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First published online May 15, 2009
Journal of Experimental Biology 212, 1620-1629 (2009)
Published by The Company of Biologists 2009
doi: 10.1242/jeb.031534
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Review Article |
Voltage coupling of primary H+ V-ATPases to secondary Na+- or K+-dependent transporters
Whitney Laboratory for Marine Bioscience, University of Florida, 9505 Ocean Shore Boulevard, St Augustine, FL 32080, USA and Department of Physiology and Functional Genomics, and Emerging Pathogens Institute, University of Florida, Gainesville, FL 32610, USA
e-mail: wharvey{at}whitney.ufl.edu
Accepted 7 April 2009
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Summary |
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, and the pH difference between the bulk solutions on
either side of the membrane, pH. The pH term implies three
phases – a bulk fluid phase on the H+ input side, the
membrane phase and a bulk fluid phase on the H+ output side. The
Mitchell theory was applied to H+ V-ATPases largely by analogy with
H+ F-ATP synthases operating in reverse as H+ F-ATPases.
We suggest an alternative, voltage coupling model. Our model for V-ATPases is
based on Douglas B. Kell's 1979 `electrodic view' of ATP synthases in which
two phases are added to the Mitchell model – an unstirred layer on the
input side and another one on the output side of the membrane. In addition, we
replace the notion that H+ V-ATPases normally acidify the output
bulk solution with the hypothesis, which we introduced in 1992, that the
primary action of a H+ V-ATPase is to charge the membrane
capacitance and impose a across the membrane; the translocated
hydrogen ions (H+s) are retained at the outer fluid–membrane
interface by electrostatic attraction to the anions that were left behind. All
subsequent events, including establishing pH differences in the outside bulk
solution, are secondary. Using the surface of an electrode as a model, Kell's
`electrodic view' has five phases – the outer bulk fluid phase, an outer
fluid–membrane interface, the membrane phase, an inner
fluid–membrane interface and the inner bulk fluid phase. Light flash,
H+ releasing and binding experiments and other evidence provide
convincing support for Kell's electrodic view yet Mitchell's chemiosmotic
theory is the one that is accepted by most bioenergetics experts today. First
we discuss the interaction between H+ V-ATPase and the
K+/2H+ antiporter that forms the caterpillar
K+ pump, and use the Kell electrodic view to explain how the
H+s at the outer fluid–membrane interface can drive two
H+ from lumen to cell and one K+ from cell to lumen via
the antiporter even though the pH in the bulk fluid of the lumen is highly
alkaline. Exchange of outer bulk fluid K+ (or Na+) with
outer interface H+ in conjunction with (K+ or
Na+)/2H+ antiport, transforms the hydrogen ion
electrochemical potential difference,
, to a K+
electrochemical potential difference,
or a Na+
electrochemical potential difference,
. The
or
drives K+- or
Na+-coupled nutrient amino acid transporters (NATs), such as KAAT1
(K+ amino acid transporter 1), which moves Na+ and an
amino acid into the cell with no H+s involved. Examples in which
the voltage coupling model is used to interpret ion and amino acid transport
in caterpillar and larval mosquito midgut are discussed.
Key words: electrogenic, electrophoretic, protonmotive force, electrochemical potential
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Introduction |
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"The obscure we see eventually, the completely apparent takes longer."Peter Mitchell, Nobel Lecture, 1978
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Central role of the electrical potential difference as a membrane energizer in prokaryotes |
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). The pmf has
two parts, the electrical potential difference, , across the
membrane and the pH difference between the bulk solutions. The pH difference
can be expressed in volts as RT/zF ln cH
o/cH in, where cH o and
cH in refer to the hydrogen ion concentrations in the bulk
solutions outside and inside the coupling membrane, respectively. Mitchell
referred to this type of coupling as `chemiosmotic' coupling. After several
years of controversy, Mitchell's ATP synthesis by chemiosmotic coupling was
accepted by the scientific community and became regarded as an established
theory for which Mitchell was awarded the Nobel Prize in Chemistry in 1978.
However, there have always been lingering doubts regarding the pH in the bulk
fluid outside the coupling membranes, especially as applied to bacterial
plasma membranes. R. J. P. Williams pointed out that the volume of the bulk
solution outside a bacterial cell could be as large as the Pacific Ocean and
that the H+ concentration there could not be increased by expulsion
of H+ from bacteria (Williams,
1962). Williams, who was skeptical about the biologist's `membrane
concept', argued that the hydrogen ions from the electron transport system
remain within the outer regions of the ATP synthesizing entities
(Williams, 1978). Harold
(Harold, 1986) reviewed the
entire topic of localized protons outside the ATP synthesizing membranes and
observed that `in recent years, a growing number of investigators have
proposed that protons translocated during respiration may be guided to the
synthase without equilibrating with protons in the bulk phase' and notes that
`there is much interest in localized protons or protonic microcircuits'. Kell
reviewed the early literature and documented the advantages of his `electrodic
view' over Mitchell's chemiosmotic theory
(Kell, 1979).
