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Magnesium transporter

April 09, 2024

Magnesium transporters are proteins that transport magnesium across the cell membrane. All forms of life require magnesium, yet the molecular mechanisms of Mg2+ uptake from the environment and the distribution of this vital element within the organism are only slowly being elucidated.

The ATPase function of MgtA is highly cardiolipin dependent and has been shown to detect free magnesium in the μM range [1]

In bacteria, Mg2+ is probably mainly supplied by the CorA protein[2] and, where the CorA protein is absent, by the MgtE protein.[3][4] In yeast the initial uptake is via the Alr1p and Alr2p proteins,[5] but at this stage the only internal Mg2+ distributing protein identified is Mrs2p.[6] Within the protozoa only one Mg2+ transporter (XntAp) has been identified.[7] In metazoa, Mrs2p[8] and MgtE homologues[9] have been identified, along with two novel Mg2+ transport systems TRPM6/TRPM7[10][11] and PCLN-1.[12] Finally, in plants, a family of Mrs2p homologues has been identified[13][14] along with another novel protein, AtMHX.[15]

Evolution edit

The evolution of Mg2+ transport appears to have been rather complicated. Proteins apparently based on MgtE are present in bacteria and metazoa, but are missing in fungi and plants, whilst proteins apparently related to CorA are present in all of these groups. The two active transport transporters present in bacteria, MgtA and MgtB, do not appear to have any homologies in higher organisms. There are also Mg2+ transport systems that are found only in the higher organisms.

Types edit

There are a large number of proteins yet to be identified that transport Mg2+. Even in the best studied eukaryote, yeast, Borrelly[16] has reported a Mg2+/H+ exchanger without an associated protein, which is probably localised to the Golgi. At least one other major Mg2+ transporter in yeast is still unaccounted for, the one affecting Mg2+ transport in and out of the yeast vacuole. In higher, multicellular organisms, it seems that many Mg2+ transporting proteins await discovery.

The CorA-domain-containing Mg2+ transporters (CorA, Alr-like and Mrs2-like) have a similar but not identical array of affinities for divalent cations. In fact, this observation can be extended to all of the Mg2+ transporters identified so far. This similarity suggests that the basic properties of Mg2+ strongly influence the possible mechanisms of recognition and transport. However, this observation also suggests that using other metal ions as tracers for Mg2+ uptake will not necessarily produce results comparable to the transporter's ability to transport Mg2+. Ideally, Mg2+ should be measured directly.[17]

Since 28Mg2+ is practically unobtainable, much of the old data will need to be reinterpreted with new tools for measuring Mg2+ transport, if different transporters are to be compared directly. The pioneering work of Kolisek[18] and Froschauer[19] using mag-fura 2 has shown that free Mg2+ can be reliably measured in vivo in some systems. By returning to the analysis of CorA with this new tool, we have gained an important baseline for the analysis of new Mg2+ transport systems as they are discovered. However, it is important that the amount of transporter present in the membrane is accurately determined if comparisons of transport capability are to be made. This bacterial system might also be able to provide some utility for the analysis of eukaryotic Mg2+ transport proteins, but differences in biological systems of prokaryotes and eukaryotes will have to be considered in any experiment.

Function edit

Comparing the functions of the characterised Mg2+ transport proteins is currently almost impossible, even though the proteins have been investigated in different biological systems using different methodologies and technologies. Finding a system where all the proteins can be compared directly would be a major advance. If the proteins could be shown to be functional in bacteria (S. typhimurium), then a combination of the techniques of mag-fura 2, quantification of protein in the envelope membrane, and structure of the proteins (X-ray crystal or cryo-TEM) might allow the determination of the basic mechanisms involved in the recognition and transport of the Mg2+ ion. However, perhaps the best advance would be the development of methods allowing the measurement of the protein's function in the patch-clamp system using artificial membranes.

Bacteria edit

Early research edit

In 1968, Lusk[20] described the limitation of bacterial (Escherichia coli) growth on Mg2+-poor media, suggesting that bacteria required Mg2+ and were likely to actively take this ion from the environment. The following year, the same group[21] and another group, Silver,[22] independently described the uptake and efflux of Mg2+ in metabolically active E. coli cells using 28Mg2+. By the end of 1971, two papers had been published describing the interference of Co2+, Ni2+ and Mn2+ on the transport of Mg2+ in E. coli[23] and in Aerobacter aerogenes and Bacillus megaterium.[24] In the last major development before the cloning of the genes encoding the transporters, it was discovered that there was a second Mg2+ uptake system that showed similar affinity and transport kinetics to the first system, but had a different range of sensitivities to interfering cations. This system was also repressible by high extracellular concentrations of Mg2+ .[25][26]

CorA edit

Main article: CorA metal ion transporter

The CorA gene and its corresponding protein are the most exhaustively studied Mg2+ transport system in any organism. Most of the published literature on the CorA gene comes from the laboratory of M. E. Maguire. Recently the group of R. J. Schweyen made a significant impact on the understanding of Mg2+ transport by CorA. The gene was originally named after the cobalt-resistant phenotype in E. coli that was caused by the gene's inactivation.[25]

The gene was genetically identified in E. coli by Park et al.,[26] but wasn't cloned until Hmiel et al.[2] isolated the Salmonella enterica serovar Typhimurium (S. typhimurium) homologue. Later it would be shown by Smith and Maguire[27] that the CorA gene was present in 17 gram-negative bacteria. With the large number of complete genome sequences now available for prokaryotes, CorA has been shown to be virtually ubiquitous among the Eubacteria, as well as being widely distributed among the Archaea.[28] The CorA locus in E. coli contains a single open reading frame of 948 nucleotides, producing a protein of 316 amino acids. This protein is well conserved amongst the Eubacteria and Archaea. Between E. coli and S. typhimurium, the proteins are 98% identical, but in more distantly related species, the similarity falls to between 15 and 20%.[28] In the more distantly related genes, the similarity is often restricted to the C-terminal part of the protein, and a short amino acid motif GMN within this region is very highly conserved. The CorA domain, also known as PF01544 in the pFAM conserved protein domain database (http://webarchive.loc.gov/all/20110506030957/http%3A//pfam.sanger.ac.uk/), is additionally present in a wide range of higher organisms, and these transporters will be reviewed below.

The CorA gene is constitutively expressed in S. typhimurium under a wide range of external Mg2+ concentrations.[29] However, recent evidence suggests that the activity of the protein may be regulated by the PhoPQ two-component regulatory system.[30] This sensor responds to low external Mg2+ concentrations during the infection process of S. typhimurium in humans.[31] In low external Mg2+ conditions, the PhoPQ system was reported to suppress the function of CorA and it has been previously shown that the transcription of the alternative Mg2+ transporters MgtA and MgtB is activated in these conditions.[29] Chamnongpol and Groisman suggest that this allows the bacteria to escape metal ion toxicity caused by the transport of other ions, particularly Fe(II), by CorA in the absence of Mg2+.[30] Papp and Maguire offer a conflicting report on the source of the toxicity.[32]

 
The originally published TM topology of the CorA protein

The figure (not to scale) shows the originally published transmembrane (TM) domain topology of the S. typhimurium CorA protein, which was said to have three membrane-spanning regions in the C-terminal part of the protein (shown in blue), as determined by Smith et al..[33] Evidence for CorA acting as a homotetramer was published by Warren et al. in 2004.[34] In December 2005 the crystal structure of the CorA channel was posted to the RSCB protein structure database. The results showed that the protein has two TM domains and exists as a homopentamer, in direct conflict with the earlier reports. Follow this link to see the structure in 3D. The soluble intracellular parts of the protein are highly charged, containing 31 positively charged and 53 negatively charged residues. Conversely, the TM domains contain only one charged amino acid, which has been shown to be unimportant in the activity of the transporter.[35] From mutagenesis experiments, it appears that the chemistry of the Mg2+ transport relies on the hydroxyl groups lining the inside of the transport pore; there is also an absolute requirement for the GMN motif (shown in red).[35][36]

Before the activity of CorA could be studied in vivo, any other Mg2+ transport systems in the bacterial host had to be identified and inactivated or deleted (see below). A strain of S. typhimurium containing a functional CorA gene but lacking MgtA and MgtB was constructed[37](also see below), and the uptake kinetics of the transporter were analysed.[38] This strain showed nearly normal growth rates on standard media (50 μM Mg2+), but the removal of all three genes created a bacterial strain requiring 100 mM external Mg2+ for normal growth.[37]

Mg2+ is transported into cells containing only the CorA transport system with similar kinetics and cation sensitivities as the Mg2+ uptake described in the earlier papers, and has additionally been quantified[38](see table). The uptake of Mg2+ was seen to plateau as in earlier studies, and although no actual mechanism for the decrease in transport has been determined, so it has been assumed that the protein is inactivated.[19] Co2+ and Ni2+ are toxic to S. typhimurium cells containing a functional CorA protein and this toxicity stems from the blocking of Mg2+ uptake (competitive inhibition) and the accumulation of these ions inside the cell.[2] Co2+ and Ni2+ have been shown to be transported by CorA by using radioactive tracer analysis,[2][39] although with lower affinities (km) and velocities (Vmax) than for Mg2+ (see table). The km values for Co2+ and Ni2+ are significantly above those expected to be encountered by the cells in their normal environment, so it is unlikely that the CorA transport system mediates the uptake of these ions under natural conditions.[2] To date, the evidence for Mn2+ transport by CorA is limited to E. coli.[26]

Mg2+ Co2+ Ni2+
km (μM) 15 30 240
Vmax (pmol/min/108 cells) 250 500 360
Ki (μM) - Mg - - 10
Ki (μM) - Co 50 - 20
Ki (μM) - Mn 30 - -
Ki (μM) - Ni 300 - 300

The table lists the transport kinetics of the CorA Mg2+ transport system. This table has been compiled from the publications of Snavely et al. (1989b),[38] Gibson et al. (1991)[39] and Smith et al. (1998a)[35] and summarises the kinetic data for the CorA transport protein expressed from the wild type promoter in bacteria lacking MgtA and MgtB. km and Vmax were determined at 20 °C as the uptake of Mg2+ at 37 °C was too rapid to measure accurately.

Recently the Mg2+-dependent fluorescence of mag-fura 2 was used to measure the free Mg2+ content of S. typhimurium cells in response to external Mg2+, which showed that CorA is the major uptake system for Mg2+ in bacteria.[19] The authors also showed for the first time that the changes in the electric potential (ΔΨ) across the plasma membrane of the cell affected both the rate of Mg2+ uptake and the free Mg2+ content of the cell; depolarisation suppressed transport, while hyperpolarisation increased transport. The kinetics of transport were defined only by the rate of change of free Mg2+ inside the cells (250 μM s−1). Because no quantification of the amount of CorA protein in the membrane was made, this value cannot be compared with other experiments on Mg2+ transporters.[18]

The efflux of Mg2+ from bacterial cells was first observed by Lusk and Kennedy (1969)[21] and is mediated by the CorA Mg2+ transport system in the presence of high extracellular concentrations of Mg2+.[38] The efflux can also be triggered by Co2+, Mn2+ and Ni2+, although not to the same degree as Mg2+.[23] No Co2+ efflux through the CorA transport system was observed. The process of Mg2+ efflux additionally requires one of the CorB, CorC or CorD genes.[39] The mutation of any single one of these genes leads to a Co2+ resistance a little less than half of that provided by a CorA mutant. This effect may be due to the inhibition of Mg2+ loss that would otherwise occur in the presence of high levels of Co2+. It is currently unknown whether Mg2+ is more toxic when the CorBCD genes are deleted.

