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First published online January 31, 2006
Journal of Experimental Biology 209, 577-589 (2006)
Published by The Company of Biologists 2006
doi: 10.1242/jeb.02014
Review Article |
The V-type H+ ATPase: molecular structure and function, physiological roles and regulation
1 Department of Biomedical Sciences, VRT 8004, Cornell University, Ithaca,
NY 14853, USA
2 Department of Biology/Chemistry, University of Osnabrück, 49069
Osnabrück, Germany
* Author for correspondence (e-mail: KWB1{at}CORNELL.EDU)
Accepted 24 November 2005
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Summary |
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 TOP Summary A brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
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First found in association with endosomal membranes, the V-type H+ ATPase is now also found in increasing examples of plasma membranes where the proton pump energizes transport across cell membranes and entire epithelia. The molecular details reveal up to 14 protein subunits arranged in (i) a cytoplasmic V1 complex, which mediates the hydrolysis of ATP, and (ii) a membrane-embedded V0 complex, which translocates H+ across the membrane. Clever experiments have revealed the V-type H+ ATPase as a molecular motor akin to F-type ATPases. The hydrolysis of ATP turns a rotor consisting largely of one copy of subunits D and F of the V1 complex and a ring of six or more copies of subunit c of the V0 complex. The rotation of the ring is thought to deliver H+ from the cytoplasmic to the endosomal or extracellular side of the membrane, probably via channels formed by subunit a. The reversible dissociation of V1 and V0 complexes is one mechanism of physiological regulation that appears to be widely conserved from yeast to animal cells. Other mechanisms, such as subunit-subunit interactions or interactions of the V-type H+ ATPase with other proteins that serve physiological regulation, remain to be explored. Some diseases can now be attributed to genetic alterations of specific subunits of the V-type H+ ATPase.
Key words: proton pump, molecular motor, V0 complex, V1 complex, subunit, endosomal membrane, plasma membrane, primary active transport, secondary active transport, channel-mediated transport, epithelial transport, actin, pathophysiology, genetic mutation
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A brief historical perspective |
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TOPSummaryA brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
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). On
first inspection, the absence of a prologue on the history of V-ATPases
suggests a casual omission. On reflection, nearly every investigator who had
made first observations of what eventually turned out as the V-ATPase had come
to Telluride, and a historically perspective may have seemed too early and
less exciting than the science each had come to report. Efraim Racker, who was
to have been the keynote speaker, would have offered at least some anecdotes.
But his passing away in September 1991 was a loss, and not to this symposium
alone. Today, a historical perspective seems timely and appropriate. Accordingly, we begin these pages with our attempt to review the history of the V-ATPase as we see it, and with an apology to all those who have not been mentioned and cited.
V-type H+ ATPases, also known as H+ V-ATPases and
V-ATPases, were not discovered in a single `Eureka' experiment; they were
gradually uncovered independently in various laboratories working with
animals, plants and fungi. In animal cells, adrenal medullary chromaffin
granules provided the first evidence for the existence of a proton ATPase in a
vacuolar system when Kirshner
(1962) showed that uptake of
catecholamines is an ATP-dependent process. But it would take another 13 years
before Radda and coworkers demonstrated the existence of a proton pump in the
membrane of chromaffin granules (Bashford
et al., 1975). Thereafter, reports accumulated on the
identification of ATP-driven proton transport and/or respective ATPase
activity in the membrane of organelles such as clathrin-coated vesicles,
platelet dense granules, lysosomes and chromaffin granules
(Apps and Reid, 1977;
Cidon and Nelson, 1983;
Dean et al., 1984;
Forgac et al., 1983;
Harikumar and Reeves, 1983;
Ohkuma et al., 1982;
Xie et al., 1983).
In plants, the finding of a salt- and ionophore-stimulated ATPase in
microsomes of turnips signaled the advent of a new transport pump
(Rungie and Wiskich, 1973).
An anion-stimulated ATPase activity was also observed in vacuolar membranes of
rubber trees and red beets which, curiously, was not inhibited by vanadate,
the classical inhibitor of P-type pumps
(D'Auzac, 1975;
Walker and Leigh, 1981).
