because DMT1 supports uptake of Mn2+, we then also tested whether hinokitiol did so as well (Fig. 3).
Results similar to Fig. 3 were obtained with HEK293 cells capable of expressing rat 1A/+ IRE DMT1. The results with hinokitiol confirm and extend those obtained before (Grillo et al. 2017) to indicate that hinokitiol does not enable Mn2+ import. Although it is clear that hinokitiol can rely on concentration gradients of external/internal Fe2+, its behavior is clearly distinct in this role from that of DMT1 because DMT1 can similarly import Mn2+ based on concentration gradients of external/internal Mn2+, gradients that are not utilized by hinokitiol. Moreover, hinokitiol directly permits Fe3+ import while DMT1 does not.
Kinetics for transport by hinokitiol
Transporters like DMT1 act as macromolecular catalysts similar to enzymes. As such they follow Michaelis–Menten kinetics (Eq. 1) (Michaelis and Menten 1913).
where E = enzyme (or transporter for this analysis); S = substrate (here, extracellular Fe); ES = enzyme/substrate complex; P = product (here, intracellular Fe) and rate constants kf, kr and kcat are assigned to the forward and reverse reactions plus to conversion to P, respectively.
Equation 1 is usually analyzed further
where v = the initial velocity for formation of product; Vmax = the maximal velocity and Km = (kr + kcat)/kf. This result assumes that [S] > [E] so that one sees a saturable process but the left hand side of Eq. 1 is symmetrical in E and S.
This property of transporters encouraged us to compare hinokitiol head-to-head to DMT1 in such an assay of transport or catalysis as one can argue that the concentration response to Fe2+ for a channel like hinokitiol could also follow Michaelis–Menten kinetics. We therefore examined this response for hinokitiol with time dependency graphs like those in Fig. 1 as the basis for the initial velocity in each point (Fig. 4). Prior to being able to use nonlinear least squares fits to estimate Km and Vmax, various transformations were used to linearize the graphs of which the classical approach (Lineweaver and Burk 1934) takes the reciprocals of both sides of Eq. 2 to give a linear result:
Supplementary Fig. S1 shows a Lineweaver–Burk plot for the same data with an acceptable linear fit. The differences in the estimates for Km (242 vs 455) and Vmax (3.5 vs 4.3) are mostly attributable to the inverse weighting in a reciprocal plot so we chose to use the latter two values in Table 1. The fit to Michaelis–Menten kinetics (Fig. 4) for 1000 nM hinokitiol as a catalyst is suitable even though the [S] values are in a range comparable to those for [E] so we used the same approach to ascertain the Km and the Vmax when 500 nM hinokitiol was present and [Fe2+] was varied (Table 1) and obtained an essentially identical Km while the Vmax was essentially halved. We also applied this approach to analyses for Fe3+ entry (Table 1) and observed that hinokitiol had a decreased apparent affinity for it but allowed more rapid entry. In contrast, the Burke group found by more direct measurements that the affinity for Fe(III) was much higher than for Fe(II) (Grillo et al. 2017). Noting that the left side of Eq. 1 is symmetrical in E and S, we tested if hinokitiol (E) could also be evaluated by this approach (Table 1) and obtained kinetic parameters again.
The results with hinokitiol extend those obtained by Grillo et al. (2017), demonstrating that this small molecule can substitute for DMT1 for Fe2+ entry into cells provided that there is a concentration gradient of the substrate across the plasma membrane. They also show that saturable kinetics apply to using hinokitiol in place of DMT1 with Fe2+ entry into cells. Hinokitiol can also do this for Fe3+ entry unaided whereas DMT1 requires reduction of the substrate prior to entry and again a Km analysis is applicable. Remarkably, one can also hold the initial concentration of ferrous or ferric ions constant, vary the hinokitiol concentration and fit the results to Michaelis–Menten kinetics. The saturable behavior could be due to the symmetry of E and S on the left hand side of Eq. 1 or to the solubility of hinokitiol in the relevant membrane (here the plasma membrane).
Assessing hinokitiol’s chelation of metal ions
It is also important to learn how hinokitiol interacts with other metal ions, given their physiological and toxicological implications. Rather than develop assays for radioactively tagged metal ions, we adapted another assay. Grillo et al. (2017) also showed that hinokitiol is able to partition metal ions into a lipid layer after chelating them. We used this assay to verify our results with Fe and Mn ions paralleled the data on import of these metal ions, then extended it to using other metal ions. Figure 5 illustrates results for 59Fe2+, 59Fe3+ and 54Mn2+ analyses.