It has been speculated that the Mg2+ ion will initially interact with any transport protein through its hydration shell.[40] Cobalt (III) hexaammine, Co(III)Hex, is a covalently bound (non-labile) analog for the first shell of hydration for several divalent cations, including Mg2+. The radius of the Co(III)Hex molecule is 244 pm, very similar to the 250 pm radius of the first hydration shell of Mg2+. This analog is a potent inhibitor of the CorA transport system, more so than Mg2+, Co2+ or Ni2+.[41] The additional strength of the Co(III)Hex inhibition might come from the blocking of the transport pore due to the inability of the protein to ‘dehydrate’ the substrate. It was also shown that Co(III)Hex was not transported into the cells,[41] suggesting that at least partial dehydration would be required for the transport of the normal substrate (Mg2+). Nickel (II) hexaammine, with a radius of 255 pm, did not inhibit the CorA transport system, suggesting a maximum size limit exists for the binding of the CorA substrate ion.[41] These results suggest that the important property involved in the recognition of Mg2+ by CorA is the size of the ion with its first shell of hydration. Hence, the volume change generally quoted for the bare to hydrated Mg2+ ion of greater than 500-fold, including the second sphere of hydration, may not be biologically relevant, and may be a reason for the first sphere volume change of 56-fold to be more commonly used.

MgtA and MgtB edit

The presence of these two genes was first suspected when Nelson and Kennedy (1972)[25] showed that there were Mg2+-repressible and non-repressible Mg2+ uptake systems in E. coli. The non-repressible uptake of Mg2+ is mediated by the CorA protein. In S. typhimurium the repressible Mg2+ uptake was eventually shown to be via the MgtA and MgtB proteins.[37]

Both MgtA and MgtB are regulated by the PhoPQ system and are actively transcribed during the process of infection of human patients by S. typhimurium.[31][42][43] Although neither gene is required for pathogenicity, the MgtB protein does enhance the long-term survival of the pathogen in the cell.[44] The genes are also upregulated in vitro when the Mg2+ concentration falls below 50 μM (Snavely et al., 1991a). Although the proteins have km values similar to CorA and transport rates approximately 10 times less, the genes may be part of a Mg2+ scavenging system. Chamnongpol and Groisman (2002) presents evidence that the role of these proteins may be to compensate for the inactivation of the CorA protein by the PhoPQ regulon.[30] The authors suggest that the CorA protein is inactivated to allow the avoidance of metal toxicity via the protein in the low Mg2+ environments S. typhimurium is subjected to by cells after infection.

The proteins are both P-type ATPases[38][45] and neither gene shows any similarity to CorA. The MgtA and MgtB proteins are 75% similar (50% identical), although it seems that MgtB may have been acquired by horizontal gene transfer as part of Salmonella Pathogenicity Island 3.[45][46] The TM topology of the MgtB protein has been experimentally determined, showing that the protein has ten TM-spanning helices with the termini of the protein in the cytoplasm (see figure ). MgtA is present in widely divergent bacteria, but is not nearly as common as CorA, while MgtB appears to have a quite restricted distribution.[47] No hypotheses for the unusual distribution have been suggested.

 
The TM topology of the MgtB protein

The figure, adapted from Smith et al. (1993b),[48] shows the experimentally determined membrane topology of the MgtB protein in S. typhimurium. The TM domains are shown in light blue and the orientation in the membrane and the positions of the N- and C-termini are indicated. The figure is not drawn to scale.

While the MgtA and MgtB proteins are very similar, they do show some minor differences in activity. MgtB is very sensitive to temperature, losing all activity (with regard to Mg2+ transport) at a temperature of 20 °C.[38] Additionally, MgtB and MgtA are inhibited by different ranges of cations (Table A10.1[38]).

The table lists cation transport characteristics of the MgtA and MgtB proteins in S. typhimurium as well as the kinetic data for the MgtA and MgtB transport proteins at 37 °C.[38] The Vmax numbers listed in parentheses are those for uptake at 20 °C. The inhibition of Mg2+ transport by Mn2+ via MgtA showed unusual kinetics (see Figure 1 of Snavely et al., 1989b[38])

Mg2+ Co2+
km (μM) Vmax (pmol/min/108 cells) Ki (μM)
Co2+ Mn2+ Ni2+
MgtA 29 115(24) 40 x 30
MgtB 6 75(<2) 8 40 13

The MgtA and MgtB proteins are ATPases, using one molecule of ATP per transport cycle, whereas the Mg2+ uptake via CorA is simply electrochemically favourable. Chamnongpol and Groisman (2002) have suggested that the MgtA and MgtB proteins form part of a metal toxicity avoidance system.[30] Alternatively, as most P-type ATPases function as efflux mediating transporters, it has been suggested that the MgtA and MgtB proteins act as efflux proteins for a currently unidentified cation, and Mg2+ transport is either non-specific or exchanged to maintain the electro-neutrality of the transport process.[49] Further experiments will be required to define the physiological function of these proteins.

MgtE edit

Main article: Magnesium transporter E
MgtE
 
Crystal structure of magnesium transporter MgtE. PDB 2zy9[50]
Identifiers
SymbolMgtE
PfamPF01769
InterProIPR006667
TCDB1.A.26
OPM protein2yvx
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary

Two papers describe MgtE, a fourth Mg2+ uptake protein in bacteria unrelated to MgtA/B or CorA.[3][4] This gene has been sequenced and the protein, 312 amino acids in size, is predicted to contain either four or five TM spanning domains that are closely arranged in the C-terminal part of the protein (see figure). This region of the protein has been identified in the Pfam database as a conserved protein domain (PF01769) and species containing proteins that have this protein domain are roughly equally distributed throughout the Eubacteria and Archaea, although it is quite rare in comparison with the distribution of CorA. However, the diversity of the proteins containing the domain is significantly larger than that of the CorA domain. The Pfam database lists seven distinct groups of MgtE domain containing proteins, of which six contain an archaic or eubacterial member. The expression of MgtE is frequently controlled by a conserved RNA structure, YkoK leader or M-box.[51]

 
The predicted TM topology of the MgtE protein

The figure (right), adapted from Smith et al. (1995)[4] and the PFAM database entry, shows the computer-predicted membrane topology of the MgtE protein in Bacillus firmus OF4. The TM domains are shown in light blue. The CBS domains, named for the protein they were identified in, cystathionine-beta synthase, shown in orange, are identified in the Pfam database as regulatory domains, but the mechanism of action has not yet been described. They are found in several voltage-gated chloride channels.[52] The orientation in the membrane and the positions of the N- and C-termini are indicated. This figure is not drawn to scale. This transporter has recently had its structure solved by x-ray crystallography.[53]

The MgtE gene was first identified by Smith et al. (1995) during a screen for CorA-like proteins in bacteria and complements the Mg2+-uptake-deficient S. typhimurium strain MM281 (corA mgtA mgtB), restoring wild type growth on standard media.[4] The kinetics of Mg2+ transport for the protein were not determined, as 28Mg2+ was unavailable. As a substitute, the uptake of 57Co2+ was measured and was shown to have a km of 82 μM and a Vmax of 354 pmol min−1 108 cells−1. Mg2+ was a competitive inhibitor with a Ki of 50 μM—the Ki of Mg2+ inhibition of 60Co2+ uptake via CorA is 10 μM.[2] A comparison of the available kinetic data for MgtA and CorA is shown in the table. Clearly, MgtE does not transport Co2+ to the same degree as CorA, and the inhibition of transport by Mg2+ is also less efficient, which suggests that the affinity of MgtE for Mg2+ is lower than that of CorA. The strongest inhibitor of Co2+ uptake was Zn2+, with a Ki of 20 μM.[4] The transport of Zn2+ by this protein may be as important as that of Mg2+.

Mg2+ Co2+
km (μM) Vmax (pmol/min/108 cells) km (μM) Vmax (pmol/min/108 cells) Ki(Mg2+) (μM)
MgtE - - 82[4] (at 37 °C) 354[4] (at 37 °C) 50[4] (at 37 °C)
CorA 15[38] (at 20 °C) 250[38] (at 20 °C) 30[2] (at 22 °C) 500[2] (at 22 °C) 10[2] (at 22 °C)

The table shows a comparison of the transport kinetics of MgtE and CorA, and key kinetic parameter values for them are listed. As shown, the data has been generated at differing incubation temperatures. km and Ki are not significantly altered by the differing incubation temperature. Conversely, Vmax shows a strong positive correlation with temperature, hence the value of Co2+ Vmax for MgtE is not directly comparable with the values for CorA.

Yeast edit

Early research edit

The earliest research showing that yeast takes up Mg2+ appears to be done by Schmidt et al. (1949). However, these authors only showed altered yeast Mg2+ content in a table within the paper, and the report's conclusions dealt entirely with the metabolism of phosphate. A series of experiments by Rothstein[54][55] shifted the focus more towards the uptake of the metal cations, showing that yeast take up cations with the following affinity series; Mg2+, Co2+, Zn2+ > Mn2+ > Ni2+ > Ca2+ > Sr2+. Additionally, it was suggested that the transport of the different cations is mediated by the same transport system[55][56][57][58] — a situation very much like that in bacteria.

In 1998, MacDiarmid and Gardner finally identified the proteins responsible for the observed cation transport phenotype in Saccharomyces cerevisiae.[5] The genes involved in this system and a second mitochondrial Mg2+ transport system, functionally identified significantly after the gene was cloned, are described in the sections below.

ALR1 and ALR2 edit

Two genes, ALR1 and ALR2, were isolated in a screen for Al3+ tolerance (resistance) in yeast.[5] Over-expression constructs containing yeast genomic DNA were introduced into wild type yeast and the transformants were screened for growth on toxic levels of Al3+. ALR1 and ALR2 containing plasmids allowed the growth of yeast in these conditions.

The Alr1p and Alr2p proteins consist of 859 and 858 amino acids respectively and are 70% identical. In a region in the C-terminal, half of these proteins are weakly similar to the full CorA protein. The computer-predicted TM topology of Alr1p is shown in the figure. The presence of a third TM domain was suggested by MacDiarmid and Gardner (1998),[5] on the strength on sequence homology, and more recently by Lee and Gardner (2006),[59] on the strength of mutagenesis studies, making the TM topology of these proteins more like that of CorA (see figure). Also, Alr1p contains the conserved GMN motif at the outside end of TM 2 (TM 2') and the mutation of the methionine (M) in this motif to a leucine (L) led to the loss of transport capability.[59]

The figure shows the two possible TM topologies of Alr1p. Part A of the figure shows the computer-predicted membrane topology of the Alr1p protein in yeast and part B shows the topology of Alr1p based on the experimental results of Lee and Gardner (2006).[59] The GMN motif location is indicated in red and the TM domains in light blue. The orientation in the membrane and the positions of the N- and C-termini are indicated, the various sizes of the soluble domains are given in amino acids (AA), and TM domains are numbered by their similarity to CorA. Where any TM domain is missing, the remaining domains are numbered with primes. The figure is not drawn to scale. A third ALR-like gene is present in S. cerevisiae and there are two homologous genes in both Schizosaccharomyces pombe and Neurospora crassa. These proteins contain a GMN motif like that of CorA, with the exception of the second N. crassa gene. No ALR-like genes have been identified in species outside of the fungi.