Moreover, these studies suggested that a proton pump acidifies vacuolar and
lysosomal compartments. By the early 1980s, several laboratories working with
isolated microsomal or vacuolar vesicles had independently attributed the
anion-stimulated and vanadate-insensitive ATPase activity to an electrogenic
proton pump. These laboratories included those of Hager
(Hager et al., 1980), Sze
(Churchill and Sze, 1983),
Spanswick (DuPont et al.,
1982) and Taiz (Mandala et
al., 1982).
Interest in the newly found proton pump grew with reports of a vacuolar
ATPase in fungi such as yeast (Kakinuma et
al., 1981) and Neurospora
(Bowman and Bowman, 1982). By
the second half of the eighties, the purification of vacuolar ATPases from
animals, plants and fungi had revealed their multisubunit composition
(Arai et al., 1987;
Bowman et al., 1986;
Moriyama and Nelson, 1987;
Randall and Sze, 1986;
Uchida et al., 1985;
Xie and Stone, 1986). In view
of (1) the location of vacuolar ATPases in organellar membranes, where they
mediate proton transport, (2) the subunit similarity among V-ATPases from
diverse sources, (3) common inhibitor profiles, and (4) the absence of a
covalent phosphorylated intermediate in the reaction cycle, the vacuolar
ATPases were acknowledged, alongside F-type and P-type ATPases (F- and
P-ATPases), as a third family of ion-motive ATPases, to be called V-type
ATPases (Pedersen and Carafoli,
1987) or V-ATPases (Nelson,
1989). Since the eukaryotic V-ATPases all transport protons, they
are also called H+ V-ATPases or V-type H+ ATPases.
To date, impressive progress has been made in elucidating the structural,
functional and regulatory properties of V-type H+ ATPases. The
discovery of bafilomycin as a specific potent inhibitor enabled the detection
of this new proton pump in a variety of unexpected locations and with
unforeseen physiological activities
(Bowman et al., 1988). The
amino acid sequences of the complete set of subunits of several V-type ATPases
have now been deduced from cDNA cloning, and much has been learned about the
interactions between subunits, the regulation of enzyme activity, and the
assembly and targeting during biogenesis
(Nishi and Forgac, 2002).
Electron microscopic images of the V-type H+ ATPase were
obtained before they were found to show parts of this proton pump. As early as
1966, Gupta and Berridge (Gupta and Berridge, 1966) had observed repeating
structures on the cytoplasmic surface of the plasma membrane in the
iontransporting epithelium of the blowfly rectum. Similar structures were
later seen at the apical plasma membrane of goblet cells in the caterpillar
midgut of Cecropia (Anderson and
Harvey, 1966). But it would take until 1983 before these
structures were noted to resemble the catalytic sector of the mitochondrial
ATP synthase and called `portasomes'
(Harvey et al., 1983).
Portasomes were subsequently observed in vesicular membranes of many
eukaryotic cells such as the vacuolar membrane of Neurospora
(Dschida and Bowman, 1992),
acidosomes of Dictyostelium
(Nolta et al., 1991),
tonoplasts of several higher plants (Klink
and Lüttge, 1991; Moore
et al., 1991; Taiz and Taiz,
1991), bovine chromaffin granules
(Moriyama et al., 1991), and
even in plasma membranes (Brown et al.,
1987), where they were called `studs'
(Fig. 1). Since then,
additional light has been shed on the topology of V-ATPases. Transmission
electron microscopy has provided the low-resolution structures of the
holoenzyme and its subcomplexes (reviewed by
Wilkens et al., 2005).
High-resolution structural analysis by X-ray crystallography of several
subunits and subcomplexes of eukaryotic V-ATPases and their bacterial
Na+-pumping relatives are now in progress
(Drory et al., 2004;
Iwata et al., 2004;
Murata et al., 2005).
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).