The source of protons in the environment of alkalophilic bacteria is
especially difficult to reconcile with the chemiosmotic theory because ATP
synthesis is clearly driven by the proton electrochemical potential difference
but the H+ concentration can be as low as 10–11
mol l–1 in the bulk fluid phase (e.g.
Krulwich and Guffanti, 1989).
However, the pmf drives H+ back into the cells and expels
Na+ that leaks in from the caustic environment. A similar problem
occurs in the case of midgut alkalinization in caterpillars and larval
mosquitoes where an H+ V-ATPase uses energy from ATP hydrolysis to
drive H+ from the cells towards the lumen even though the lumen
H+ concentration can be less than 10–11 mol
l–1 (Dow,
1984; Boudko et al.,
2001).
During Na+ expulsion by alkalophilic bacteria, the hydrogen ion
electrochemical potential difference
() that is generated by the primary
electron transport system drives secondary cation exchangers such as the
Na+/2H+ antiporter, NhaA
(Krulwich et al., 1998;
Padan et al., 2005). NhaA has
been cloned, characterized, crystallized and its reaction mechanism determined
(Hunte et al., 2005;
Padan et al., 2005;
Padan et al., 2009). In the
case of caterpillar K+ secretion the
is generated by a primary
H+ V-ATPase (Wieczorek et al.,
1989), which drives a secondary K+/2H+
antiporter (Wieczorek et al.,
1991). The H+ V-ATPase is well established and widely
reviewed (e.g. Beyenbach and Wieczorek,
2006; Nelson and Harvey,
1999) and the K+/2H+ antiporter has been
well established biochemically (Azuma et
al., 1995; Grinstein and
Wieczorek, 1994; Wieczorek et
al., 1991) but only recently have attempts to clone the
K+/2H+ antiporter been fruitful as discussed below.
Membrane energization by the H+ V-ATPase is simpler to analyze than
that by the electron transport system because the source of H+s for
plasma membrane H+ V-ATPases is simply the cell cytoplasm, whereas
the source of H+s for the ATP synthase is a complex set of linked
redox reactions within inner mitochondrial, thylakoid or bacterial plasma
membranes.
Let us consider membrane energization by an H+ V-ATPase more
closely, assuming that H+ is the only ion translocated by the
V-ATPase and that electroneutrality is preserved in the bulk solutions. A
H+ V-ATPase, by itself in an ideal lipid bilayer that is
impermeable to all charged solutes and with identical bulk solutions on either
side would display but one activity upon addition of ATP: a H+
current would flow across the bilayer, charge the membrane capacitance and
stop; the charge separation between the H+ on the output side and
its former gegenion, A–, on the input side would appear as a
membrane potential difference, , with size limited by the
phosphorylation potential of ATP, ADP and inorganic phosphate (Pi)
(Mandel et al., 1975) on the
input side and the stoichiometric number of the H+ transported per
ATP hydrolyzed (Fig. 1).
Secondarily, the H+ would exchange with whatever cation is present
in the outside bulk fluid. If the outside bulk fluid is simply H2O
then exchange of H+ between the fluid–membrane interface and
bulk fluid would not change the pH; if the outside fluid were NaCl then
exchange of Na+ with H+ at the interface would acidify
the fluid (Fig. 2). If
Cl– were to follow the H+ then the output side
would be more strongly acidified. If H+ from the bulk solution were
exchanged for K+ or Na+ the output side would be
alkalinized (Fig. 3). These
deductions were made explicitly regarding H+ V-ATPases
(Harvey, 1992) and had been
implied much earlier in publications on prokaryotic ATP synthases and
Na+/H+ antiporters which were summarized in a seminal
paper by Kell (Kell, 1979).
Kell's so-called `lectrodic view' (Figs
1,
2,
3,
4) is widely cited by
bioenergeticists but largely ignored by epithelial transport
physiologists.
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drives ATP synthases in
phosphorylating membranes, Na+/2H+ antiporters in
alkalophilic bacterial plasma membranes and K+/2H+
antiporters in caterpillar apical plasma membranes (the latter two from a
compartment with H+ concentration <10–11 mol
l–1) where does the high [H+]o come
from? The three problems would have a common solution if Kell's `electrodic
view' were applied – thus, Kell's cH L would refer
to the [H+] in the bulk fluid phase outside the membrane but there
is a higher cH SL at the bulk fluid–membrane
interface (Fig. 1). (Of course,
the H+s that make up the `higher cH SL' are the same
ones that make up the , which is another objection to the pmf
concept). Direct evidence for a separate outer fluid–membrane interface
phase and an outer bulk fluid phase is provided by Cherepanov, Mulkidjanian,
Junge and associates (Cherepanov et al.,
2003; Cherepanov et al.,
2004) (for a review, see
Mulkidjanian et al., 2005).