Membrane fractionation and green fluorescent protein (GFP) fusion studies established that Alr1p is localised to the plasma membrane.[60][61] The localisation of the Alr1p was observed to be internalised and degraded in the vacuole in response to extracellular cations. Mg2+, at very low extracellular concentrations (100 μM; < 10% of the standard media Mg2+ content), and Co2+ and Mn2+ at relatively high concentrations (> 20× standard media), induced the change in Alr1p protein localisation, and the effect was dependent on functional ubiquitination, endocytosis and vacuolar degradation.[60] This mechanism was proposed to allow the regulation of Mg2+ uptake by yeast. However, a recent report [61] indicates that several of the observations made by Stadler et al.[60] were not reproducible.[61] For example, regulation of ALR1 mRNA accumulation by Mg2+ supply was not observed, and the stability of the Alr1 protein was not reduced by exposure to excess Mg2+. The original observation of Mg-dependent accumulation of the Alr1 protein under steady-state low-Mg conditions was replicated, but this effect was shown to be an artifact caused by the addition of a small peptide (epitope) to the protein to allow its detection. Despite these problems, Alr1 activity was demonstrated to respond to Mg supply,[61] suggesting that the activity of the protein is regulated directly, as was observed for some bacterial CorA proteins.[19]

A functional Alr1p (wild type) or Alr2p (overexpressed) is required for S. cerevisiae growth in standard conditions (4 mM Mg2+[5]), and Alr1p can support normal growth at Mg2+ concentrations as low as 30 μM.[60] 57Co2+ is taken up into yeast via the Alr1p protein with a km of 77 – 105 μM (;[56] C. MacDiarmid and R. C. Gardner, unpublished data), but the Ki for Mg2+ inhibition of this transport is currently unknown. The transport of other cations by the Alr1p protein was assayed by the inhibition of yeast growth. The overexpression of Alr1p led to increased sensitivity to Ca2+, Co2+, Cu2+, La3+, Mn2+, Ni2+ and Zn2+, an array of cations similar to those shown to be transported into yeast by a CorA-like transport system.[5] The increased toxicity of the cations in the presence of the transporter is assumed to be due to the increased accumulation of the cation inside the cell.

The evidence that Alr1p is primarily a Mg2+ transporter is that the loss of Alr1p leads to a decreased total cell content of Mg2+, but not of other cations. Additionally, two electrophysiological studies where Alr1p was produced in yeast or Xenopus oocytes showed a Mg2+-dependent current in the presence of the protein;[62] Salih et al., in prep.

The kinetics of Mg2+ uptake by Alr1p have been investigated by electrophysiology techniques on whole yeast cells.[62] The results suggested that Alr1p is very likely to act as an ion-selective channel. In the same paper, the authors reported that Mg2+ transport by Alr1p varied from 200 pA to 1500 pA, with a mean current of 264 pA. No quantification of the amount of protein producing the current was presented, so the results lack comparability with the bacterial Mg2+ transport proteins.

The alternative techniques of 28Mg2+ radiotracer analysis and mag-fura 2 to measure Mg2+ uptake have not yet been used with Alr1p. 28Mg2+ is currently not available and the mag-fura 2 system is unlikely to provide simple uptake data in yeast. The yeast cell maintains a heterogeneous distribution of Mg2+[63] suggesting that multiple systems inside the yeast are transporting Mg2+ into storage compartments. This internal transport will very likely mask the uptake process. The expression of ALR1 in S. typhimurium without Mg2+ uptake genes may be an alternative, but, as stated earlier, the effects of a heterologous expression system would need to be taken into account.

MNR2 edit

The MNR2 gene encodes a protein closely related to the Alr proteins, but includes conserved features that define a distinct subgroup of CorA proteins in fungal genomes, suggesting a distinct role in Mg2+ homeostasis. Like an alr1 mutant, growth of an mnr2 mutant was sensitive to Mg2+-deficient conditions, but the mnr2 mutant was observed to accumulate more Mg2+ than a wild-type strain under these conditions.[64] These phenotypes suggested that Mnr2 may regulate Mg2+ storage within an intracellular compartment. Consistent with this interpretation, the Mnr2 protein was localized to the membrane of the vacuole, an internal compartment implicated in the storage of excess mineral nutrients by yeast. A direct role of Mnr2 in Mg2+ transport was suggested by the observation that increased Mnr2 expression, which redirected some Mnr2 protein to the cell surface, also suppressed the Mg2+-requirement of an alr1 alr2 double mutant strain. The mnr2 mutation also altered accumulation of other divalent cations, suggesting this mutation may increase Alr gene expression or protein activity. Recent work [61] supported this model, by showing that Alr1 activity was increased in an mnr2 mutant strain, and that the mutation was associated with induction of Alr1 activity at a higher external Mg concentration than was observed for an Mnr2 wild-type strain. These effects were observed without any change in Alr1 protein accumulation, again indicating that Alr1 activity may be regulated directly by the Mg concentration within the cell.

MRS2 and Lpe10 edit

Like the ALR genes, the MRS2 gene was cloned and sequenced before it was identified as a Mg2+ transporter. The MRS2 gene was identified in the nuclear genome of yeast in a screen for suppressors of a mitochondrial gene RNA splicing mutation,[65] and was cloned and sequenced by Wiesenberger et al. (1992).[66] Mrs2p was not identified as a putative Mg2+ transporter until Bui et al. (1999).[6] Gregan et al. (2001a) identified LPE10 by homology to MRS2 and showed that both LPE10 and MRS2 mutants altered the Mg2+ content of yeast mitochondria and affected RNA splicing activity in the organelle.[67][68] Mg2+ transport has been shown to be directly mediated by Mrs2p,[18] but not for Lpe10p.

The Mrs2p and Lpe10p proteins are 470 and 413 amino acid residues in size, respectively, and a 250–300 amino acid region in the middle of the proteins shows a weak similarity to the full CorA protein. The TM topologies of the Mrs2p and Lpe10p proteins have been assessed using a protease protection assay[6][67] and are shown in the figure. TM 1 and 2 correspond to TM 2 and 3 in the CorA protein. The conserved GMN motif is at the outside end of the first TM domain, and when the glycine (G) in this motif was mutated to a cysteine (C) in Mrs2p, Mg2+ transport was strongly reduced.[18]

 
The TM topology of the MRS2 and LPE10 proteins

The figure shows the experimentally determined topology of Mrs2p and Lpe10p as adapted from Bui et al. (1999)[6] and Gregan et al. (2001a).[67] The GMN motif location is indicated in red and the TM domains in light blue. The orientation in the membrane and the positions of the N- and C-termini are indicated. The various sizes of the soluble domains are given in amino acids (AA), TM domains are numbered, and the figure is not drawn to scale.

Mrs2p has been localised to the mitochondrial inner membrane by subcellular fractionation and immunodetection[6] and Lpe10p to the mitochondria.[67] Mitochondria lacking Mrs2p do not show a fast Mg2+ uptake, only a slow ‘leak’, and overaccumulation of Mrs2p leads to an increase in the initial rate of uptake.[18] Additionally, CorA, when fused to the mitochondrial leader sequence of Mrs2p, can partially complement the mitochondrial defect conferred by the loss of either Mrs2p or Lpe10p. Hence, Mrs2p and/or Lpe10p may be the major Mg2+ uptake system for mitochondria. A possibility is that the proteins form heterodimers, as neither protein (when overexpressed) can fully complement the loss of the other.[67]

The characteristics of Mg2+ uptake in isolated mitochondria by Mrs2p were quantified using mag-fura 2.[18] The uptake of Mg2+ by Mrs2p shared a number of attributes with CorA. First, Mg2+ uptake was directly dependent on the electric potential (ΔΨ) across the boundary membrane. Second, the uptake is saturated far below that which the ΔΨ theoretically permits, so the transport of Mg2+ by Mrs2p is likely to be regulated in a similar manner to CorA, possibly by the inactivation of the protein. Third, Mg2+ efflux was observed via Mrs2p upon the artificial depolarisation of the mitochondrial membrane by valinomycin. Finally, the Mg2+ fluxes through Mrs2p are inhibited by cobalt (III) hexaammine.[18]

The kinetics of Mg2+ uptake by Mrs2p were determined in the Froschauer et al. (2004) paper on CorA in bacteria.[19] The initial change in free Mg2+ concentration was 150 μM s-1 for wild type and 750 μM s-1 for mitochondria from yeast overexpressing MRS2. No attempt was made to scale the observed transport to the amount of transporter present.

Protozoan (Paramecium) edit

The transport of Mg2+ into Paramecium has been characterised largely by R. R. Preston and his coworkers. Electrophysiological techniques on whole Paramecium were used to identify and characterise Mg2+ currents in a series of papers[69][70][71][72] before the gene was cloned by Haynes et al. (2002).[7]

The open reading frame for the XNTA gene is 1707 bp in size, contains two introns and produces a predicted protein of 550 amino acids.[7] The protein has been predicted to contain 11 TM domains and also contains the α1 and α2 motifs (see figure) of the SLC8 (Na+/Ca2+ exchanger[73]) and SLC24 (K+ dependent Na+/Ca2+ exchanger[74]) human solute transport proteins. The XntAp is equally similar to the SLC8 and SLC24 protein families by amino acid sequence, but the predicted TM topology is more like that of SLC24, but the similarity is at best weak and the relationship is very distant.[7] The AtMHX protein from plants also shares a distant relationship with the SLC8 proteins.

 
The TM topology of the XNTA protein

The figure shows the predicted TM topology of XntAp. Adapted from Haynes et al. (2002),[7] this figure shows the computer predicted membrane topology of XntAp in Paramecium. The orientation in the membrane was determined using HMMTOP.[75][76] The TM domains are shown in light blue, the α1 and α2 domains are shown in green. The orientation in the membrane and the positions of the N- and C-termini are indicated and the figure is not drawn to scale.

The Mg2+-dependent currents carried by XntAp are kinetically like that of a channel protein and have an ion selectivity order of Mg2+ > Co2+, Mn2+ > Ca2+ — a series again very similar to that of CorA.[72] Unlike the other transport proteins reported so far, XntAp is dependent on intracellular Ca2+. The transport is also dependent on ΔΨ, but again Mg2+ is not transported to equilibrium, being limited to approximately 0.4 mM free Mg2+ in the cytoplasm. The existence of an intracellular compartment with a much higher free concentration of Mg2+ (8 mM) was supported by the results.

Animals edit

The investigation of Mg2+ in animals, including humans, has lagged behind that in bacteria and yeast. This is largely because of the complexity of the systems involved, but also because of the impression within the field that Mg2+ was maintained at high levels in all cells and was unchanged by external influences. Only in the last 25 years has a series of reports begun to challenge this view, with new methodologies finding that free Mg2+ content is maintained at levels where changes might influence cellular metabolism.[77]

MRS2 edit

A bioinformatic search of the sequence databases identified one homologue of the MRS2 gene of yeast in a range of metazoans.[8] The protein has a very similar sequence and predicted TM topology to the yeast protein, and the GMN motif is intact at the end of the first TM domain. The human protein, hsaMrs2p, has been localised to the mitochondrial membrane in mouse cells using a GFP fusion protein.

Very little is known about the Mg2+ transport characteristics of the protein in mammals, but Zsurka et al. (2001) has shown that the human Mrs2p complements the mrs2 mutants in the yeast mitochondrial Mg2+ uptake system.[8]

SLC41 (MgtE) edit

The identification of this gene family in the metazoa began with a signal sequence trap method for isolating secreted and membrane proteins.[9] Much of the identification has come from bioinformatic analyses. Three genes were eventually identified in humans, another three in mouse and three in Caenorhabditis elegans, with a single gene in Anopheles gambiae. The pFAM database lists the MgtE domain as pFAM01769 and additionally identifies a MgtE domain-containing protein in Drosophila melanogaster. The proteins containing the MgtE domain can be divided into seven classes, as defined by pFAM using the type and organisation of the identifiable domains in each protein. Metazoan proteins are present in three of the seven groups. All of the metazoa proteins contain two MgtE domains, but some of these have been predicted only by context recognition (Coin, Bateman and Durbin, unpublished. See the pFAM website for further details).

The human SLC41A1 protein contains two MgtE domains with 52% and 46% respective similarity to the PF01769 consensus sequence and is predicted to contain ten TM domains, five in each MgtE domain (see figure), which suggests that the MgtE protein of bacteria may work as a dimer.