Best known are the contributions made by the V-type H+ ATPase to
the acidification of intracellular compartments. In lysosomes and in vacuoles
of plants and fungi, a pH of about 5 serves the breakdown of macromolecules by
up to 40 types of acid hydrolases including proteases, glycosidases, lipases,
nucleases and phosphatases. A further function of the vacuole aided by the
V-type H+ ATPase is the regulation of cytosolic pH and the uptake
of cations such as Na+, Ca2+ and Cd2+
via H+-driven antiport
(Dietz et al., 2001). The
acidification of endocytotic and exocytotic organelles mediated by the V-type
H+ ATPase in animal cells provides optimal pH values for diverse
functions. For instance, in the endocytotic pathway the endosomal pH of 6
causes the release of ligands such as transferrin or low density lipoprotein
from their respective receptors (Johnson
et al., 1993). In the exocytotic pathway, peptides and proteins in
acidic secretory vesicles are often proteolytically processed from
pro-proteins by acid proteases to yield, for example, enkephalin or
insulin.
Next to the V-type H+ ATPase, synaptic vesicles possess
transporters for glutamate (SLC17), monoamines and acetylcholine (SLC18), and
-aminobutyrate (SLC32). What these families of vesicular solute-linked
carriers (SLC) share in common is H+-dependent transport of
neurotransmitter (Hediger et al.,
2004; Parsons,
2000). The uptake of monoamines and -aminobutyrate is
driven by the outward proton concentration difference, and the uptake of
anionic glutamate is driven by the membrane voltage, positive inside
(Moriyama et al., 1992). Both
proton concentration difference and membrane voltage are generated by the
V-type H+ ATPase.
The V-type H+ ATPase also supports important functions in
protozoans. In Paramecium, the proton pump is located in the
decorated spongiome of radial arms that extend from the contractile vacuole
complex (Fok et al., 1995).
Concanomycin, an inhibitor of V-type H+ ATPases, significantly
decreases the rate of fluid uptake by the contractile vesicle complex,
suggesting that the proton pump serves volume regulation in
Paramecium (Gronlien et al.,
2002). In the malaria parasite Plasmodium, the V-type
H+ ATPase occurs not only in the membranes of cell organelles but
also in the plasma membrane, where it may be involved, among other functions,
in energizing the secondary transport of diverse solutes
(Moriyama et al., 2003). What
is more, the Plasmodium-encoded V-type H+ ATPase is
exported to the cytoplasm of the host erythrocyte and targeted to the plasma
membrane, where it has a role in maintaining the intracellular pH of the
infected erythrocyte (Marchesini et al.,
2005).
Located in plasma membranes of cells, the V-type H+ ATPase can
acidify the extracellular compartment that serves a number of roles: the
resorption of bone by osteoclasts
(Schlesinger et al., 1997),
the maturation and storage of sperm in the epididymal lumen
(Breton et al., 1996), the
reabsorption of bicarbonate in renal proximal tubules
(Wagner et al., 2004), the
urinary acidification in the distal nephron
(Al Awqati, 1996), and the
regulation of pH in the inner ear
(Stankovic et al., 1997).
Even frog skin, the hallmark epithelium of Na+/K+-ATPase
driven epithelial transport, has been found to use the plasma membrane V-type
H+ ATPase to secrete H+ and absorb Na+ across
the epithelium (Ehrenfeld and Klein,
1997). Freshwater crustaceans, amphibians and fish employ the
V-type H+ ATPase in osmoregulation
(Kirschner, 2004). Located in
the plasma membrane, the proton pump is implicated in transepithelial
Cl- absorption across the gill of freshwater crab
(Weihrauch et al., 2004) and
in transepithelial Na+ absorption across the gill of freshwater
fish via channels and/or carriers that are ultimately dependent on
the V-type H+ ATPase
(Kirschner, 2004;
Wilson et al., 2000).
Metastasizing cells are thought to use the V-type H+ ATPase in
the plasma membrane to acidify the extracellular fluid, with the effect of
destroying normal tissue in advance of the invading tumor
(Sennoune et al., 2004). The
fusion of viral and endosomal membranes that delivers the viral genome to the
cytoplasm is dependent on the V-type H+ ATPase
(Perez and Carrasco,
1994).
When anion channels are absent in membranes inhabited by the V-type
H+ ATPase, acidification is much reduced
(Harvey, 1992). Under this
condition the proton pump generates large membrane voltages at small
pH, driving a diversity of electrogenic secondary active transport
systems such as nH+/cation antiport or nH+/oligopeptide
symport (Grinstein and Wieczorek,
1994; Leibach and Ganapathy,
1996).