They used light flashes to activate enzymes that capture or eject hydrogen
ions either in the outer bulk fluid or at the surface of
H+-energized plasma membranes. The light activation technique
showed that H+s reach the membrane-bound enzymes in microseconds
whereas they reach enzymes in the bulk fluid only after milliseconds; thus
H+ appears along the membrane outer-face 1000 times faster than it
appears in the bulk fluid (Mulkidjanian et
al., 2005). These experimental results imply that and
cH across the coupling membranes are more important than
pH in the inside and outside bulk solutions as the driving forces for
H+ entry coupled to Na+ exit from cells via a
Na+/nH+ antiporter. The importance of
is consistent with evidence that the much studied Escherichia
coli Na+/2H+ antiporter, EcNhaA, is electrophoretic
(Taglicht et al., 1993). As
noted above, the source of H+ and its gegenions for eukaryotic
H+ V-ATPases is more obvious than that for the electron transport
system and the remainder of this paper will focus on the identification,
isolation, and characterization of the insect primary H+ V-ATPase
and two classes of secondary electrophoretic transporters, (Na+ or
K+)/nH+ antiporters (NHAs) and Na+-
or K+-coupled nutrient amino acid transporters (NATs) that are
driven primarily by the voltage generated by H+ V-ATPases.
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H+ V-ATPases as membrane energizers in eukaryotes |
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;
Nelson, 1987); now they are
recognized to be widely distributed plasma membrane energizers
(Beyenbach and Wieczorek, 2006;
Nelson and Harvey, 1999;
Wieczorek et al., 1999)
especially in freshwater organisms and insects.
Role of the component in H+ V-ATPase-generated electrochemical forces
As discussed above a H+ V-ATPase residing by itself in an
ideally impermeable lipid bilayer would first generate a membrane potential
difference, , across the ATPase-containing membrane
(Harvey, 1992). The
translocated H+ would transiently be held at the
membrane–bulk solution interface by the electrostatic attraction of the
anion from which it was separated during H+ translocation
(Fig. 1). If the H+
concentration in the external solution were, say, 10–7 mol
l–1 (pH 7) and the Na+ concentration were
10–2 mol l–1, there would be 100,000
Na+s for every H+ bombarding the external membrane; so
H+s sequestered at the membrane–bulk solution interface would
be exchanged for Na+ from the bulk solution and the H+
electrochemical potential difference,
, would be replaced by a
Na+ electrochemical potential difference,
(see
Fig. 2). This exchange would
take time and contribute to the delayed appearance of H+ in the
bulk fluid outside H+-ejecting sources. A similar argument applies
for any other ionic species in the bulk solutions. Thus, the motive force for
any ionic species, k, is given by Gibbs's electrochemical potential, in which
,
where: µko is the standard chemical potential of k,
µk is the chemical potential of k which is given by RT
ln ck, where ck is the concentration of the
ion, z is the valency, F is Faraday's number and is
the electrical potential on each side of a membrane. The more convenient ion
`concentration' rather than `activity' can be used because the activity
coefficient can be regarded as the same on both sides of the membrane and the
ratios of activities and concentrations in the equations to follow are
identical. The driving force for any ionic species is the difference in
electrochemical potential across the membrane. To calculate it, assume that
µko is the same on both sides of the membrane and
cancels out; by convention the reference potential is outside so:
i–o. As noted above, Mitchell
called the driving force for hydrogen ions the protonmotive force (pmf) but we
will use the more explicit term `electrochemical potential difference',
µk (in volts), for any other ionic species, as
follows.
For hydrogen ions the electrochemical potential difference is
ln
(cH o/cH i) (when
µH is given as pH the `ln' must be replaced by `log') at
30°C, RT/zF ln10
60 mV so the expression becomes:
mV log
(cH o/cH i).
For sodium ions the difference in electrochemical potential is
mV log
(cNa o/cNa i).
For potassium ions it is
mV log
(cK o/cK i).
For chloride ions it is
mV log
(cCl o/cCl i).
For any ion, k, the difference in electrochemical potential is,
ln
(ck o/ck i).
Clearly the electrical potential term, , applies equally to all
ionic species. However, the chemical potential term, RT/zF
ln (ck o/ck i), would depend upon the
ionic species made available by pumps, transporters, channels or other
conductances in the membrane. As discussed above, a Cl–
channel would allow Cl– to accompany H+ into the
output bulk solution and acidify it, as in lysosomes and other intracellular
vacuoles as well as in the lumen of renal tubules and many other organs. As we
will see below, a K+/2H+ antiporter would allow the
voltage to drive two H+s back into the cells across the membrane in
exchange for one K+ and alkalinize rather than acidify the side
toward which the V-ATPase is translocating H+
(Fig. 3). Moreover, a
Na+-coupled nutrient amino acid transporter (NAT) would allow the
voltage to drive Na+ along with an amino acid into the cell with no
involvement of H+ (Fig.