 
The predicted TM topology of MgtE from H. sapiens

Adapted from Wabakken et al. (2003)[9] and the pFAM database, the figure shows the computer predicted membrane topology of MgtE in H. sapiens. The TM domains are shown in light blue, the orientation in the membrane and the positions of the N- and C-termini are indicated, and the figure is not drawn to scale.

Wabakken et al. (2003)[9] found that the transcript of the SLC41A1 gene was expressed in all human tissues tested, but at varying levels, with the heart and testis having the highest expression of the gene. No explanation of the expression pattern has been suggested with regard to Mg2+-related physiology.

It has not been shown whether the SLC41 proteins transport Mg2+ or complement a Mg2+ transport mutation in any experimental system. However, it has been suggested that as MgtE proteins have no other known function, they are likely to be Mg2+ transporters in the metazoa as they are in the bacteria.[9] This will need to be verified using one of the now standard experiment systems for examining Mg2+ transport.

TRPM6/ TRPM7 edit

The investigation of the TRPM genes and proteins in human cells is an area of intense recent study and, at times, debate. Montell et al. (2002)[78] have reviewed the research into the TRP genes, and a second review by Montell (2003)[79] has reviewed the research into the TRPM genes.

The TRPM family of ion channels has members throughout the metazoa. The TRPM6 and TRPM7 proteins are highly unusual, containing both an ion channel domain and a kinase domain (Figure 1.7), the role of which brings about the most heated debate.[79]

The activity of these two proteins has been very difficult to quantify. TRPM7 by itself appears to be a Ca2+ channel[80] but in the presence of TRPM6 the affinity series of transported cations places Mg2+ above Ca2+.[10][81] The differences in reported conductance were caused by the expression patterns of these genes. TRPM7 is expressed in all cell types tested so far, while TRPM6 shows a more restricted pattern of expression.[82] An unfortunate choice of experimental system by Voets et al., (2004)[83] led to the conclusion that TRPM6 is a functional Mg2+ transporter. However, later work by Chubanov et al. (2004)[82] clearly showed that TRPM7 is required for TRPM6 activity and that the results of Voets et al. are explained by the expression of TRPM7 in the experimental cell line used by Voets et al. in their experiments. Whether TRPM6 is functional by itself is yet to be determined.

 
The predicted TM topology of the TRPM6 and TRPM7 proteins

The predicted TM topology of the TPRM6 and TRPM7 proteins has been adapted from Nadler et al. (2001),[10] Runnels et al. (2001)[84] and Montell et al. (2002),[78] this figure shows the computer predicted membrane topology of the TRPM6 and TRPM7 proteins in Homo sapiens. At this time, the topology shown should be considered a tentative hypothesis. The TM domains are shown in light blue, the pore loop in purple, the TRP motif in red and the kinase domain in green. The orientation in the membrane and the positions of the N- and C-termini are indicated and the figure is not drawn to scale.

The conclusions of the Voets et al. (2004)[83] paper are probably incorrect in attributing the Mg2+ dependent currents to TRPM7 alone, and their kinetic data are likely to reflect the combined TRPM7/ TRPM6 channel. The report presents a robust collection of data consistent with a channel-like activity passing Mg2+, based on both electrophysiological techniques and also mag-fura 2 to determine changes in cytoplasmic free Mg2+.

Paracellular transport edit

Claudins allow for Mg2+ transport via the paracellular pathway; that is, it mediates the transport of the ion through the tight junctions between cells that form an epithelial cell layer. In particular, Claudin-16 allows the selective reuptake of Mg2+ in the human kidney. Some patients with mutations in the CLDN19 gene also have altered magnesium transport.[85][86]

The gene Claudin-16 was cloned by Simon et al. (1999),[12] but only after a series of reports described the Mg2+ flux itself with no gene or protein.[87][88][89] The expression pattern of the gene was determined by RT-PCR, and was shown to be very tightly confined to a continuous region of the kidney tubule running from the medullary thick descending limb to the distal convoluted tubule.[12] This localisation was consistent with the earlier reports for the location of Mg2+ re-uptake by the kidney. Following the cloning, mutations in the gene were identified in patients with familial hypomagnesaemia with hypercalciuria and nephrocalcinosis,[90][91] strengthening the links between the gene and the uptake of Mg2+.

Plants edit

The current knowledge of the molecular mechanisms for Mg2+ transport in plants is very limited, with only three publications reporting a molecular basis for Mg2+ transport in plants.[13][14][15] However, the importance of Mg2+ to plants has been well described, and physiological and ecophysiological studies about the effects of Mg2+ are numerous. This section will summarise the knowledge of a gene family identified in plants that is distantly related to CorA. Another gene, a Mg2+/H+ exchanger (AtMHX[15]), unrelated to this gene family and to CorA has also been identified, is localised to the vacuolar membrane, and will be described last.

The AtMRS2 gene family edit

Schock et al. (2000) identified and named the family AtMRS2 based on the similarity of the genes to the MRS2 gene of yeast.[13] The authors also showed that the AtMRS2-1 gene could complement a Δmrs2 yeast mutant phenotype. Independently, Li et al. (2001)[14] published a report identifying the family and showing that two additional members could complement Mg2+ transport deficient mutants, one in S. typhimurium and the other in S. cerevisiae.

The three genes that have been shown to transport Mg2+ are AtMRS2-1, AtMRS2-10 and AtMRS2-11, and these genes produce proteins 442, 443 and 459 amino acids in size, respectively. Each of the proteins shows significant similarity to Mrs2p of yeast and a weak similarity to CorA of bacteria, contains the conserved GMN amino acid motif at the outside end of the first TM domain, and is predicted to have two TM domains.

The AtMRS2-1 gene, when expressed in yeast from the MRS2 promoter and being fused C-terminally to the first 95 amino acids of the Mrs2p protein, was directed to the mitochondria, where it complemented a Δmrs2 mutant both phenotypically (mitochondrial RNA splicing was restored) and with respect to the Mg2+ content of the organelle.[13] No data on the kinetics of the transport was presented. The AtMRS2-11 gene was analysed in yeast (in the alr1 alr2 strain), where it was shown that expression of the gene significantly increased the rate of Mg2+ uptake into starved cells over the control, as measured using flame atomic absorption spectroscopy of total cellular Mg2+ content. However, Alr1p was shown to be significantly more effective at transporting Mg2+ at low extracellular concentrations, suggesting that the affinity of AtMRS2-11 for Mg2+ is lower than that of Alr1p.[14] An electrophysiological (voltage clamp) analysis of the AtMRS2-11 protein in Xenopus oocytes also showed a Mg2+-dependent current at membrane potentials (ΔΨ) of –100 – –150 mV inside.[92] These values are physiologically significant, as several membranes in plants maintain ΔΨ in this range. However, the author had difficulty reproducing these results due to an apparent "death" of oocytes containing the AtMRS2-11 protein, and therefore these results should be viewed with caution.

The AtMRS2-10 transporter has been analysed using radioactive tracer uptake analysis.[14] 63Ni2+ was used as the substitute ion and Mg2+ was shown to inhibit the uptake of 63Ni2+ with a Ki of 20 μM. Uptake was also inhibited by Co(III)Hex and by other divalent cations. Only Co2+ and Cu2+ inhibited transport with Ki values less than 1 mM.

The AtMRS2-10 protein was fused to GFP, and was shown to be localised to the plasma membrane.[14] A similar experiment was attempted in the Schock et al. (2000) paper,[13] but the observed localisation was not significantly different from that seen with unfused GFP. The most likely reason for the lack of a definitive localisation of AtMRS2-1 in the Schock et al. paper is that the authors removed the TM domains from the protein, thereby precluding its insertion into a membrane.

The exact physiological significance of the AtMRS2-1 and AtMRS2-10 proteins in plants has yet to be clarified. The AtMRS2-11 gene has been overexpressed (from the CaMV 35S promoter) in A. thaliana.[92] The transgenic line has been shown to accumulate high levels of the AtMRS2-11 transcript. A strong Mg2+ deficiency phenotype (necrotic spots on the leaves, see Chapter 1.5 below) was recorded during the screening process (in both the T1 and T2 generations) for a homozygote line, but this phenotype was lost in the T3 generation and could not be reproduced when the earlier generations were screened a second time. The author suggested that environmental effects were the most likely cause of the inconsistent phenotype.

AtMHX edit

The first magnesium transporter isolated in any multicellular organism, AtMHX shows no similarity to any previously isolated Mg2+ transport protein.[15] The gene was initially identified in the A. thaliana genomic DNA sequence database, by its similarity to the SLC8 family of Na+/Ca2+ exchanger genes in humans.

The cDNA sequence of 1990 bp is predicted to produce a 539-amino acid protein. AtMHX is quite closely related to the SLC8 family at the amino acid level and shares a topology with eleven predicted TM domains (Figure A10.5). There is one major difference in the sequence, in that the long non-membranal loop (see Figure A10.5) is 148 amino acids in the AtMHX protein but 500 amino acids in the SLC8 proteins. However, this loop is not well conserved and is not required for transport function in the SLC8 family.[15]

The AtMHX gene is expressed throughout the plant but most strongly in the vascular tissue.[15] The authors suggest that the physiological role of the protein is to store Mg2+ in these tissues for later release when needed. The protein localisation to the vacuolar membrane supports this suggestion (see also Chapter 1.5).

The protein transports Mg2+ into the vacuolar space and H+ out, as demonstrated by electrophysiological techniques.[15] The transport is driven by the ΔpH maintained between the vacuolar space (pH 4.5 – 5.9) and the cytoplasm (pH 7.3 – 7.6) by an H+-ATPase.[93][94] How the transport of Mg2+ by the protein is regulated was not determined. Currents were observed to pass through the protein in both directions, but the Mg2+ out current required a ‘cytoplasmic’ pH of 5.5, a condition not found in plant cells under normal circumstances. In addition to the transport of Mg2+, Shaul et al. (1999)[15] also showed that the protein could transport Zn2+ and Fe2+, but did not report on the capacity of the protein to transport other divalent cations (e.g. Co2+ and Ni2+) or its susceptibility to inhibition by cobalt (III) hexaammine.

The detailed kinetics of Mg2+ transport have not been determined for AtMHX. However, physiological effects have been demonstrated. When A. thaliana plants were transformed with overexpression constructs of the AtMHX gene driven by the CaMV 35S promoter, the plants over-accumulated the protein and showed a phenotype of necrotic lesions in the leaves, which the authors suggest is caused by a disruption in the normal function of the vacuole, given their observation that the total Mg2+ (or Zn2+) content of the plants was not altered in the transgenic plants.

 
The predicted TM topology of the AtMHX protein

The image has been adapted from Shaul et al. (1999)[15] and Quednau et al. (2004),[73] and combined with an analysis using HMMTOP, this figure shows the computer predicted membrane topology of the AtMHX protein in Arabidopsis thaliana. At this time the topology shown should be considered a tentative hypothesis. The TM domains are shown in light blue, the orientation in the membrane and the positions of the N- and C-termini are indicated, and the figure is not drawn to scale. The α1 and α2 domains, shown in green, are both quite hydrophobic and may both be inserted into the membrane.