These results with hinokitiol also confirm and extend those obtained by Grillo et al. (2017) showing that ferrous (Fig. 5a) and ferric (Fig. 5b) iron both bind to hinokitiol rendering the iron able to partition to the organic phase. Consistent with more effective import by hinokitiol of ferrous (Fig. 1c) than ferric (Fig. 2c but note the y-scale) iron, ferric iron extracts less well after binding to hinokitiol. Based on the transport results, one might also expect that hinokitiol does not chelate Mn2+ without an excess of the chelator so that it will not appear in the organic phase. This expectation was tested and met (Fig. 5c).
Because of the regulatory complexity of working with radioisotopes for the other metals of interest, we chose to modify this extraction assay to have the results ascertained via inductively coupled plasma-optical emission spectrometry (ICP-OES). First, however, we examined the concentration dependence in the assay above to assure that the higher concentrations needed for ICP-OES should produce interpretable results. Supplementary Fig. S2 portrays these analyses with the data indicating that C2d binds neither ferrous (S2a) nor ferric (S2b) ions consistent with Figs. 1b and 2b, respectively, where the control does not support their import. Fig. S2 shows that hinokitiol, however, does bind the two ions with ferrous (S2a) clearly associating more effectively than ferric (S2b), consistent with the Km results in Table 1.
The next experiments tested whether the results for ICP-OES were equivalent to those with radioisotope tags for the three metal ions already examined. Supplementary Fig. S3 illustrates results for Fe2+ analysis. The bar graph like Fig. 5a supports the distinction between hinokitiol as chelating ferrous ions and allowing their extraction into an organic phase versus the negative control that does not chelate them is a property that reproduces over at least a 5000-fold range of Fe2+ concentrations. We surveyed some of the metals ultimately tested at this level (10 µEq/L with 20 µM hinokitiol) and were usually unable to detect partitioning (data not shown). Because the Burke group found that they had to use higher, non-physiological concentrations of most other metals, we also tested similar high levels; data for Cd2+ are representative (Supplementary Fig. S4). The results show that statistically significant amounts of this toxic ion appear in the organic phase when hinokitiol is present; but the actual quantity is close to minimal. These data are summarized in Table 2 as also are similar data for Pb2+; they indicate that accumulation of toxic levels of either metal ion due to hinokitiol substituting for DMT1 is not a likely problem.
These results with hinokitiol also confirm and extend those obtained by Grillo et al. (2017). The portion of 59Fe2+ that is extracted with C2d is 0; while with hinokitiol it is 34.7 ± 0.5% (Table 2). These results illustrate the properties of hinokitiol that permit it to substitute for DMT1 in ferrous ion import. One might also expect that hinokitiol must chelate Fe3+ so that it too will appear in the organic phase. This expectation was tested in a similar fashion; again the control does not lead to any counts in the organic phase while hinokitiol retrieves 11.0 ± 0.5% (Table 2). Mn is clearly not transported nor is it extracted (Table 2) until non-physiological levels are present. Whereas DMT1 imports multiple other metal ions of physiological or toxicological relevance and has also been tested for other ions that remain controversial, Table 2 indicates that substituting hinokitiol for DMT1 is unlikely to cause import any of these ions to an extent that will ordinarily impact their metabolic behavior.
Discussion
Can hinokitiol substitute for DMT1 and does that ability depend on a ferrous ion concentration gradient?
The initial premise for this project was that an ion gradient generated to reveal DMT1 activity would also reveal the ability of hinokitiol to import that ion, here Fe2+. Initial support for that premise came from how well the small molecule substituted for the major iron importer when conditions were chosen to assess DMT1 activity (Fig. 1). Given that hinokitiol alleviates the anemia of the Belgrade rat (Grillo et al. 2017) and that the anemia derives from a G185R mutation in DMT1 (Fleming et al. 1998), this result is not surprising but its novelty depends on the gradient here coming from experimental intervention rather than the mutational loss of the gene product. The next experiments compared some of the ions with which the transporter and the small molecule interacted.
Metal ion interactions, round 1
While hinokitiol binds to and supports the import of ferric ions, DMT1 does not (Fig. 2). This result is a reminder that nearly two decades have passed since clear published results showed that there were separate pathways for ferrous and ferric iron import (Conrad et al. 2000), yet only the path for the former has seen more publications to elaborate on it. The participants in the latter pathway remain largely uncharacterized except to the extent that multiple ferrireductases that divert Fe3+ into the Fe2+ pathway are now known (McKie et al. 2001; Ohgami et al. 2006; Tripathi et al. 2015). Hinokitiol, however, can import Fe3+ without prior reduction.