4). The bottom line is that the H+ V-ATPase is a
powerful and versatile voltage generator not simply a pH gradient
generator.
The importance of plasma membrane H+ V-ATPases
The H+ V-ATPase was first isolated and characterized from
intracellular vacuoles; hence the name vacuolar-type
H+-translocating ATPase (Cidon
and Nelson, 1986; Uchida et
al., 1985). Its role in vesicle acidification was established
early so the notion that H+ V-ATPases acidify the side to which the
H+s are translocated was emphasized rather than its role in
generating . Soon after, the role of H+ V-ATPase in
energizing animal cell plasma membranes such as osteoclasts, kidney tubules,
ocular ciliary epithelium, fish gills, frog skin and more became apparent
(Nelson and Harvey, 1999;
Wieczorek et al., 1999 and
references therein). Among the clearest examples of H+
V-ATPase-voltage-driven secondary transport are the K+ pumps of
insect epithelia, especially those in Malpighian tubules, salivary glands,
sensory sensilla and midgut (Beyenbach and
Wieczorek, 2006; Harvey and
Wieczorek, 1997; Wieczorek et
al., 2009) and we will examine one of them in depth.
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K+ pumps in insect ion-transporting epithelia |
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). Simon Maddrell, John Wood, Michael O'Donnell and
colleagues studied this process for many years and developed the concept of a
`common ion pump' (Maddrell and O'Donnell,
1992; Maddrell,
1981). Simultaneously, efforts to isolate and characterize the
K+ pump were underway. Brij Gupta and Michael Berridge had located
the active K+ transport mechanism in the apical plasma membrane of
blowfly salivary glands (Gupta et al.,
1978) where they also identified transport particles similar to
those that they had first discovered in rectal papillae
(Gupta and Berridge, 1966).
Electrical studies by Küppers and Thurm located the key voltage step on
the apical membrane of cells in the Dipteran sensory sensilla, which also
contained similar particles (Küppers
and Thurm, 1979). The K+ pump had been shown earlier to
be independent of Na+ by tracer flux measurements on the isolated
and short-circuited caterpillar midgut
(Harvey and Nedergaard, 1964).
A hint that it was localized in the goblet cell apical membrane (GCAM) was the
presence of particles that Anderson and Harvey
(Anderson and Harvey, 1966)
recognized to be similar to the `elementary particles' on mitochondrial inner
membranes and to the particles discovered by Gupta and Berridge
(Gupta and Berridge, 1966).
Electrical studies showed that the K+ pump is electrogenic and
localized on the apical plasma membrane of the midgut epithelial cells (e.g.
Dow, 1992;
Moffett and Koch, 1988a;
Moffett and Koch, 1988b;
Wood et al., 1969). Intensive
studies during the 1970s were guided by the hypothesis that the postulated
K+-transport particles and their thermodynamic relationships are
similar to those of the elementary particles on mitochondrial inner membranes,
which led to the suggestion that they both be called portasomes (reviewed by
Harvey, 1980;
Harvey et al., 1981). Cioffi
and Harvey (Cioffi and Harvey,
1981) showed that the portasome-containing goblet cell apical
membranes in posterior midgut do not enclose mitochondria (which would
contaminate prospective isolates); nevertheless, posterior midgut transports
K+. Based on this information the K+-pump-containing
goblet cell apical membrane (GCAM) was isolated by a novel assay based on
ultrastructural features, mainly portasomes
(Cioffi and Wolfersberger,
1983; Harvey et al.,
1983). Dow et al. (Dow et al.,
1984) confirmed that the K+-pump is on the GCAM by
X-ray microanalysis (see Fig.
5).
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H+ V-ATPase-K+/2H+ antiporter paradigm |
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; Harvey et al.,
1983), they were frustrated because two days work yielded
sufficient enzyme for only two or three activity assays. The impasse was
broken when Helmut Wieczorek appeared at their door; he had been trying to
isolate the K+-ATPase from blowfly labella and had developed a
micro assay that enabled one to do hundreds of assays on a tiny sample. Using
Wieczorek's assay on the purified membranes the combined group determined that
the ATPase activity was much higher in the isolated GCAM fraction than in the
columnar cell apical membranes (a.k.a. microvilli, brush border membrane or
BBM), lateral membranes or basal membranes (for locations see
Fig. 5), moreover the GCAM
ATPase was stimulated by K+
(Wieczorek et al., 1986).
Abandoning sensory sensilla, Wieczorek and associates solubilized the
caterpillar GCAM ATPase and made a paradigm-altering discovery – the
GCAM ATPase is an H+ V-ATPase
(Schweikl et al., 1989;
Wieczorek et al., 1989).
Starting with Gill and Ross (Gill and
Ross, 1991) and continuing throughout the 1990s all of the
caterpillar GCAM V-ATPase subunits have been cloned, localized and
characterized (reviewed by Wieczorek et
al., 2000) and attention has shifted to its structure (reviewed by
Gruber et al., 2000),
mechanism of action and regulation (reviewed by
Beyenbach and Wieczorek, 2006;
Wieczorek et al., 2009).