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Molecular architecture and mechanistic interpretations |
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TOPSummaryA brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
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). In general, F-ATPases produce ATP and V-ATPases consume ATP
in eukaryotic cells. In principle, the function of both ATPases is reversible
(Hirata et al., 2000). ATP is
synthesized when the ionic electrochemical potential is greater than the free
energy of ATP hydrolysis. In contrast, when the free energy of ATP hydrolysis
is greater than the ionic electrochemical potential, the hydrolysis of ATP
drives the uphill transport of ions. The V- and F-ATPases are multisubunit proteins of up to 14 different polypeptides, which assemble as two major ring structures: (1) a peripheral V1 or F1 complex (400-600 kDa) that interacts with ATP, ADP and inorganic phosphate, and (2) an integral membrane V0 or F0 complex (150-350 kDa) that mediates the transport of H+ or Na+. In the case of eukaryotic V-type H+ ATPases, the V1 complex is invariably present in the cytoplasm such that the pump transports H+ into vesicles and vacuoles when expressed in endosomal membranes and into the extracellular fluid when expressed in the plasma membrane.
By convention, the subunits of V1 and V0 complexes
are distinguished with large and small letters respectively
(Fig. 2). The V1
complex consists of: (1) a globular headpiece with three alternating copies of
subunits A and B that form a ring, (2) a central rotational stalk composed of
single copies of subunits D and F, and (3) a peripheral stalk made of subunits
C, E, G and H. Subunits A and B mediate the hydrolysis of ATP at three
reaction sites associated with subunit A. Both the central rotational stalk
and fixed peripheral stalk connect the V1 complex with the
V0 complex (Fig. 2).
The fixed peripheral stalk holds the V1 complex in place, aided in
part by subunits B and C of the V1 complex that bind to actin.
Subunit C alone is capable of binding monomeric actin as well as cross-linking
and stabilizing actin filaments. The proton-transporting V0 complex
consists of six or more c subunits, also forming a ring structure
(Fig. 2). As many as 10
subunits form a concave ring structure in the eubacterial V-type
Na+ ATPase of Enterococcus hirae
(Murata et al., 2005).
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A functional model that is widely accepted considers the V-type H+ ATPase to consist of a stationary and a mobile part, the stator and rotor, respectively. The rotor consists of subunits D, F and the ring of subunits c (Fig. 2B). The remaining structures are considered the stator. The function of the V0 subunits d and e remains enigmatic.
How rotation of the rotor mediates the linear transfer of H+
across the membrane is hypothetically constructed in
Fig. 2, based on the innovative
models proposed for the F-ATPases (Feniouk
et al., 2004; Junge et al.,
1997; Junge et al.,
2001) and V-ATPases (Grabe et
al., 2000; Murata et al.,
2005). Fundamental to the model are (1) two H+
half-channels across the membrane, provided by subunit a in close proximity to
the c-ring, (2) a H+ binding site on each c subunit of the c-ring,
and (3) the rotation of the c-ring driven by the hydrolysis of ATP
(Fig. 2). The inner half
channel of subunit a is thought to allow cytoplasmic H+ to access
and bind to one subunit of the c-ring. After the nearly 360° rotation of
the c-ring, clockwise when viewed from the cytoplasm
(Meier et al., 2005),
H+ can unbind and exit the membrane through the outer half channel
(Fig. 2B). Variations of this
model have been proposed. For example, inlet and outlet half channels are
thought to be located in stator and rotor, respectively, in the
F1F0-ATPase of the anaerobic bacterium
Propionigenium modestum (Xing et
al., 2004), and another model
(Aksimentiev et al., 2004)
proposes swiveling motions of individual helices of subunit c as well as the
rotation of the entire c-ring.
As to the number of protons transported per ATP consumed, coupling ratios
determined for V-type H+ ATPases agree on 2H+/1ATP
(Tomashek and Brusilow,
2000). The 2:1 functional stoichiometry is consistent with the
structural stoichiometry of six binding sites for H+ on the c-ring
of the V0 complex and three sites binding sites for ATP on the
V1 complex (Fig. 2).
Moreover, F-ATPases can be observed to hydrolyze three ATP molecules with each
revolution of the rotor (Yasuda et al.,
1998). Nevertheless, coupling ratios must be neither integral nor
constant (Junge and Nelson,
2005; Murata et al.,
2005; Tomashek and Brusilow,
2000).