The situation is also different for Mn2+ (Fig. 3) with DMT1 effectively importing this metal ion, but hinokitol unable to do so until the level of Mn2+ (Table 2) is far above what is physiological. The potential for DMT1 to transport Mn in addition to iron was initially noted in the study that led to the acronym DCT1 (Gunshin et al. 1997)—for divalent cation-transporter 1—but it soon generated a better appreciation for how iron and manganese metabolism interact in both physiological and toxic fashions (Roth and Garrick 2003). One would therefore not expect hinokitiol to have a direct impact on these interactions in the ways that DMT1 does.
Transport kinetics
The original treatment of Eq. 2 (Michaelis and Menten 1913) relied on the assumption that [S] ≫ [E] so that one could use the input concentration of S as [S]. If, however, one considers that the activities of S and E are the more chemically appropriate values, this treatment might still apply [as well as the linearization in Eq. 3 (Lineweaver and Burk 1934)] despite our using concentrations of hinokitiol not much below the range (~ 3–4 μM) of the Km for DMT1. We chose therefore to find out whether similar saturation curves and linearizations were the result for varying [Fe2+], asking if they were similar to those for DMT1 (Garrick et al. 2006a). They were (Fig. 4, Supplementary Fig. S1) and the Km’s (Table 1) even indicated that hinokitiol had a higher affinity for Fe2+ by nearly an order of magnitude. We also then did similar analyses for Fe3+ to find that the affinity of hinokitiol for these ions was × ~ 5 less (Table 2). Because it was easy to vary the level of the hinokitiol, we also did Km studies for it. We again observed a saturable process (Table 2). It is beyond the scope of the current paper to address whether the process was due to limiting constant quantities of the substrate or another component of the system like the ability to solubilize hinokitiol in the plasma membrane. It is novel to find that this type of kinetic analysis can be applied to a small molecule substituting for the transporter and hence inverted between the catalyst and the reactant.
Metal ion interactions, round 2
There have been many studies showing that DMT1 is relatively promiscuous in terms of which metal ions it can transport (Arredondo et al. 2003, 2014; Bannon et al. 2002, 2003; Davidson et al. 2005; Garrick et al. 2003, 2006a, b; Gunshin et al. 1997; Illing et al. 2012; Jiang et al. 2013; Knöpfel et al. 2005; Roth and Garrick 2003) while dysfunction after mutation implies it serves iron homeostasis primarily (Fleming et al. 1997, 1998; Gunshin et al. 2005). The consensus adds Cd2+, Mn2+, Co2+, Ni2+, Pb2+, VO2+ and Zn2+ to the metal ions it can transport, while excluding Fe3+ and Cu2+. Cu1+ has seen some debate but current support looks sufficient (Arredondo et al. 2003, 2014; Jiang et al. 2013). Clearly this promiscuity indicates that DMT1 not only serves iron import but also involves some toxic risks and may support other metal ion transporters by providing some redundancy to exploit. We therefore asked if hinokitiol was similarly promiscuous. To screen the variety of cations, we verified that the combination of lipophilicity and chelation as properties of hinokitiol (Grillo et al. 2017) to which the Burke lab attributed its ability to substitute for DMT1 did parallel our positive metal ion import results with radioisotope tagged Fe2+ and Fe3+ (Fig. 5, Supplementary Fig. S2) and the negative results with Mn2+ (Fig. 5). Adopting a variation of the assay relying on ICP-OES, we still saw consistency with the Fe data (Supplementary Fig. S3) and established that hinokitiol works, but minimally for the toxic metal ion, Cd2+ (Supplementary Fig. S4). To the extent that one can rely on this partition assay, our data do not support physiological transport of the other metal ions tested in Table 2. Thus we conclude that hinokitiol has a narrower substrate specificity than DMT1, a property that may be an advantage in terms of interacting with the homeostasis of these metal ions and particularly in terms of not importing toxic metals like Cd and Pb. Hinokitiol’s ability to import Fe3+ could pose an issue relative to iron overload but clearly Fe2+ import by hinokitiol is more effective than for Fe3+ so a little caution in monitoring iron status while using hinokitiol appears to be what this property calls for rather than excluding the use of hinokitiol.
Conclusions
Hinokitiol relies as predicted on concentration gradients of Fe2+ and Fe3+ similar to those needed to assay for DMT1 or those generated when DMT1 deficiency exists. Because hinokitiol is serving in the place of a transporter, the same type of kinetic analyses that apply to transporter kinetics also serve to describe metal ion import dependent on hinokitiol. Hinokitiol is less promiscuous in interacting with metal ions than DMT1; this property should help in determining whether the smaller molecule can be used as a gene therapy replacement for genes involved in iron homeostasis like SLC11A2.