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April 09, 2024
magnesium, transporter, proteins, that, transport, magnesium, across, cell, membrane, forms, life, require, magnesium, molecular, mechanisms, uptake, from, environment, distribution, this, vital, element, within, organism, only, slowly, being, elucidated, atpa. Magnesium transporters are proteins that transport magnesium across the cell membrane All forms of life require magnesium yet the molecular mechanisms of Mg2 uptake from the environment and the distribution of this vital element within the organism are only slowly being elucidated The ATPase function of MgtA is highly cardiolipin dependent and has been shown to detect free magnesium in the mM range 1 In bacteria Mg2 is probably mainly supplied by the CorA protein 2 and where the CorA protein is absent by the MgtE protein 3 4 In yeast the initial uptake is via the Alr1p and Alr2p proteins 5 but at this stage the only internal Mg2 distributing protein identified is Mrs2p 6 Within the protozoa only one Mg2 transporter XntAp has been identified 7 In metazoa Mrs2p 8 and MgtE homologues 9 have been identified along with two novel Mg2 transport systems TRPM6 TRPM7 10 11 and PCLN 1 12 Finally in plants a family of Mrs2p homologues has been identified 13 14 along with another novel protein AtMHX 15 Contents 1 Evolution 2 Types 3 Function 4 Bacteria 4 1 Early research 4 2 CorA 4 3 MgtA and MgtB 4 4 MgtE 5 Yeast 5 1 Early research 5 2 ALR1 and ALR2 5 3 MNR2 5 4 MRS2 and Lpe10 6 Protozoan Paramecium 7 Animals 7 1 MRS2 7 2 SLC41 MgtE 7 3 TRPM6 TRPM7 7 4 Paracellular transport 8 Plants 8 1 The AtMRS2 gene family 8 2 AtMHX 9 ReferencesEvolution editThe evolution of Mg2 transport appears to have been rather complicated Proteins apparently based on MgtE are present in bacteria and metazoa but are missing in fungi and plants whilst proteins apparently related to CorA are present in all of these groups The two active transport transporters present in bacteria MgtA and MgtB do not appear to have any homologies in higher organisms There are also Mg2 transport systems that are found only in the higher organisms Types editThere are a large number of proteins yet to be identified that transport Mg2 Even in the best studied eukaryote yeast Borrelly 16 has reported a Mg2 H exchanger without an associated protein which is probably localised to the Golgi At least one other major Mg2 transporter in yeast is still unaccounted for the one affecting Mg2 transport in and out of the yeast vacuole In higher multicellular organisms it seems that many Mg2 transporting proteins await discovery The CorA domain containing Mg2 transporters CorA Alr like and Mrs2 like have a similar but not identical array of affinities for divalent cations In fact this observation can be extended to all of the Mg2 transporters identified so far This similarity suggests that the basic properties of Mg2 strongly influence the possible mechanisms of recognition and transport However this observation also suggests that using other metal ions as tracers for Mg2 uptake will not necessarily produce results comparable to the transporter s ability to transport Mg2 Ideally Mg2 should be measured directly 17 Since 28Mg2 is practically unobtainable much of the old data will need to be reinterpreted with new tools for measuring Mg2 transport if different transporters are to be compared directly The pioneering work of Kolisek 18 and Froschauer 19 using mag fura 2 has shown that free Mg2 can be reliably measured in vivo in some systems By returning to the analysis of CorA with this new tool we have gained an important baseline for the analysis of new Mg2 transport systems as they are discovered However it is important that the amount of transporter present in the membrane is accurately determined if comparisons of transport capability are to be made This bacterial system might also be able to provide some utility for the analysis of eukaryotic Mg2 transport proteins but differences in biological systems of prokaryotes and eukaryotes will have to be considered in any experiment Function editComparing the functions of the characterised Mg2 transport proteins is currently almost impossible even though the proteins have been investigated in different biological systems using different methodologies and technologies Finding a system where all the proteins can be compared directly would be a major advance If the proteins could be shown to be functional in bacteria S typhimurium then a combination of the techniques of mag fura 2 quantification of protein in the envelope membrane and structure of the proteins X ray crystal or cryo TEM might allow the determination of the basic mechanisms involved in the recognition and transport of the Mg2 ion However perhaps the best advance would be the development of methods allowing the measurement of the protein s function in the patch clamp system using artificial membranes Bacteria editEarly research edit In 1968 Lusk 20 described the limitation of bacterial Escherichia coli growth on Mg2 poor media suggesting that bacteria required Mg2 and were likely to actively take this ion from the environment The following year the same group 21 and another group Silver 22 independently described the uptake and efflux of Mg2 in metabolically active E coli cells using 28Mg2 By the end of 1971 two papers had been published describing the interference of Co2 Ni2 and Mn2 on the transport of Mg2 in E coli 23 and in Aerobacter aerogenes and Bacillus megaterium 24 In the last major development before the cloning of the genes encoding the transporters it was discovered that there was a second Mg2 uptake system that showed similar affinity and transport kinetics to the first system but had a different range of sensitivities to interfering cations This system was also repressible by high extracellular concentrations of Mg2 25 26 CorA edit Main article CorA metal ion transporter The CorA gene and its corresponding protein are the most exhaustively studied Mg2 transport system in any organism Most of the published literature on the CorA gene comes from the laboratory of M E Maguire Recently the group of R J Schweyen made a significant impact on the understanding of Mg2 transport by CorA The gene was originally named after the cobalt resistant phenotype in E coli that was caused by the gene s inactivation 25 The gene was genetically identified in E coli by Park et al 26 but wasn t cloned until Hmiel et al 2 isolated the Salmonella enterica serovar Typhimurium S typhimurium homologue Later it would be shown by Smith and Maguire 27 that the CorA gene was present in 17 gram negative bacteria With the large number of complete genome sequences now available for prokaryotes CorA has been shown to be virtually ubiquitous among the Eubacteria as well as being widely distributed among the Archaea 28 The CorA locus in E coli contains a single open reading frame of 948 nucleotides producing a protein of 316 amino acids This protein is well conserved amongst the Eubacteria and Archaea Between E coli and S typhimurium the proteins are 98 identical but in more distantly related species the similarity falls to between 15 and 20 28 In the more distantly related genes the similarity is often restricted to the C terminal part of the protein and a short amino acid motif GMN within this region is very highly conserved The CorA domain also known as PF01544 in the pFAM conserved protein domain database http webarchive loc gov all 20110506030957 http 3A pfam sanger ac uk is additionally present in a wide range of higher organisms and these transporters will be reviewed below The CorA gene is constitutively expressed in S typhimurium under a wide range of external Mg2 concentrations 29 However recent evidence suggests that the activity of the protein may be regulated by the PhoPQ two component regulatory system 30 This sensor responds to low external Mg2 concentrations during the infection process of S typhimurium in humans 31 In low external Mg2 conditions the PhoPQ system was reported to suppress the function of CorA and it has been previously shown that the transcription of the alternative Mg2 transporters MgtA and MgtB is activated in these conditions 29 Chamnongpol and Groisman suggest that this allows the bacteria to escape metal ion toxicity caused by the transport of other ions particularly Fe II by CorA in the absence of Mg2 30 Papp and Maguire offer a conflicting report on the source of the toxicity 32 nbsp The originally published TM topology of the CorA proteinThe figure not to scale shows the originally published transmembrane TM domain topology of the S typhimurium CorA protein which was said to have three membrane spanning regions in the C terminal part of the protein shown in blue as determined by Smith et al 33 Evidence for CorA acting as a homotetramer was published by Warren et al in 2004 34 In December 2005 the crystal structure of the CorA channel was posted to the RSCB protein structure database The results showed that the protein has two TM domains and exists as a homopentamer in direct conflict with the earlier reports Follow this link to see the structure in 3D The soluble intracellular parts of the protein are highly charged containing 31 positively charged and 53 negatively charged residues Conversely the TM domains contain only one charged amino acid which has been shown to be unimportant in the activity of the transporter 35 From mutagenesis experiments it appears that the chemistry of the Mg2 transport relies on the hydroxyl groups lining the inside of the transport pore there is also an absolute requirement for the GMN motif shown in red 35 36 Before the activity of CorA could be studied in vivo any other Mg2 transport systems in the bacterial host had to be identified and inactivated or deleted see below A strain of S typhimurium containing a functional CorA gene but lacking MgtA and MgtB was constructed 37 also see below and the uptake kinetics of the transporter were analysed 38 This strain showed nearly normal growth rates on standard media 50 mM Mg2 but the removal of all three genes created a bacterial strain requiring 100 mM external Mg2 for normal growth 37 Mg2 is transported into cells containing only the CorA transport system with similar kinetics and cation sensitivities as the Mg2 uptake described in the earlier papers and has additionally been quantified 38 see table The uptake of Mg2 was seen to plateau as in earlier studies and although no actual mechanism for the decrease in transport has been determined so it has been assumed that the protein is inactivated 19 Co2 and Ni2 are toxic to S typhimurium cells containing a functional CorA protein and this toxicity stems from the blocking of Mg2 uptake competitive inhibition and the accumulation of these ions inside the cell 2 Co2 and Ni2 have been shown to be transported by CorA by using radioactive tracer analysis 2 39 although with lower affinities km and velocities Vmax than for Mg2 see table The km values for Co2 and Ni2 are significantly above those expected to be encountered by the cells in their normal environment so it is unlikely that the CorA transport system mediates the uptake of these ions under natural conditions 2 To date the evidence for Mn2 transport by CorA is limited to E coli 26 Mg2 Co2 Ni2 km mM 15 30 240Vmax pmol min 108 cells 250 500 360Ki mM Mg 10Ki mM Co 50 20Ki mM Mn 30 Ki mM Ni 300 300The table lists the transport kinetics of the CorA Mg2 transport system This table has been compiled from the publications of Snavely et al 1989b 38 Gibson et al 1991 39 and Smith et al 1998a 35 and summarises the kinetic data for the CorA transport protein expressed from the wild type promoter in bacteria lacking MgtA and MgtB km and Vmax were determined at 20 C as the uptake of Mg2 at 37 C was too rapid to measure accurately Recently the Mg2 dependent fluorescence of mag fura 2 was used to measure the free Mg2 content of S typhimurium cells in response to external Mg2 which showed that CorA is the major uptake system for Mg2 in bacteria 19 The authors also showed for the first time that the changes in the electric potential DPS across the plasma membrane of the cell affected both the rate of Mg2 uptake and the free Mg2 content of the cell depolarisation suppressed transport while hyperpolarisation increased transport The kinetics of transport were defined only by the rate of change of free Mg2 inside the cells 250 mM s 1 Because no quantification of the amount of CorA protein in the membrane was made this value cannot be compared with other experiments on Mg2 transporters 18 The efflux of Mg2 from bacterial cells was first observed by Lusk and Kennedy 1969 21 and is mediated by the CorA Mg2 transport system in the presence of high extracellular concentrations of Mg2 38 The efflux can also be triggered by Co2 Mn2 and Ni2 although not to the same degree as Mg2 23 No Co2 efflux through the CorA transport system was observed The process of Mg2 efflux additionally requires one of the CorB CorC or CorD genes 39 The mutation of any single one of these genes leads to a Co2 resistance a little less than half of that provided by a CorA mutant This effect may be due to the inhibition of Mg2 loss that would otherwise occur in the