Clever experiments have visualized the rotation of the central stalk in the
bacterial ATP synthase (Noji et al.,
1997). In brief, the catalytic F1 complex was
immobilized upside down via a His-tag on a coverslip, and a
fluorescent actin filament was attached to the central stalk via
streptavidin. Adding ATP triggered the rotation of the fluorescent actin
filament and the stalk. Furthermore, the reversibility of this motor was
demonstrated by constructing a `molecular sparkler'
(Itoh et al., 2004). Here, a
magnetic bead rather than fluorescent actin was attached to the central stalk.
The bead was then rotated using an external magnet. The medium contained
luciferin and luciferase such that one photon was emitted upon each capture
and hydrolysis of ATP newly formed with each rotation. Rotation of the
magnetic bead in one direction increased the number of chemiluminescent
photons beyond those observed upon rotation in the opposite direction, proving
vectorial ATP synthesis. The rotation of a eubacterial V1 complex
has now also been visualized with the aid of flurorescent actin filaments
(Imamura et al., 2003),
leaving little doubt that rotational catalysis is the mechanism of both F- and
V-ATPases in vivo.
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Energizer of endosomal membranes, plasma membranes and whole epithelia |
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TOPSummaryA brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
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). In subapical membrane vesicles of the renal proximal
tubule, the V-type H+ ATPase colocalizes with ClC-5 that once was
thought to be a voltage-gated Cl- channel
(Jentsch et al., 2002). Today
ClC-5, ClC-4, and possibly other endosomal Cl- transporters are
considered electrogenic Cl-/H+ exchangers
(Scheel et al., 2005). The
collaboration between the V-type H+ ATPase and the
Cl-/H+ exchanger ClC-5 is thought to be fundamental to
(1) the recycling of apical membrane proteins such as megalin, the
Na+/Pi cotransporter, the Na+-dependent
D-glucose cotransporter SGLT, and other transporters, and (2) the endocytotic
reabsorption of filtered proteins in renal proximal tubules
(Fig. 3B). Loss of function
mutation in the Cl-/H+ exchanger ClC-5 produces the
signs of Dent's disease and Fanconi-like syndrome, which include not only the
renal loss of low molecular mass proteins, but also calcium, phosphate,
glucose, salt and water (Jentsch et al.,
2002). A defective Cl-/H+ exchanger is expected to hyperpolarize the endocytotic membrane, bringing its voltage towards the electromotive force of the V-type H+ ATPase with the effect of reducing both H+ and Cl- transport into the vesicle. Vesicular acidification would thereby be reduced, with possible negative effects on trafficking the vesicle in the endocytotic pathway.
In synaptic regions of neurons, the pas-de-deux of the V-type H+
ATPase and the H+/neurotransmitter antiporter of the VMAT-type
(vesicular monoamine transporter, SLC18)
(Eiden et al., 2004) is
responsible for accumulating and storing neurotransmitters such as serotonin,
dopamine, adrenaline, noradrenaline and histamine
(Fig. 3C). Here the V-type
H+ ATPase generates (1) a vesicular pH about 1.4 pH lower
than cytoplasm pH, and (2) a membrane voltage of 40 mV (positive inside).
Since VMAT exchanges 2 H+ ions for each serotonin
(Parsons, 2000), the
pH concentrates serotonin (S+) 630-fold in the vesicle:
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and the membrane voltage concentrates serotonin 4.8-fold in the vesicle:
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where 26 mV is the product RT/zF (R, gas constant; T, temperature; z, valence; F, Faraday constant). Together, chemical and electrical potentials yield a total 3000-fold concentration difference. If the serotonin concentration in the cytoplasm is 10 µmol l-1, then the vesicular serotonin concentration can reach a maximal value of about 30 mmol l-1 as the 2H+/S+ antiporter goes to electrochemical equilibrium. Due to intravesicular association, the serotonin concentration may reach values up to 100 mmol l-1 in the vesicle.