The insect K+-pump is an H+ V-ATPase-K+/2H+ antiporter hybrid
Had the focus on K+ rather than H+ led the field
astray for two decades? The answer is no! K+ not H+ is
the ion that is transported across the isolated midgut and accounts for all of
the short-circuit current within experimental error
(Cioffi and Harvey, 1981);
moreover the output side is alkaline (pH 10–14) not acidic
(Dow, 1984). Then, Wieczorek
proposed the second paradigm-changing hypothesis – the H+
V-ATPase imposes a across the goblet cell apical membrane and the
drives electrophoretic K+/nH+ antiport,
explaining how K+, not H+, is transported
(Wieczorek et al., 1991).
Moffett and associates had pointed out earlier that the antiport must be
electrophoretic (Chao et al.,
1991) and Azuma et al. (Azuma
et al., 1995) showed that, indeed, the antiport stoichiometry is
one K+ for two H+.
The quest for the K+/2H+ antiporter
The quest for the insect K+ pump had taken nearly forty years,
from the Ramsay `active K+ transport' concept in 1953 to the
Wieczorek–Harvey `H+ V-ATPase-K+/2H+
antiporter' concept in 1991. Now a new quest began – to isolate the
antiporter and determine its structure and properties. The new quest would be
more difficult than the old one because, even though the antiporter is present
in the same GCAM preparation that yielded the V-ATPase there is no equivalent
of ATPase activity and portasomes to use as assay; antiporter activity must be
measured in intact membrane vesicles
(Wieczorek et al., 1991);
moreover the turnover number of secondary transporters is an order of
magnitude greater than that of primary pumps and their density is
correspondingly lower. So membrane biochemistry was replaced by molecular
biology. Wieczorek's brilliant group, especially Alexandra Lepier, and many
other groups attempted for several years to clone the gene encoding the
transporter. They were able to show that K+/2H+ antiport
is insensitive to bafilomycin, a specific V-ATPase inhibitor, but is inhibited
by amiloride or concanavalin A. Lepier et al. identified several glycosylated
polypeptides in GCAM that are not subunits of the V-ATPase and thus would be
candidates for the antiporter protein
(Lepier et al., 1994).
However, attempts to clone the gene encoding the antiporter by available
techniques were increasingly frustrating and were largely abandoned (for a
review see Grinstein and Wieczorek,
1994).
Genomes to the rescue
With the advent of the new millennium the Drosophila melanogaster
genome was published (Adams et al.,
2000) and a new strategy for cloning the antiporter emerged
– the antiporter gene must be present in a genome and the trick is to
find it. Two classes of membrane proteins, Na+/H+
exchangers (NHEs) and Na+/H+ antiporters (NHAs) were
soon characterized. Metazoan NHEs use the inwardly directed Na+
gradient established by the Na+/K+ P-ATPase to drive
Na+ into cells and expel metabolically produced H+
(Orlowski and Grinstein, 2004)
whereas bacterial NHAs use the redox-generated voltage to drive H+
into cells and Na+ out, as discussed above. Nevertheless, nothing
was known about genomic insect NHEs and NHAs so both types were candidates for
the missing antiporter.
Within a year Giannakou and Dow
(Giannakou and Dow, 2001) had
identified three Na+/H+ exchanger (NHE) genes by
cyber-screening, determined their positions relative to human and other genes
in a phylogenetic tree, identified the genes in Southern blots, determined
their primary sequences and amiloride binding regions of the encoded proteins,
determined their transcription patterns by RT-PCR and unlatched the door to
the antiporter's hiding place (Giannakou and Dow numbered the NHEs in order of
their identification). Fluxes and fluid secretion in insect Malpighian tubules
had been studied by electrophysiological methods
(Beyenbach, 1995;
Beyenbach et al., 2000) which
served as a background for molecular cloning studies by Gill and associates
that opened the door to the hiding place (reviewed by
Pullikuth et al., 2003).
Gill's group identified five genes and named them by their evolutionary
relationships to characterized vertebrate counterparts. Later Brett et al.
(Brett et al., 2005) placed
the five exchangers in broad phylogenetic context and assigned new names; all
three nomenclatures are listed in Table
1 for the reader's convenience.
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AeNHE3 (Brett's NHE2) from Aedes aegypti was the first insect NHE
to be cloned and its location identified in mosquitoes and characterized in
yeast and fibroblasts (Pullikuth et al.,
2006). The authors reported that AeNHE3 is present in basal
membranes in almost all tissues of Ae. aegypti adults but they noted
that splice variants might change the polarity of expression. They studied the
relationship of AgNHE3 to V-ATPase and concluded that it is a basal,
amiloride-insensitive mediator of transepithelial ion and fluid transport.