Materials and methods
Materials
59FeCl3 (NEZ0375) and 54MnCl2 (NEZ040) were purchased from Perkin Elmer (Boston, MA) supplied in 0.5 M HCl. Hinokitiol and C2doxyhinokitiol were synthesized in the Burke laboratory as described (Grillo et al. 2017). HEK293 cells permanently transfected with 1A/+ IRE or 1B/− IRE DMT1 subject to tet-on regulation have been described (Garrick et al. 2006a).
Incubations
Briefly, HEK293 cells were grown to 70–80% confluence in 6 well plates then treated with doxycycline (when DMT1 activity was the goal) or just its solvent (when endogenous transport was the goal) then grown fully to confluence (24–48 h) all as described before (Garrick et al. 2006a). Incubations also included 500 nM hinokitiol or C2d for the periods indicated and 59Fe2+, 59Fe3+ or 54Mn2+ with the labeling conditions also all as described before (Garrick et al. 2006a). When determining the kinetics, we varied either the iron concentration or the hinokitiol concentration while holding the hinokitiol or the iron concentration constant, respectively, as indicated in the figure or table legends.
Extractions
For 59Fe experiments, [Fe] = 200 nEq/L in Hank’s Buffered Saline Solution (HBSS) unless otherwise specified; while hinokitiol and C2d were 500 nM. As iron binding of hinokitiol is tridentate, the concentrations chosen provided a modest excess of Fe. When Fe2+ was present, this status was achieved by having a × 10 excess of FeSO4 relative to the 59Fe and a × 10 excess of ascorbic acid relative to the FeSO4. When Fe3+was present, this status was achieved by having a × 10 excess of ferric ammonium citrate (FAC) present relative to the 59Fe. For 54Mn experiments, [Mn] = 350 nEq/L was achieved by adding MnCl2. All extractions involved 1 mL for the aqueous phase and an equal volume of hexane. Tubes were vortexed at low speed, allowed to settle and aliquots of the two phases removed and allowed to dry in a fume hood then counted in a LKB Compugamma 1282 γ counter.
For nonradioactive experiments, the metals were at 10 or 100 μEq/L in HBSS; while hinokitiol and C2d were 20 or 200 μM, respectively, leading to a slightly larger excess of metal ion than in the radioactive extractions. Metals were provided as FeSO4 (with a × 10 excess of ascorbate), FAC, MnCl2, Pb(CH3CO2)2, Cd(CH3CO2)2, CoCl2, NiCl2, VOSO4, Cu(CH3CO2)2 with a × 10 excess of histidine, Zn(CH3CO2)2 and CuSO4 with both histidine and ascorbate in × 10 excess. Extractions were performed as above but metals were determined using ICP-OES (Model Optima 4300D, Perkin Elmer, Norwalk, CT) after drying the two phases in a fume hood and dissolving an aliquot of each in 3 N HCl/10% trichloracetic acid.
Statistical analysis
Statistical analysis were done with Stata version 15.1 (StataCorp, College Station, TX). Although P < 0.05 was treated as significant, we report P where possible. We used no correction for multiple statistical tests when making them because we tested only experimental hypotheses but readers should be aware that this approach was employed.