The observation of electrogenic H+ secretion dependent on
metabolism in the turtle urinary bladder gave the first hint of an
ATP-dependent proton pump in a plasma membrane
(Al Awqati, 1978). The
characterization of this proton pump in membrane fractions of the turtle
bladder (Gluck et al., 1982)
and mammalian kidney (Gluck and Al Awqati,
1984) revealed striking functional similarities with proton pumps
of vacuolar membranes. Striking structural similarities with the V-type
H+ ATPase of yeast were observed upon the isolation of the kidney
proton pump (Gluck and Caldwell,
1987; Gluck and Caldwell,
1988). Antibodies prepared against the isolated kidney proton pump
confirmed its location in the apical plasma membrane of epithelial cells
(Brown et al., 1987).
Wieczorek et al. (1991)
were the first to recognize that the V-type H+ ATPase can energize
secondary active transport across the plasma membrane. As shown in
Fig. 4A, the V-type
H+ ATPase (and not the Na+/K+ ATPase) was
found to power the active transport of K+ via
nH+/K+ antiport in a highly purified preparation of the
apical membrane of the midgut of the tobacco hornworm Manduca sexta.
In mammals, the association of the V-type H+ ATPase with
Cl- channels in the ruffled membrane of osteoclasts
(Fig. 4B) is known to secrete
the strong acid HCl that serves the digestion and remodeling of bone
(Chatterjee et al., 1992;
Cleiren et al., 2001;
Schlesinger et al., 1997). In
renal proximal tubules, H+ secreted into the tubule lumen by the
apical membrane V-type H+ ATPase is thought to account for 40% of
HCO3- reabsorption via the formation of
CO2 (Wagner et al.,
2004). In addition, the transmembrane H+
electrochemical potential drives H+-oligopeptide cotransport
via PEPT1 and PEPT2 (Fig.
4C). In the renal medulla, the V-type H+ ATPase
contributes to urinary acidification when the proton pump is expressed in the
apical membrane of 
-intercalated cells, and it contributes to urinary
alkalinization when the proton pump is expressed in the basolateral membrane
of ß-intercalated cells (Brown and
Breton, 1996).
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The laboratory of Beyenbach has extended the concept of energizing plasma
membranes by the V-type H+ ATPase to energizing whole epithelia
(Beyenbach, 2001). Malpighian
tubules of the yellow fever mosquito Aedes aegypti express the V-type
H+ ATPase at the apical membrane of principal cells
(Fig. 5). The tubules have no
measurable activity of the Na+/K+ ATPase. Instead, most
ATPase activity stems from the V-type H+ ATPase
(Weng et al., 2003). The
electromotive force of the proton pump (Ep,
Fig. 5) serves largely to
polarize the apical membrane to voltage that on average is 111 mV (negative
inside). The small transmembrane proton concentration difference (pH
0.16) supports H+ transport from cell to tubule lumen, i.e.
opposite to the gradient needed to drive outward Na+ and
K+ (cat+) transport via exchange transport with
H+ (Petzel et al.,
1999). Since electroneutral antiport is insensitive to membrane
voltage, an electrogenic antiporter that exchanges 2H+ for each
Na+ or K+ would overcome the outward directed proton
gradient and take advantage of the high apical membrane voltage generated by
the V-type H+ ATPase (Fig.
5). At the prevailing pH and voltage difference across the apical
membrane, an antiport stoichiometry of 2H+/cat+ would
generate luminal K+ and Na+ concentrations approximately
40 times higher than their respective concentrations in the cell:
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The apical membrane voltage generated by the V-type H+ ATPase
also drives paracellular Cl- transport and the entry of
K+ into the cell across the basolateral membrane. In brief,
positive current carried by H+ across the apical membrane must
return to the cytoplasmic face of the pump. Positive pump current returning to
the peritubular side of the epithelium is carried by Cl- passing in
the opposite direction through the paracellular pathway as the mechanism of
paracellular Cl- secretion
(Pannabecker et al., 1993).
Positive current carried by K+ and Na+ across the
basolateral membrane completes the electrical circuit
(Masia et al., 2000;
Sawyer and Beyenbach, 1985).
Similar patterns of coupling the electromotive force of the proton pump
located at the apical membrane to transport across the basolateral membrane
are likely to be found in other epithelia.