Then Kang'ethe et al. (Kang'ethe et al.,
2007) cloned and characterized AeNHE8 (Brett's NHE1) and reported
that it mediates amiloride-sensitive exchange across Malpighian tubules. It is
expressed in the apical membranes of Malpighian tubules, gastric caeca and
rectum. They proposed that `AeNHE8 may be coupled to the inward H+
gradient across the Malpighian tubules and plays a role in the extrusion of
excess sodium and potassium...'. However, Piermarini et al. were not able to
confirm the apical localization in Malpighian tubules
(Piermarini et al., 2009).
Mosquito NHEs are not electrophoretic plasma membrane proteins
In a detailed study of an NHE that was cloned from Ae. aegypti
adult Malpighian tubules, Piermarini, Beyenbach and associates were able to
work around the pitfalls of an endogenous conductance that is activated by
xenic cRNA and showed that AeNHE8 is an endosomal transporter
(Piermarini et al., 2009).
Using quantitative PCR (qPCR) and immunohistochemistry they showed that AeNHE8
is widely distributed in adult mosquito tissues and not especially prominent
in Malpighian tubules. That it is not a plasma membrane protein was determined
by western blots of Malpighian tubules and confirmed by labeling with an
affinity-purified antibody that is specific to AeNHE8. The intracellular
transporter was located in the principal cells in the distal, secretory region
of Malpighian tubules. The prospect that AeNHE8 is contained in vesicles that
fuse with the plasma membrane under conditions of diuresis was ruled out by
feeding mosquitoes a blood meal and application of dibutyryl-cAMP to isolated
tubules, both of which stimulate Na+ excretion but did not alter
the localization of the transporter. Efforts to characterize the exchanger
that was expressed heterologously in Xenopus laevis oocytes by
two-electrode voltage clamp techniques were frustrated by the activation of
well known Na+ conductances
(Nessler et al., 2004;
Reifarth et al., 1999;
Tzounopoulos et al., 1995).
However, Piermarini et al. were able to analyze the transporter by measuring
changes in pHi with pH-selective electrodes. The
Na+/H+ exchange was inhibited by ethyl isopropyl
amiloride (EIPA). Na+ could be replaced partially by Li+
but only poorly by K+.
Piermarini et al. provided a comprehensive review of insect NHEs and
concluded that none of the three NHEs in the Ae. aegypti genome was a
reasonable candidate for the K+/2H+ antiporter. They
noted that although NHAs have not been studied in Aedes the data from
Dow's group on Drosophila (discussed below) show that both DmNHA1 and
DmNHA2 are present on the brush border of principal cells and data from
Anopheles gambiae obtained by Harvey's group show that AgNHA1 is
present in Malpighian tubules (Okech et
al., 2008). Piermarini et al. note that `NHAs are the best
candidates for apical cation/H+ exchangers in Malpighian tubules of
Aedes'. They conclude that the potential of AgNHA1 for mediating
K+/2H+ or Na+/2H+ antiport
(Rheault et al., 2007) makes
NHAs even more attractive because they could use the high apical-membrane
voltage that is established by the H+ V-ATPase
(Day et al., 2008).
Drosophila NHAs are plasma membrane proteins
All three NHE genes are expressed in Drosophila melanogaster
Malpighian tubules (Giannakou and Dow,
2001). However, none of them appear to be expressed near V-ATPases
in plasma membranes, as revealed by a search of the FlyAtlas expression
resource (Chintapalli et al.,
2007). From their lack of success in identifying any of the NHEs
at apical plasma membranes in Drosophila, Day et al. concluded the
transporters most probably function in endosomes
(Day et al., 2008). However,
both of the two NHA genes are expressed in Drosophila
(CG10806/Nha1) and (CG31052/Nha2) in the same CPA2 (NHA)
family as bacterial electrophoretic antiporters
(Brett et al., 2005). Using
immunocytochemistry and over-expression of GFP-tagged NHA both DmNHA1 and
DmNHA1 were found to often be present in the same membrane as V-ATPases
(Day et al., 2008). These
results prompted the authors to title their paper `Identification of two
partners from the bacterial Kef exchanger family for the apical plasma
membrane V-ATPase of Metazoa'. This pattern of association between NHAs and
H+ V-ATPases is similar to that reported earlier for An
gambiae (Okech et al.,
2008; Rheault et al.,
2007; Smith et al.,
2008) and supports the notion that the voltage from electrogenic
H+ V-ATPases drives cation exchange by electrophoretic NHA.
If NHEs are not located in plasma membranes then how are metabolic acids
expelled from the cells. Since H+ V-ATPases are present and
nutrient amino acid transporters (NATs) are very likely to be present in these
cells, it has been proposed that in mosquito larval midgut V-ATPases
transporting H+ outwardly across the same membrane in which
Na+- or K+-coupled NATs are transporting Na+
inwardly, constitute NHEs; they have been called NHEVNATs
(Harvey et al., 2009) and may
be functional replacements for the missing NHEs.