References
Arredondo M, Munoz P, Mura CV, Nuñez MT (2003) DMT1, a physiologically relevant apical Cu1+ transporter of intestinal cells. Am J Physiol Cell Physiol 284:C1525–C1530
Arredondo M, Mendiburo M, Flores S, Singleton S, Garrick M (2014) Mouse divalent metal transporter 1 is a copper transporter in HEK293 cells. Biometals 27:115–123. https://doi.org/10.1007/s10534-013-9691-6
Bannon DI, Portnoy ME, Olivi L, Lees P, Culotta VC, Bressler JP (2002) Uptake of lead and iron by divalent metal transporter 1 in yeast and mammalian cells. Biochem Biophys Res Commun 295:978–984
Bannon DI, Abounader R, Lees P, Bressler JP (2003) Effect of DMT1 knockdown on iron, cadmium, and lead uptake in Caco-2 cells. Am J Physiol Cell Physiol 284:C44–C50
Conrad ME et al (2000) Separate pathways for cellular uptake of ferric and ferrous iron. Am J Physiol Gastrointest Liver Physiol 279:G767–G774
Davidson T, Chen H, Garrick MD, D’Angelo G, Costa M (2005) Soluble nickel interferes with cellular iron homeostasis. Mol Cell Biochem 279:157–162
Fleming MD, Trenor CI, Su MA, Foernzler D, Beier DR, Dietrich WF, Andrews NC (1997) Microcytic anaemia mice have a mutation in Nramp2, a candidate iron transporter gene. Nat Genet 16:383–386
Fleming MD, Romano MA, Su MA, Garrick LM, Garrick MD, Andrews NC (1998) Nramp2 is mutated in the anemic Belgrade (b) rat: evidence of a role for Nramp2 in endosomal iron transport. Proc Natl Acad Sci USA 95:1148–1153
Garrick MD et al (2003) DMT1 (divalent metal transporter 1): a mammalian transporter for multiple metals. Biometals 16:41–54
Garrick MD et al (2006a) Comparison of mammalian cell lines expressing distinct isoforms of divalent metal transporter 1 in a tetracycline-regulated fashion. Biochem J 398:539–546. https://doi.org/10.1042/bj20051987
Garrick MD et al (2006b) DMT1: which metals does it transport? Biol Res 39:79–85
Grillo AS et al (2017) Restored iron transport by a small molecule promotes absorption and hemoglobinization in animals. Science 356:608–616. https://doi.org/10.1126/science.aah3862
Gunshin H et al (1997) Cloning and characterization of a mammalian proton-coupled metal-ion transporter. Nature 388:482–488
Gunshin H, Fujiwara Y, Custodio AO, DiRenzo C, Robine S, Andrews NC (2005) Slc11a2 is required for intestinal iron absorption and erythropoiesis but dispensable in placenta and liver. J Clin Investig 115:1258–1266. https://doi.org/10.1172/jci200524356
Illing AC, Shawki A, Cunningham CL, Mackenzie B (2012) Substrate profile and metal-ion selectivity of human divalent metal-ion transporter-1. J Biol Chem 287:30485–30496. https://doi.org/10.1074/jbc.m112.364208
Jiang L, Garrick MD, Garrick LM, Zhao L, Collins JF (2013) Divalent metal transporter 1 (Dmt1) mediates copper transport in the duodenum of iron-deficient rats and when overexpressed in iron-deprived HEK-293 cells. J Nutr 143:1927–1933. https://doi.org/10.3945/jn.113.181867
Knöpfel M, Zhao L, Garrick MD (2005) Transport of divalent transition-metal ions is lost in small-intestinal tissue of b/b Belgrade rats. Biochemistry 44:3454–3465
Lineweaver H, Burk D (1934) The determination of enzyme dissociation constants. J Am Chem Soc 56:658–666. https://doi.org/10.1021/ja01318a036
Mackenzie B, Garrick MD (2005) Iron imports. II. Iron uptake at the apical membrane in the intestine. Am J Physiol 289:G981–G986. https://doi.org/10.1152/ajpgi.00363.2005
McKie AT et al (2001) An iron-regulated ferric reductase associated with the absorption of dietary iron. Science 291:1755–1759
Michaelis L, Menten ML (1913) Die Kinetik der Invertinwirkung. Biochem Z 49:333–369
Ohgami RS, Campagna DR, McDonald A, Fleming MD (2006) The Steap proteins are metalloreductases. Blood 108:1388–1394. https://doi.org/10.1182/blood-2006-02-003681
Roth JA, Garrick MD (2003) Iron interactions and other biological reactions mediating the physiological and toxic actions of manganese. Biochem Pharmacol 66:1–13
Tripathi AK et al (2015) Prion protein functions as a ferrireductase partner for ZIP14 and DMT1. Free Radic Biol Med 84:322–330. https://doi.org/10.1016/j.freeradbiomed.2015.03.037
Acknowledgements
This research depended on support from the USA NIH 5R01DK109717 and the Laura and Michael Garrick Fund. We are also grateful to Dr. Martin D. Burke of Carle Illinois College of Medicine, University of Illinois at Urbana-Champaign, Champaign, IL, USA and Dr. Daniel J. Kosman of the Department of Biochemistry, University at Buffalo, Buffalo, NY, USA for useful discussions and sending hinokitiol plus 2-deoxyhinokitiol (MDB) or sharing some 59Iron and 54Manganese (DJK). We thank Adam Dannenhoffer of Northwestern University for helping to draw the inserts to Fig. 1.
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Garrick, M.D., Garrick, L.M., Zhao, L. et al. A direct comparison of divalent metal-ion transporter (DMT1) and hinokitiol, a potential small molecule replacement. Biometals 32, 745–755 (2019). https://doi.org/10.1007/s10534-019-00207-2
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DOI: https://doi.org/10.1007/s10534-019-00207-2