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Regulation of the V-type H+ ATPase |
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TOPSummaryA brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
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). Alone, the native V1 complex does not hydrolyze
ATP in the presence of cytosolic Mg2+ concentrations
(Gräf et al., 1996), and
free V0 complexes normally do not allow the passage of protons
(Beltran and Nelson, 1992;
Zhang et al., 1992). The
dissociation of the holoenzyme was subsequently confirmed in yeast, where
glucose deprivation for as little as 5 min triggered the dissociation of 70%
of holoenzyme (Kane, 1995).
The addition of glucose reversed the process, bringing about the reassembly of
V0 and V1 complexes. Holoenzyme association/dissociation
is now thought a universal regulatory mechanism of V-ATPases
(Fig. 6).
|
).
Though glucose-induced, the RAVE-mediated reassembly is not glucose-dependent,
because RAVE binds to V1 whenever it is present in the cytosol. In
contrast, glucose dramatically increases the interaction of the V-ATPase with
the glycolytic enzyme aldolase (Lu et al.,
2004). It appears that aldolase uses three different sites to bind
respectively to subunits B and E of the V1 complex and to subunit a
of the V0 complex, thereby facilitating the assembly of the
holoenzyme. Thus, glucose stimulates the aldolase-mediated assembly of
holoenzyme. In this role aldolase acquires the additional function as glucose
sensor for regulating the activity of V-type H+ ATPase activity
(Lu et al., 2004).
Other mechanisms for triggering the assembly of holoenzyme may abound. For
example, in renal epithelial cells, glucose activates phosphatidylinositol
3-kinase dependent signaling and the assembly of V1 and
V0 complexes (Sautin et al.,
2005). Still, the molecular details for enhancing the reassembly
of holoenzyme by RAVE, aldolase and kinase(s) remain to be elucidated. Also
intriguing are the molecular mechanisms that couple glucose withdrawal to
V1-V0 dissociation, since apparently conventional signal
transduction pathways are not activated by glucose depletion
(Parra and Kane, 1998).
Though hormones can activate the assembly of holoenzyme, the molecular
details are unknown. For example, it has been known for decades that
transepithelial secretion of a KCl-rich primary saliva in the blowfly
Calliphora is stimulated by serotonin
(Berridge et al., 1976).
Apparently, the serotonin-induced increase in cyclic AMP (cAMP) activates an
electrogenic K+ transport mechanism
(Berridge et al., 1976) that
today is thought to derive from the V-type H+ ATPase working in
parallel with a K+/H+ antiporter
(Wieczorek et al., 1999).
Immunofluorescent labeling of different V-ATPase subunits, as well as
measurements of enzyme activity, have shown that serotonin recruits
V1 subunits from the cytosol, consistent with the assembly of the
V1V0 holoenzyme
(Zimmermann et al., 2003). In
Malpighian tubules of insects, where intracellular second messengers of
diuresis and antidiuresis have been identified, it remains unknown whether
cAMP, cGMP, Ca2+ and NO affect the disassembly/reassembly of the
V1V0 holoenzyme.
Subunit C of the V1 complex is unique among V-ATPase subunits in
that it is released from the V1 complex upon its dissociation from
the V0 complex (Gräf et
al., 1996; Kane,
1995; Merzendorfer et al.,
2000; Vitavska et al.,
2003). Recent studies suggest that subunit C may play a central
role in holoenzyme disassembly/reassembly. Subunit C appears to bridge the
V1 and V0 complexes, binding to subunits E and G of the
V1 complex and to subunit a of the V0 complex
(Inoue and Forgac, 2005).
Subunit C is thus a good candidate for modulating the stability of the
V1V0 holoenzyme. Indeed, the structural changes observed
in subunit C in yeast and Arabidopsis may depend on the ATP/ADP ratio
(Armbrüster et al., 2005).
Since this ratio can be influenced by the availability of glucose, subunit C
might also serve indirectly as a glucose sensor, responding to changing
concentrations of glucose with conformational changes, which in turn affect
the stability of the V1V0 holoenzyme.
Subunit C of the caterpillar midgut of Manduca sexta binds with
high affinity to actin filaments, either as an isolated protein, as subunit of
the V1V0 holoenzyme, or reconstituted into the
V1 complex (Vitavska et al.,
2003). Morevoer, subunit C, occurring in micromolar concentrations
in the cytosol, cross-links actin filaments and even binds monomeric G-actin
(Vitavska et al., 2005).