Assuming that the H+ V-ATPase–K+/2H+
antiporter hypothesis is correct, the next question is – how does it
work? We assume that the couple moves K+ into the goblet cell
cavity where the H+ concentration is only 10–7.23
mol l–1 (Chao et al.,
1991) but the K+ concentration is
>10–1 mol l–1
(Dow et al., 1984)
(Fig. 5). What is the source of
the H+s that are driven from cavity to cell? The most obvious
hypothesis is that the large >240 mV membrane potential
(Dow and Peacock, 1989) across
the GCAM is equivalent to a 10,000-fold concentration difference of a
monovalent cation and can drive the electrophoretic antiport without regard to
the concentrations of H+ and K+. But the membrane
potential would also drive K+ toward the cells, placing the entire
burden for H+ re-entry on the affinity of H+ for its
binding site on the antiporter being much greater than the affinity of
K+ for its site. An alternative hypothesis is that the GCAM is like
ATP synthesizing membranes (Kell,
1979; Cherepanov et al.,
2004; Mulkidjanian and
Cherepanov, 2006) and the H+ concentration in the
unstirred layer adjacent to the membrane lining the cavity is much higher than
that in the bulk fluid.
|
 s drive K+- or Na+-amino acid symport without H+
|
|---|
) and CAATCH1 (cation amino acid transporter channel)
(Feldman et al., 2000) from
caterpillars and Na+/amino acid symport by AeAAT1i (Ae.
aegypti amino acid transporter 1)
(Boudko et al., 2005a), AgNAT6
(An. gambiae nutrient amino acid transporter 6)
(Meleshkevitch et al., 2009)
and AgNAT8 (Meleshkevitch et al.,
2006) from mosquito larvae. Details have been reviewed recently
(Harvey et al., 2009) and only
a brief summary is presented here.
Caterpillars grow more than 1,000-fold in less than a month on a leafy diet
that is rich in K+ and poor in Na+; they use amino acids
both as substrates for protein synthesis and for energy. K+ rather
than Na+ is the coupling cation but K+ gradients are
insufficient to drive the symport (Dow et
al., 1984) whereas large voltage gradients are present
(Dow and Peacock, 1989)
(Fig. 5). Amino acid uptake by
isolated caterpillar midgut is K+ dependent and voltage driven
(Nedergård, 1972). Electrophoretic K+-coupled amino acid
transport across the apical plasma membrane of wild silkworm larval posterior
midgut was demonstrated in brush border membrane vesicle studies by Giordana,
Sacchi, Parenti and associates (Giordana
et al., 1989; Hanozet et al.,
1980). Much of their work was confirmed in studies on Manduca
sexta by Wolfersberger, Harvey and associates (e.g.
Hennigan et al., 1993a;
Hennigan et al., 1993b). The
uptake is clearly driven by the voltage generated by the H+
V-ATPase in adjacent goblet cells. The Italian and American groups, joined by
Matthias Hediger, cloned KAAT1 (Castagna
et al., 1998). Soon after CAATCH1, a second cation-coupled amino
acid transporter was also cloned from caterpillar midgut
(Feldman et al., 2000).
Mosquito larvae, unlike leaf-eating caterpillars, can live on highly varied
diets found in habitats ranging from alkaline salt marshes to
alkali-ion-dilute fresh water. The pH of their alimentary canal ranges from
near neutrality in the foregut to >10.5 in anterior midgut and back to near
neutrality in posterior midgut in the absence of diffusion barriers
(Clements, 1992;
Dadd, 1975;
Ramsay, 1950). Fresh water
mosquitoes take up Na+, use it for amino acid symport in the midgut
and conserve it by reabsorption in the Malpighian tubules and hindgut
(Clements, 1992;
Ramsay, 1953b;
Smith et al., 2008). A
mosquito amino acid/Na+ symporter, AeAAT1i, that has high sequence
identify with caterpillar KAAT1 and CAATCH1, was cloned from Ae.
aegypti larvae (Boudko et al.,
2005a). More recently AgNAT8
(Meleshkevitch et al., 2006)
and AgNAT6 (Meleshkevitch et al.,
2009) were cloned from An. gambiae larvae.
A total of more than a dozen Na+-coupled amino acid transporters
have been cloned by Gill's group (Umesh et
al., 2003), Boudko and Harvey's group and others (reviewed by
Boudko et al., 2005b). When
expressed in Xenopus oocytes, the five NATs from mosquito larvae
exhibited characteristic profiles for uptake of the 20 structural amino acids.