presence of high levels of Co2 It is currently unknown whether Mg2 is more toxic when the CorBCD genes are deleted It has been speculated that the Mg2 ion will initially interact with any transport protein through its hydration shell 40 Cobalt III hexaammine Co III Hex is a covalently bound non labile analog for the first shell of hydration for several divalent cations including Mg2 The radius of the Co III Hex molecule is 244 pm very similar to the 250 pm radius of the first hydration shell of Mg2 This analog is a potent inhibitor of the CorA transport system more so than Mg2 Co2 or Ni2 41 The additional strength of the Co III Hex inhibition might come from the blocking of the transport pore due to the inability of the protein to dehydrate the substrate It was also shown that Co III Hex was not transported into the cells 41 suggesting that at least partial dehydration would be required for the transport of the normal substrate Mg2 Nickel II hexaammine with a radius of 255 pm did not inhibit the CorA transport system suggesting a maximum size limit exists for the binding of the CorA substrate ion 41 These results suggest that the important property involved in the recognition of Mg2 by CorA is the size of the ion with its first shell of hydration Hence the volume change generally quoted for the bare to hydrated Mg2 ion of greater than 500 fold including the second sphere of hydration may not be biologically relevant and may be a reason for the first sphere volume change of 56 fold to be more commonly used MgtA and MgtB edit The presence of these two genes was first suspected when Nelson and Kennedy 1972 25 showed that there were Mg2 repressible and non repressible Mg2 uptake systems in E coli The non repressible uptake of Mg2 is mediated by the CorA protein In S typhimurium the repressible Mg2 uptake was eventually shown to be via the MgtA and MgtB proteins 37 Both MgtA and MgtB are regulated by the PhoPQ system and are actively transcribed during the process of infection of human patients by S typhimurium 31 42 43 Although neither gene is required for pathogenicity the MgtB protein does enhance the long term survival of the pathogen in the cell 44 The genes are also upregulated in vitro when the Mg2 concentration falls below 50 mM Snavely et al 1991a Although the proteins have km values similar to CorA and transport rates approximately 10 times less the genes may be part of a Mg2 scavenging system Chamnongpol and Groisman 2002 presents evidence that the role of these proteins may be to compensate for the inactivation of the CorA protein by the PhoPQ regulon 30 The authors suggest that the CorA protein is inactivated to allow the avoidance of metal toxicity via the protein in the low Mg2 environments S typhimurium is subjected to by cells after infection The proteins are both P type ATPases 38 45 and neither gene shows any similarity to CorA The MgtA and MgtB proteins are 75 similar 50 identical although it seems that MgtB may have been acquired by horizontal gene transfer as part of Salmonella Pathogenicity Island 3 45 46 The TM topology of the MgtB protein has been experimentally determined showing that the protein has ten TM spanning helices with the termini of the protein in the cytoplasm see figure MgtA is present in widely divergent bacteria but is not nearly as common as CorA while MgtB appears to have a quite restricted distribution 47 No hypotheses for the unusual distribution have been suggested nbsp The TM topology of the MgtB proteinThe figure adapted from Smith et al 1993b 48 shows the experimentally determined membrane topology of the MgtB protein in S typhimurium The TM domains are shown in light blue and the orientation in the membrane and the positions of the N and C termini are indicated The figure is not drawn to scale While the MgtA and MgtB proteins are very similar they do show some minor differences in activity MgtB is very sensitive to temperature losing all activity with regard to Mg2 transport at a temperature of 20 C 38 Additionally MgtB and MgtA are inhibited by different ranges of cations Table A10 1 38 The table lists cation transport characteristics of the MgtA and MgtB proteins in S typhimurium as well as the kinetic data for the MgtA and MgtB transport proteins at 37 C 38 The Vmax numbers listed in parentheses are those for uptake at 20 C The inhibition of Mg2 transport by Mn2 via MgtA showed unusual kinetics see Figure 1 of Snavely et al 1989b 38 Mg2 Co2 km mM Vmax pmol min 108 cells Ki mM Co2 Mn2 Ni2 MgtA 29 115 24 40 x 30MgtB 6 75 lt 2 8 40 13The MgtA and MgtB proteins are ATPases using one molecule of ATP per transport cycle whereas the Mg2 uptake via CorA is simply electrochemically favourable Chamnongpol and Groisman 2002 have suggested that the MgtA and MgtB proteins form part of a metal toxicity avoidance system 30 Alternatively as most P type ATPases function as efflux mediating transporters it has been suggested that the MgtA and MgtB proteins act as efflux proteins for a currently unidentified cation and Mg2 transport is either non specific or exchanged to maintain the electro neutrality of the transport process 49 Further experiments will be required to define the physiological function of these proteins MgtE edit Main article Magnesium transporter E MgtE nbsp Crystal structure of magnesium transporter MgtE PDB 2zy9 50 IdentifiersSymbolMgtEPfamPF01769InterProIPR006667TCDB1 A 26OPM protein2yvxAvailable protein structures Pfam structures ECOD PDBRCSB PDB PDBe PDBjPDBsumstructure summaryTwo papers describe MgtE a fourth Mg2 uptake protein in bacteria unrelated to MgtA B or CorA 3 4 This gene has been sequenced and the protein 312 amino acids in size is predicted to contain either four or five TM spanning domains that are closely arranged in the C terminal part of the protein see figure This region of the protein has been identified in the Pfam database as a conserved protein domain PF01769 and species containing proteins that have this protein domain are roughly equally distributed throughout the Eubacteria and Archaea although it is quite rare in comparison with the distribution of CorA However the diversity of the proteins containing the domain is significantly larger than that of the CorA domain The Pfam database lists seven distinct groups of MgtE domain containing proteins of which six contain an archaic or eubacterial member The expression of MgtE is frequently controlled by a conserved RNA structure YkoK leader or M box 51 nbsp The predicted TM topology of the MgtE proteinThe figure right adapted from Smith et al 1995 4 and the PFAM database entry shows the computer predicted membrane topology of the MgtE protein in Bacillus firmus OF4 The TM domains are shown in light blue The CBS domains named for the protein they were identified in cystathionine beta synthase shown in orange are identified in the Pfam database as regulatory domains but the mechanism of action has not yet been described They are found in several voltage gated chloride channels 52 The orientation in the membrane and the positions of the N and C termini are indicated This figure is not drawn to scale This transporter has recently had its structure solved by x ray crystallography 53 The MgtE gene was first identified by Smith et al 1995 during a screen for CorA like proteins in bacteria and complements the Mg2 uptake deficient S typhimurium strain MM281 corA mgtA mgtB restoring wild type growth on standard media 4 The kinetics of Mg2 transport for the protein were not determined as 28Mg2 was unavailable As a substitute the uptake of 57Co2 was measured and was shown to have a km of 82 mM and a Vmax of 354 pmol min 1 108 cells 1 Mg2 was a competitive inhibitor with a Ki of 50 mM the Ki of Mg2 inhibition of 60Co2 uptake via CorA is 10 mM 2 A comparison of the available kinetic data for MgtA and CorA is shown in the table Clearly MgtE does not transport Co2 to the same degree as CorA and the inhibition of transport by Mg2 is also less efficient which suggests that the affinity of MgtE for Mg2 is lower than that of CorA The strongest inhibitor of Co2 uptake was Zn2 with a Ki of 20 mM 4 The transport of Zn2 by this protein may be as important as that of Mg2 Mg2 Co2 km mM Vmax pmol min 108 cells km mM Vmax pmol min 108 cells Ki Mg2 mM MgtE 82 4 at 37 C 354 4 at 37 C 50 4 at 37 C CorA 15 38 at 20 C 250 38 at 20 C 30 2 at 22 C 500 2 at 22 C 10 2 at 22 C The table shows a comparison of the transport kinetics of MgtE and CorA and key kinetic parameter values for them are listed As shown the data has been generated at differing incubation temperatures km and Ki are not significantly altered by the differing incubation temperature Conversely Vmax shows a strong positive correlation with temperature hence the value of Co2 Vmax for MgtE is not directly comparable with the values for CorA Yeast editEarly research edit The earliest research showing that yeast takes up Mg2 appears to be done by Schmidt et al 1949 However these authors only showed altered yeast Mg2 content in a table within the paper and the report s conclusions dealt entirely with the metabolism of phosphate A series of experiments by Rothstein 54 55 shifted the focus more towards the uptake of the metal cations showing that yeast take up cations with the following affinity series Mg2 Co2 Zn2 gt Mn2 gt Ni2 gt Ca2 gt Sr2 Additionally it was suggested that the transport of the different cations is mediated by the same transport system 55 56 57 58 a situation very much like that in bacteria In 1998 MacDiarmid and Gardner finally identified the proteins responsible for the observed cation transport phenotype in Saccharomyces cerevisiae 5 The genes involved in this system and a second mitochondrial Mg2 transport system functionally identified significantly after the gene was cloned are described in the sections below ALR1 and ALR2 edit Two genes ALR1 and ALR2 were isolated in a screen for Al3 tolerance resistance in yeast 5 Over expression constructs containing yeast genomic DNA were introduced into wild type yeast and the transformants were screened for growth on toxic levels of Al3 ALR1 and ALR2 containing plasmids allowed the growth of yeast in these conditions The Alr1p and Alr2p proteins consist of 859 and 858 amino acids respectively and are 70 identical In a region in the C terminal half of these proteins are weakly similar to the full CorA protein The computer predicted TM topology of Alr1p is shown in the figure The presence of a third TM domain was suggested by MacDiarmid and Gardner 1998 5 on the strength on sequence homology and more recently by Lee and Gardner 2006 59 on the strength of mutagenesis studies making the TM topology of these proteins more like that of CorA see figure Also Alr1p contains the conserved GMN motif at the outside end of TM 2 TM 2 and the mutation of the methionine M in this motif to a leucine L led to the loss of transport capability 59 The figure shows the two possible TM topologies of Alr1p Part A of the figure shows the computer predicted membrane topology of the Alr1p protein in yeast and part B shows the topology of Alr1p based on the experimental results of Lee and Gardner 2006 59 The GMN motif location is indicated in red and the TM domains in light blue The orientation in the membrane and the positions of the N and C termini are indicated the various sizes of the soluble domains are given in amino acids AA and TM domains are numbered by their similarity to CorA Where any TM domain is missing the remaining domains are numbered with primes The figure is not drawn to scale A third ALR like gene is present in S cerevisiae and there are two homologous genes in both Schizosaccharomyces pombe and Neurospora crassa These proteins contain a GMN motif like that of CorA with the exception of the second N crassa gene No ALR like genes have been identified in species outside of the fungi Membrane fractionation and green fluorescent protein GFP fusion studies established that Alr1p is localised to the plasma membrane 60 61 The localisation of the Alr1p was observed to be internalised and degraded in the vacuole in response to extracellular cations Mg2 at very low extracellular concentrations 100 mM lt 10 of the standard media Mg2 content and Co2 and Mn2 at relatively high concentrations gt 20 standard media induced the change in Alr1p protein localisation and the effect was dependent on functional ubiquitination endocytosis and vacuolar degradation 60 This mechanism was proposed to allow the regulation of Mg2 uptake by yeast However a recent report 61 indicates that several of the observations made by Stadler et al 60 were not reproducible 61 For example regulation of ALR1 mRNA accumulation by Mg2 supply was not observed and the stability of the Alr1 protein was not reduced by exposure to excess Mg2 The original observation of Mg dependent accumulation of the Alr1 protein under steady state low Mg conditions was replicated but this effect was shown to be an artifact caused by the addition of a small peptide epitope to the protein to allow its detection Despite these problems Alr1 activity was demonstrated to respond to Mg supply 61 suggesting that the activity of the protein is regulated directly as was observed for some bacterial CorA proteins 19 A functional Alr1p wild