F-actin crosslinking is likely to stabilize actin filament bundles in the
apical microvilli of goblet cells of Manduca sexta. In addition,
subunit C may play an important role in controlling the dynamics of the actin
cytoskeleton because it binds F-actin and G-actin
(Vitavska et al., 2005).
Furthermore, F-actin binding to subunits B and C of the membrane-embedded
V1V0 holoenzyme could serve to stabilize the stator
(Fig. 2). In the intact cell,
this hypothetical novel function of F-actin may strengthen the stator to
withstand the torque generated by the rotor.
|
Subunit knockouts, gene mutations and some diseases |
|---|
|
TOPSummaryA brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
|---|
).
Since then, the same lethal effect has been demonstrated for every knock-out
of a V-ATPase single-copy gene in yeast
(Nelson, 2003). A lethal
effect after knockout of the gene encoding subunit A was also observed for
Neurospora (Ferea and Bowman,
1996). Later on it was shown that, as in yeast, lethality occurred
only at physiological pH values slightly above 7; at acidic pH values (<pH
6) Neurospora was able to survive
(Bowman et al., 2000).
Inactivation of single-copy genes encoding subunit A in
Neurospora, subunit B in Drosophila, and subunit c in mice
also resulted in lethal phenotypes (Davies
et al., 1996; Ferea and
Bowman, 1996; Inoue et al.,
1999).
When more than one gene encodes a V-ATPase subunit, different subunit
isoforms are usually found at different locations. In yeast, one of the two
isoforms of subunit a is targeted to the vacuolar membrane, whereas the second
isoform is targeted to the late Golgi apparatus
(Kawasaki-Nishi et al., 2001).
In multicellular higher eukaryotes, different isoforms often show cell-type or
tissue-specific locations. For example, in mammals different isoforms of
several subunits have been selectively identified in the kidney
(Oka et al., 2001;
Smith et al., 2002;
Sun-Wada et al., 2003a;
Sun-Wada et al., 2003b),
inner ear (Dou et al., 2003),
brain (Murata et al., 2002),
osteoclasts (Manolson et al.,
2003), alveolar cells
(Sun-Wada et al., 2003a;
Sun-Wada et al., 2003b) and
the acrosome (Sun-Wada et al.,
2002). Genetic defects in a tissue-specific isoform must not
necessarily result in a lethal phenotype, but it may give rise to inherited
disorders.
Mutations in the genes encoding the kidney-specific isoforms B1 and a4 are
partly responsible for inheritable forms of distal renal tubular acidosis,
characterized by elevated H+ and Cl- concentrations in
the plasma due to the impaired renal excretion of acid
(Karet et al., 1999;
Smith et al., 2000). Gene
mutations of subunits B1 and a4 in the cochlea can result in sensorineural
deafness, evidently due to impaired contractile responses of hair cells
(Karet et al., 1999;
Stover et al., 2002).
Mutations in the gene encoding subunit a3 lead to one type of infantile
malignant autosomal recessive osteopetrosis, a disease where the bone
progressively hardens due to reduced osteoclast activity
(Frattini et al., 2000;
Susani et al., 2004). In
contrast to the tissue-specific isoforms B1 and a4, a3 is found in all
mammalian tissues so far examined (Nishi
and Forgac, 2000). In osteoclasts, a3 is part of the V-type
H+ ATPase inhabiting the ruffled border membrane
(Fig. 4B) while a1 appears to
be restricted to endomembranes, leading to the suggestion
(Toyomura et al., 2000) that
V-ATPases housing the a3 isoform in transport vesicles may interact with
microtubules to be carried to the ruffled border membrane. Thus, a defect in
the gene encoding a crucial site in subunit a3 may impair the targeting of the
holoenzyme from the endosomal system to the ruffled border in osteoclasts.
|
Concluding thoughts |
|---|
|
TOPSummaryA brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
|---|
). |
Acknowledgments |
|---|
|
References |
|---|
|
TOPSummaryA brief historical perspectiveMolecular architecture and...Energizer of endosomal...Regulation of the V-type...Subunit knockouts, gene...Concluding thoughtsReferences |
|---|
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