Of most concern here, the application of amino acids induced large,
amino-acid-specific, inward Na+ currents. Evidently the
non-specific endogenous Na+ or K+ currents of oocytes
were not an overwhelming problem because the amplitude of the amino
acid-induced currents depended upon the specific amino acid, the pH of the
bathing solution and the transmembrane voltage; thus, all of the cloned NATs
appear to be electrophoretic transporters in which K+- or
Na+-coupled amino acid uptake is driven by the voltage generated by
H+ V-ATPases that are invariably present in the apical plasma
membranes in mosquito posterior midgut cells.
|
H+ V-ATPase activity interpreted by Kell's electrodic model |
|---|
 TOPSummaryIntroductionCentral role of the...H+ V-ATPases as membrane...K+ pumps in insect...H+ V-ATPase-K+/2H+ antiporter...{Delta}{Psi}s drive K+- or... H+ V-ATPase activity interpreted... References |
|---|
pH in Mitchell's three-phase chemiosmotic theory
(Mitchell, 1961;
Mitchell, 1991) refers to the
difference in H+ concentration between the outside bulk fluid (L)
and the inside bulk fluid (R) (Kell,
1979). Primary ATP synthesis and secondary
Na+/2H+ antiport in alkalophilic bacteria and
K+ or Na+ antiport in larval insect midguts are hard to
interpret by this three-phase model. By contrast, the ATP synthesis and cation
exchange are easily interpreted by Kell's five-phase electrodic model
(Kell, 1979;
Kell, 1992). Similarly,
V-ATPase energization of insect midguts is hard to interpret in terms of pH in
the bulk fluid of cells and lumen but easy to interpret by the five-phase
model (Figs 3 and
4). We postulate that the
plasma membrane H+ V-ATPase translocates H+ from the
cytoplasmic fluid (R) across the dielectric lipid bilayer (M) and charges the
transmembrane capacitance (SL versus SR) creating a membrane
potential, , with the outside of the cells positive to the inside.
The H+ is held within the outside fluid membrane interface
(Fig. 3, SL) by electrostatic
attraction to the negative gegenion that is held within the inside interface
phase (SR), but can exchange with any cation in the outside bulk fluid phase
(L) and acidify it to an extent limited by the capacitance. The
can drive an anion outwardly via a transporter or channel and drive
H+ back inwardly via a transporter such as (tentatively)
AgNHA1 (A in Figs 3 and
4) or channel in a steady-state
flow while the charge separation is maintained. The can also
drive a cation-coupled amino acid transport, e.g. via AgNAT8 (N in
Fig. 4) into the cells. This
coupling corresponds to Kell's `electrodic' coupling and might be called
`voltage coupling'. Voltage coupling across the membrane's lipid bilayer
appears to explain the H+ V-ATPase coupling process much more
clearly than Mitchell's `protonmotive force' between two bulk phases.
Complexity of membrane energization and energy utilization
In these early days of the post-genomic era discrepancies are to be
expected. Thus, the analyses of AeNHE8 by Gill's group and Beyenbach's group
both used technically sound techniques but led to very different conclusions.
Recall that Gill's group concluded that AeNHE8 (Brett's AeNHE1) is located in
apical membranes of Malpighian tubules, gastric caeca and rectum whereas
Beyenbach's group concluded that none of the three mosquito NHEs are located
in plasma membranes but play roles in endosomes instead. But Gill's people
believe that NHE8 is also localized in the apical membrane, in addition to
being present in endosomes. This discrepancy may be due to detection of
processed and unprocessed forms of NHE3. Similarly, Dow's group concluded that
Drosophila H+ V-ATPase is located in apical membranes
(Day et al., 2008), a
conclusion supported by Tripathi and associates who provided direct
electrophysiological evidence for V-ATPase-generated fluxes of H+
toward the basal membranes (Shanbhag and
Tripathi, 2009). Again, new evidence from Onken et al. (Onken et
al., 2009) shows that the apical region of the cytoplasm in epithelial cells
of anterior midgut of mosquitoes has a pH as high as 8, which will lead to a
re-evaluation of models of pH regulation in mosquito alimentary canal.
With thousands of genes in the insect genomes and discrepancies in reported
results from identical mosquitoes it is increasingly clear that the analysis
of Na+ and K+/H+ antiport (exchange) has just
begun. Circuit diagrams for ion and pH regulation systems of epithelia will
increasingly resemble those of modern color television sets whereas our
current diagrams resemble those of crystal radio sets. In an initial attempt
to deal with this complexity, explicit parameters in the 1992 version of the
voltage coupling model (Harvey,
1992) were incorporated into circuit diagrams that enabled
semi-quantitative computer simulations of ion and pH regulation as well as
amino acid uptake in the caterpillar midgut
(Martin and Harvey, 1994).
Hopefully, the wealth of new experimental data along with the new insight
provided by Kell's five-phase electrodic model will enable circuit diagrams to
become ever more sophisticated and realistic.
|
Footnotes |
|---|
|
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at the
interface is replaced by 
.
The voltage is changed but little and a steady state is established in which
H+ can recycle and Na+ can move out of the cells and
alkalinize the lumen as long as there is a K+ or Na+
salt and ATP in the inside bulk fluid. The pH of the outside bulk fluid
changes from <6.0 to >10.5 as H2CO3 is converted
to K2CO3 or Na2CO3.