type or Alr2p overexpressed is required for S cerevisiae growth in standard conditions 4 mM Mg2 5 and Alr1p can support normal growth at Mg2 concentrations as low as 30 mM 60 57Co2 is taken up into yeast via the Alr1p protein with a km of 77 105 mM 56 C MacDiarmid and R C Gardner unpublished data but the Ki for Mg2 inhibition of this transport is currently unknown The transport of other cations by the Alr1p protein was assayed by the inhibition of yeast growth The overexpression of Alr1p led to increased sensitivity to Ca2 Co2 Cu2 La3 Mn2 Ni2 and Zn2 an array of cations similar to those shown to be transported into yeast by a CorA like transport system 5 The increased toxicity of the cations in the presence of the transporter is assumed to be due to the increased accumulation of the cation inside the cell The evidence that Alr1p is primarily a Mg2 transporter is that the loss of Alr1p leads to a decreased total cell content of Mg2 but not of other cations Additionally two electrophysiological studies where Alr1p was produced in yeast or Xenopus oocytes showed a Mg2 dependent current in the presence of the protein 62 Salih et al in prep The kinetics of Mg2 uptake by Alr1p have been investigated by electrophysiology techniques on whole yeast cells 62 The results suggested that Alr1p is very likely to act as an ion selective channel In the same paper the authors reported that Mg2 transport by Alr1p varied from 200 pA to 1500 pA with a mean current of 264 pA No quantification of the amount of protein producing the current was presented so the results lack comparability with the bacterial Mg2 transport proteins The alternative techniques of 28Mg2 radiotracer analysis and mag fura 2 to measure Mg2 uptake have not yet been used with Alr1p 28Mg2 is currently not available and the mag fura 2 system is unlikely to provide simple uptake data in yeast The yeast cell maintains a heterogeneous distribution of Mg2 63 suggesting that multiple systems inside the yeast are transporting Mg2 into storage compartments This internal transport will very likely mask the uptake process The expression of ALR1 in S typhimurium without Mg2 uptake genes may be an alternative but as stated earlier the effects of a heterologous expression system would need to be taken into account MNR2 edit The MNR2 gene encodes a protein closely related to the Alr proteins but includes conserved features that define a distinct subgroup of CorA proteins in fungal genomes suggesting a distinct role in Mg2 homeostasis Like an alr1 mutant growth of an mnr2 mutant was sensitive to Mg2 deficient conditions but the mnr2 mutant was observed to accumulate more Mg2 than a wild type strain under these conditions 64 These phenotypes suggested that Mnr2 may regulate Mg2 storage within an intracellular compartment Consistent with this interpretation the Mnr2 protein was localized to the membrane of the vacuole an internal compartment implicated in the storage of excess mineral nutrients by yeast A direct role of Mnr2 in Mg2 transport was suggested by the observation that increased Mnr2 expression which redirected some Mnr2 protein to the cell surface also suppressed the Mg2 requirement of an alr1 alr2 double mutant strain The mnr2 mutation also altered accumulation of other divalent cations suggesting this mutation may increase Alr gene expression or protein activity Recent work 61 supported this model by showing that Alr1 activity was increased in an mnr2 mutant strain and that the mutation was associated with induction of Alr1 activity at a higher external Mg concentration than was observed for an Mnr2 wild type strain These effects were observed without any change in Alr1 protein accumulation again indicating that Alr1 activity may be regulated directly by the Mg concentration within the cell MRS2 and Lpe10 edit Like the ALR genes the MRS2 gene was cloned and sequenced before it was identified as a Mg2 transporter The MRS2 gene was identified in the nuclear genome of yeast in a screen for suppressors of a mitochondrial gene RNA splicing mutation 65 and was cloned and sequenced by Wiesenberger et al 1992 66 Mrs2p was not identified as a putative Mg2 transporter until Bui et al 1999 6 Gregan et al 2001a identified LPE10 by homology to MRS2 and showed that both LPE10 and MRS2 mutants altered the Mg2 content of yeast mitochondria and affected RNA splicing activity in the organelle 67 68 Mg2 transport has been shown to be directly mediated by Mrs2p 18 but not for Lpe10p The Mrs2p and Lpe10p proteins are 470 and 413 amino acid residues in size respectively and a 250 300 amino acid region in the middle of the proteins shows a weak similarity to the full CorA protein The TM topologies of the Mrs2p and Lpe10p proteins have been assessed using a protease protection assay 6 67 and are shown in the figure TM 1 and 2 correspond to TM 2 and 3 in the CorA protein The conserved GMN motif is at the outside end of the first TM domain and when the glycine G in this motif was mutated to a cysteine C in Mrs2p Mg2 transport was strongly reduced 18 nbsp The TM topology of the MRS2 and LPE10 proteinsThe figure shows the experimentally determined topology of Mrs2p and Lpe10p as adapted from Bui et al 1999 6 and Gregan et al 2001a 67 The GMN motif location is indicated in red and the TM domains in light blue The orientation in the membrane and the positions of the N and C termini are indicated The various sizes of the soluble domains are given in amino acids AA TM domains are numbered and the figure is not drawn to scale Mrs2p has been localised to the mitochondrial inner membrane by subcellular fractionation and immunodetection 6 and Lpe10p to the mitochondria 67 Mitochondria lacking Mrs2p do not show a fast Mg2 uptake only a slow leak and overaccumulation of Mrs2p leads to an increase in the initial rate of uptake 18 Additionally CorA when fused to the mitochondrial leader sequence of Mrs2p can partially complement the mitochondrial defect conferred by the loss of either Mrs2p or Lpe10p Hence Mrs2p and or Lpe10p may be the major Mg2 uptake system for mitochondria A possibility is that the proteins form heterodimers as neither protein when overexpressed can fully complement the loss of the other 67 The characteristics of Mg2 uptake in isolated mitochondria by Mrs2p were quantified using mag fura 2 18 The uptake of Mg2 by Mrs2p shared a number of attributes with CorA First Mg2 uptake was directly dependent on the electric potential DPS across the boundary membrane Second the uptake is saturated far below that which the DPS theoretically permits so the transport of Mg2 by Mrs2p is likely to be regulated in a similar manner to CorA possibly by the inactivation of the protein Third Mg2 efflux was observed via Mrs2p upon the artificial depolarisation of the mitochondrial membrane by valinomycin Finally the Mg2 fluxes through Mrs2p are inhibited by cobalt III hexaammine 18 The kinetics of Mg2 uptake by Mrs2p were determined in the Froschauer et al 2004 paper on CorA in bacteria 19 The initial change in free Mg2 concentration was 150 mM s 1 for wild type and 750 mM s 1 for mitochondria from yeast overexpressing MRS2 No attempt was made to scale the observed transport to the amount of transporter present Protozoan Paramecium editThe transport of Mg2 into Paramecium has been characterised largely by R R Preston and his coworkers Electrophysiological techniques on whole Paramecium were used to identify and characterise Mg2 currents in a series of papers 69 70 71 72 before the gene was cloned by Haynes et al 2002 7 The open reading frame for the XNTA gene is 1707 bp in size contains two introns and produces a predicted protein of 550 amino acids 7 The protein has been predicted to contain 11 TM domains and also contains the a1 and a2 motifs see figure of the SLC8 Na Ca2 exchanger 73 and SLC24 K dependent Na Ca2 exchanger 74 human solute transport proteins The XntAp is equally similar to the SLC8 and SLC24 protein families by amino acid sequence but the predicted TM topology is more like that of SLC24 but the similarity is at best weak and the relationship is very distant 7 The AtMHX protein from plants also shares a distant relationship with the SLC8 proteins nbsp The TM topology of the XNTA proteinThe figure shows the predicted TM topology of XntAp Adapted from Haynes et al 2002 7 this figure shows the computer predicted membrane topology of XntAp in Paramecium The orientation in the membrane was determined using HMMTOP 75 76 The TM domains are shown in light blue the a1 and a2 domains are shown in green The orientation in the membrane and the positions of the N and C termini are indicated and the figure is not drawn to scale The Mg2 dependent currents carried by XntAp are kinetically like that of a channel protein and have an ion selectivity order of Mg2 gt Co2 Mn2 gt Ca2 a series again very similar to that of CorA 72 Unlike the other transport proteins reported so far XntAp is dependent on intracellular Ca2 The transport is also dependent on DPS but again Mg2 is not transported to equilibrium being limited to approximately 0 4 mM free Mg2 in the cytoplasm The existence of an intracellular compartment with a much higher free concentration of Mg2 8 mM was supported by the results Animals editThe investigation of Mg2 in animals including humans has lagged behind that in bacteria and yeast This is largely because of the complexity of the systems involved but also because of the impression within the field that Mg2 was maintained at high levels in all cells and was unchanged by external influences Only in the last 25 years has a series of reports begun to challenge this view with new methodologies finding that free Mg2 content is maintained at levels where changes might influence cellular metabolism 77 MRS2 edit A bioinformatic search of the sequence databases identified one homologue of the MRS2 gene of yeast in a range of metazoans 8 The protein has a very similar sequence and predicted TM topology to the yeast protein and the GMN motif is intact at the end of the first TM domain The human protein hsaMrs2p has been localised to the mitochondrial membrane in mouse cells using a GFP fusion protein Very little is known about the Mg2 transport characteristics of the protein in mammals but Zsurka et al 2001 has shown that the human Mrs2p complements the mrs2 mutants in the yeast mitochondrial Mg2 uptake system 8 SLC41 MgtE edit The identification of this gene family in the metazoa began with a signal sequence trap method for isolating secreted and membrane proteins 9 Much of the identification has come from bioinformatic analyses Three genes were eventually identified in humans another three in mouse and three in Caenorhabditis elegans with a single gene in Anopheles gambiae The pFAM database lists the MgtE domain as pFAM01769 and additionally identifies a MgtE domain containing protein in Drosophila melanogaster The proteins containing the MgtE domain can be divided into seven classes as defined by pFAM using the type and organisation of the identifiable domains in each protein Metazoan proteins are present in three of the seven groups All of the metazoa proteins contain two MgtE domains but some of these have been predicted only by context recognition Coin Bateman and Durbin unpublished See the pFAM website for further details The human SLC41A1 protein contains two MgtE domains with 52 and 46 respective similarity to the PF01769 consensus sequence and is predicted to contain ten TM domains five in each MgtE domain see figure which suggests that the MgtE protein of bacteria may work as a dimer nbsp The predicted TM topology of MgtE from H sapiensAdapted from Wabakken et al 2003 9 and the pFAM database the figure shows the computer predicted membrane topology of MgtE in H sapiens The TM domains are shown in light blue the orientation in the membrane and the positions of the N and C termini are indicated and the figure is not drawn to scale Wabakken et al 2003 9 found that the transcript of the SLC41A1 gene was expressed in all human tissues tested but at varying levels with the heart and testis having the highest expression of the gene No explanation of the expression pattern has been suggested with regard to Mg2 related physiology It has not been shown whether the SLC41 proteins transport Mg2 or complement a Mg2 transport mutation in any experimental system However it has been suggested that as MgtE proteins have no other known function they are likely to be Mg2 transporters in the metazoa as they are in the bacteria 9 This will need to be verified using one of the now standard experiment systems for examining Mg2 transport TRPM6 TRPM7 edit The investigation of the TRPM genes and proteins in human cells is an area of intense recent study and at times debate Montell et al 2002 78 have reviewed the research into the TRP genes and a second review by Montell 2003 79 has reviewed the research into the TRPM genes The TRPM family of ion channels has members throughout the metazoa The TRPM6 and TRPM7 proteins are highly unusual containing both an ion channel domain and a kinase domain Figure 1 7 the role of which brings about the most heated debate 79 The activity of these two proteins has been very difficult to quantify TRPM7 by itself appears to be a Ca2 channel 80 but in the presence of TRPM6 the affinity series of transported cations places Mg2 above Ca2 10 81 The differences in reported conductance were caused by the expression patterns of these genes TRPM7 is expressed in all cell types tested so far while TRPM6 shows a more restricted pattern of expression 82 An unfortunate choice of experimental system by Voets et al 2004 83 led to the conclusion that TRPM6 is a functional Mg2 transporter However later work by Chubanov et al 2004 82 clearly showed that TRPM7 is required for TRPM6 activity and that the results of Voets et al are explained by the expression of TRPM7 in the experimental cell line used by Voets et al in their experiments Whether TRPM6 is functional by itself is yet to be determined nbsp The predicted TM topology of the TRPM6 and TRPM7 proteinsThe predicted TM topology of the TPRM6 and TRPM7 proteins has been adapted from Nadler et al 2001 10 Runnels et al 2001 84 and Montell et al 2002 78 this figure shows the computer predicted membrane topology of the TRPM6 and TRPM7 proteins in Homo sapiens At this time the topology shown should be considered a tentative hypothesis The TM domains are shown in light blue the pore loop in purple the TRP motif in red and the kinase domain in green The orientation in the membrane and the positions of the N and C termini are indicated and the figure is not drawn to scale The conclusions of the Voets et al 2004 83 paper are probably incorrect in attributing the Mg2 dependent currents to TRPM7 alone and their kinetic data are likely to reflect the combined TRPM7 TRPM6 channel The report presents a robust collection of data consistent with a channel like activity passing Mg2 based on both electrophysiological techniques and also mag fura 2 to determine changes in cytoplasmic free Mg2 Paracellular transport edit Claudins allow for Mg2 transport via the paracellular pathway that is it mediates the transport of the ion through the tight junctions between cells that form an epithelial cell layer In particular Claudin 16 allows the selective reuptake of Mg2 in the human kidney Some patients with mutations in the CLDN19 gene also have altered magnesium transport 85 86 The gene Claudin 16 was cloned by Simon et al 1999 12 but only after a series of reports described the Mg2 flux itself with no gene or protein 87 88 89 The expression pattern of the gene was determined by RT PCR and was shown to be very tightly confined to a continuous region of the kidney tubule running from the medullary thick descending limb to the distal convoluted tubule 12 This localisation was consistent with the earlier reports for the location of Mg2 re uptake by the kidney Following the cloning mutations in the gene were identified in patients with familial hypomagnesaemia with hypercalciuria and nephrocalcinosis 90 91 strengthening the links between the gene and the uptake of Mg2 Plants editThe current knowledge of the molecular mechanisms for Mg2 transport in plants is very limited with only three publications reporting a molecular basis for Mg2 transport in plants 13 14 15 However the importance of Mg2 to plants has been well described and physiological and ecophysiological studies about the effects of Mg2 are numerous This section will summarise the knowledge of a gene family identified in plants that is distantly related to CorA Another gene a Mg2 H exchanger AtMHX 15 unrelated to this gene family and to CorA has also been identified is localised to the vacuolar membrane and will be described last The AtMRS2 gene family edit Schock et al 2000 identified and named the family AtMRS2 based on the similarity of the genes to the MRS2 gene of yeast 13 The authors also showed that the AtMRS2 1 gene could complement a Dmrs2 yeast mutant phenotype Independently Li et al 2001 14 published a report identifying the family and showing that two additional members could complement Mg2 transport deficient mutants one in S typhimurium and the other in S cerevisiae The three genes that have been shown to transport Mg2 are AtMRS2 1 AtMRS2 10 and AtMRS2 11 and these genes produce proteins 442 443 and 459 amino acids in size respectively Each of the proteins shows significant similarity to Mrs2p of yeast and a weak similarity to CorA of bacteria contains the conserved GMN amino acid motif at the outside end of the first TM domain and is predicted to have two TM domains The AtMRS2 1 gene when expressed in yeast from the MRS2 promoter and being fused C terminally to the first 95 amino acids of the Mrs2p protein was directed to the mitochondria where it complemented a Dmrs2 mutant both phenotypically mitochondrial RNA splicing was restored and with respect to the Mg2 content of the organelle 13 No data on the kinetics of the transport was presented The AtMRS2 11 gene was analysed in yeast in the alr1 alr2 strain where it was shown that expression of the gene significantly increased the rate of Mg2 uptake into starved cells over the control as measured using flame atomic absorption spectroscopy of total cellular Mg2 content However Alr1p was shown to be significantly more effective at transporting Mg2 at low extracellular concentrations suggesting that the affinity of AtMRS2 11 for Mg2 is lower than that of Alr1p 14 An electrophysiological voltage clamp analysis of the AtMRS2 11 protein in Xenopus oocytes also showed a Mg2 dependent current at membrane potentials DPS of 100 150 mV inside 92 These values are physiologically significant as several membranes in plants maintain DPS in this range However the author had difficulty reproducing these results due to an apparent death of oocytes containing the AtMRS2 11 protein and therefore these results should be viewed with caution The AtMRS2 10 transporter has been analysed using radioactive tracer uptake analysis 14 63Ni2 was used as the substitute ion and Mg2 was shown to inhibit the uptake of 63Ni2 with a Ki of 20 mM Uptake was also inhibited by Co III Hex and by other divalent cations Only Co2 and Cu2 inhibited transport with Ki values less than 1 mM The AtMRS2 10 protein was fused to GFP and was shown to be localised to the plasma membrane 14 A similar experiment was attempted in the Schock et al 2000 paper 13 but the observed localisation was not significantly different from that seen with unfused GFP The most likely reason for the lack of a definitive localisation of AtMRS2 1 in the Schock et al paper is that the authors removed the TM domains from the protein thereby precluding its insertion into a membrane The exact physiological significance of the AtMRS2 1 and AtMRS2 10 proteins in plants has yet to be clarified The AtMRS2 11 gene has been overexpressed from the CaMV 35S promoter in A thaliana 92 The transgenic line has been shown to accumulate high levels of the AtMRS2 11 transcript A strong Mg2 deficiency phenotype necrotic spots on the leaves see Chapter 1 5 below was recorded during the screening process in both the T1 and T2 generations for a homozygote line but this phenotype was lost in the T3 generation and could not be reproduced when the earlier generations were screened a second time The author suggested that environmental effects were the most likely cause of the inconsistent phenotype AtMHX edit The first magnesium transporter isolated in any multicellular organism AtMHX shows no similarity to any previously isolated Mg2 transport protein 15 The gene was initially identified in the A thaliana genomic DNA sequence database by its similarity to the SLC8 family of Na Ca2 exchanger genes in humans The cDNA sequence of 1990 bp is predicted to produce a 539 amino acid protein AtMHX is quite closely related to the SLC8 family at the amino acid level and shares a topology with eleven predicted TM domains Figure A10 5 There is one major difference in the sequence in that the long non membranal loop see Figure A10 5 is 148 amino acids in the AtMHX protein but 500 amino acids in the SLC8 proteins However this loop is not well conserved and is not required for transport function in the SLC8 family 15 The AtMHX gene is expressed throughout the plant but most strongly in the vascular tissue 15 The authors suggest that the physiological role of the protein is to store Mg2 in these tissues for later release when needed The protein localisation to the vacuolar membrane supports this suggestion see also Chapter 1 5 The protein transports Mg2 into the vacuolar space and H out as demonstrated by electrophysiological techniques 15 The transport is driven by the DpH maintained between the vacuolar space pH 4 5 5 9 and the cytoplasm pH 7 3 7 6 by an H ATPase 93 94 How the transport of Mg2 by the protein is regulated was not determined Currents were observed to pass through the protein in both directions but the Mg2 out current required a cytoplasmic pH of 5 5 a condition not found in plant cells under normal circumstances In addition to the transport of Mg2 Shaul et al 1999 15 also showed that the protein could transport Zn2 and Fe2 but did not report on the capacity of the protein to transport other divalent cations e g Co2 and Ni2 or its susceptibility to inhibition by cobalt III hexaammine The detailed kinetics of Mg2 transport have not been determined for AtMHX However physiological effects have been demonstrated When A thaliana plants were transformed with overexpression constructs of the AtMHX gene driven by the CaMV 35S promoter the plants over accumulated the protein and showed a phenotype of necrotic lesions in the leaves which the authors suggest is caused by a disruption in the normal function of the vacuole given their observation that the total Mg2 or Zn2 content of the plants was not altered in the transgenic plants nbsp The predicted TM topology of the AtMHX proteinThe image has been adapted from Shaul et al 1999 15 and Quednau et al 2004 73 and combined with an analysis using HMMTOP this figure shows the computer predicted membrane topology of the AtMHX protein in Arabidopsis thaliana At this time the topology shown should be considered a tentative hypothesis The TM domains are shown in light blue the orientation in the membrane and the positions of the N and C termini are indicated and the figure is not drawn to scale The a1 and a2 domains shown in green are both quite hydrophobic and may both be inserted into the membrane References edit Subramani Saranya Perdreau Dahl Harmonie Morth Jens Preben 2016 01 01 The magnesium transporter A is activated by cardiolipin and is highly sensitive to free magnesium in vitro eLife 5 doi 10 7554 eLife 11407 ISSN 2050 084X PMC 4758953 PMID 26780187 a b c d e f g h i Hmiel SP Snavely MD Miller CG Maguire ME Dec 1986 Magnesium transport in Salmonella typhimurium characterization of magnesium influx and cloning of a transport gene Journal of Bacteriology 168 3 1444 50 doi 10 1128 jb 168 3 1444 1450 1986 PMC 213658 PMID 3536881 a b Townsend DE Esenwine AJ George J Bross D Maguire ME Smith RL Sep 1995 Cloning of the mgtE Mg2 transporter from Providencia stuartii and the distribution of mgtE in gram negative and gram positive bacteria Journal of Bacteriology 177 18 5350 4 doi 10 1128 jb 177 18 5350 5354 1995 PMC 177332 PMID 7665526 a b c d e f g h Smith RL Thompson LJ Maguire ME Mar 1995 Cloning and characterization of MgtE a putative new class of Mg2 transporter from Bacillus firmus OF4 Journal of Bacteriology 177 5 1233 8 doi 10 1128 jb 177 5 1233 1238 1995 PMC 176728 PMID 7868596 a b c d e f MacDiarmid CW Gardner RC Jan 1998 Overexpression of the Saccharomyces cerevisiae magnesium transport system confers resistance to aluminum ion The Journal of Biological Chemistry 273 3 1727 32 doi 10 1074 jbc 273 3 1727 PMID 9430719 a b c d e Bui DM Gregan J Jarosch E Ragnini A Schweyen RJ Jul 1999 The bacterial magnesium transporter CorA can functionally substitute for its putative homologue Mrs2p in the yeast inner mitochondrial membrane The Journal of Biological Chemistry 274 29 20438 43 doi 10 1074 jbc 274 29 20438 PMID 10400670 a b c d e Haynes WJ Kung C Saimi Y Preston RR Nov 2002 An exchanger like protein underlies the large Mg2 current in Paramecium Proceedings of the National Academy of Sciences of the United States of America 99 24 15717 22 Bibcode 2002PNAS 9915717H doi 10 1073 pnas 242603999 PMC 137782 PMID 12422021 a b c Zsurka G Gregan J Schweyen RJ Mar 2001 The human mitochondrial Mrs2 protein functionally substitutes for its yeast homologue a candidate magnesium transporter Genomics 72 2 158 68 doi 10 1006 geno 2000 6407 PMID 11401429 a b c d e Wabakken T Rian E Kveine M Aasheim HC Jul 2003 The human solute carrier SLC41A1 belongs to a novel eukaryotic subfamily with homology to prokaryotic MgtE Mg2 transporters Biochemical and Biophysical Research Communications 306 3 718 24 doi 10 1016 S0006 291X 03 01030 1 PMID 12810078 a b c Nadler MJ Hermosura MC Inabe K Perraud AL Zhu Q Stokes AJ Kurosaki T Kinet JP Penner R Scharenberg AM Fleig A May 2001 LTRPC7 is a Mg ATP regulated divalent cation channel required for cell viability Nature 411 6837 590 5 Bibcode 2001Natur 411 590N doi 10 1038 35079092 PMID 11385574 S2CID 4426202 Walder RY Landau D Meyer P Shalev H Tsolia M Borochowitz Z Boettger MB Beck GE Englehardt RK Carmi R Sheffield VC Jun 2002 Mutation of TRPM6 causes 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