MINIREVIEW
The Rotary Machine in the Cell, ATP Synthase*,

Hiroyuki NojiDagger and Masasuke Yoshida§

From the Dagger  CREST (Core Research for Evolutional Science and Technology) "Genetic Programming" Team 13, Teikyo University Biotechnology Research Center 3F, Nogawa 907, Miyamae-ku, Kawasaki 216-0001, Japan and the § Chemical Resource Laboratory, Tokyo Institute of Technology, Yokohama 226-8503, Japan



    INTRODUCTION
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

ATP synthase, a major ATP supplier in the cell, is a rotary machine found next to the bacterial flagella motor in the biological world. This enzyme is composed of two motors, F0 and F1, connected by a common rotor shaft to exchange the energy of proton translocation and ATP synthesis/hydrolysis through mechanical rotation. Rotation of the isolated F1 motor driven by ATP hydrolysis was directly observed with an optical microscope, and its marvelous performance has been revealed. The motor rotates with discrete 120° steps, each driven by hydrolysis of one ATP molecule with nearly perfect energy efficiency. Apparently a cooperative domain bending motion of the catalytic beta  subunits initiated by ATP binding generates the torque. In the F0 motor, which we know less about, it has been proposed that torque may be generated by the large twist of one helix of F0c subunits or by the change in electrostatic forces between rigid subunits.


    ATP Synthase
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

ATP synthase is a ubiquitous enzyme that is located in the inner membranes of mitochondria, thylakoid membranes of chloroplasts, or the plasma membranes of bacteria. As implicated by the binding change mechanism proposed by Boyer (1), ATP synthase employs mechanical rotation to convert the electrochemical potential energy of protons across the membranes (Delta <A><AC>&mgr;</AC><AC>˜</AC></A> H+), built up by respiration or a photoreaction, to the chemical energy of ATP synthesis. This enzyme is comprised of two motors sharing a common rotor shaft (Fig. 1A). The F1 motor, a subcomplex of the ATP synthase corresponding to the protruding portion from the membrane, can generate rotary torque using the energy of ATP hydrolysis (Fig. 1B). Its subunit composition is alpha 3beta 3gamma 1delta 1epsilon 1 and the Mr is ~380,000. The F0 motor, a membrane-embedded subcomplex, generates torque coupled with proton movement down (Delta <A><AC>&mgr;</AC><AC>˜</AC></A> H+) (Fig. 1C). Bacterial F0 has the simplest subunit structure (a1b2c10-14(?)) with an Mr of ~150,000. The eukaryotic F0 contains several kinds of subunits. The gamma  and epsilon  of F1 constitute a rotor shaft and are attached to the F0c subunits. A stator stalk, made up of delta  and F0b2, also connects F1 and F0 keeping the stators (alpha 3beta 3 and F0a) from spinning with the rotor. Under physiological conditions where the driving force for the F0 motor is larger than that for the F1 motor, the F0 motor rotates the common shaft in its intrinsic direction so as to reverse the F1 motor enforcing the ATP synthesis (Fig. 1A). When the driving force for the F1 motor is larger, the F1 motor reverses the F0 motor to pump protons to the opposite side of a membrane.



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Fig. 1.   Schematic diagram of the ATP synthase. A, side view of the ATP synthase. ATP synthase is composed of the F1 and F0 motor sharing a common rotary shaft (gray). A stator stalk connects two motors (red) that do not slip. The F0 motor generates a rotary torque powered by the proton flow-enforcing F1 motor to synthesize ATP. The rotational direction is clockwise viewed from the membrane side. B, cross-section and side view of F1 motor. The alpha 3beta 3 cylinder hydrolyzing ATP makes an anti-clockwise rotation of the rotor part composed of the gamma  and epsilon  subunits. C, cross-section and side view of the F0 motor. Proton flow accompanies a clockwise rotation of the ring structure made of 10-14 copies of the c subunit.



    Structure of F1
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

F1 can be easily and reversibly dissociated from F0 as a soluble enzyme that only hydrolyzes ATP and is often called F1-ATPase. The catalytic sites are mainly located on the beta  subunit, but the minimum stable ATPase-active complex is the alpha 3beta 3gamma subcomplex (2). The crystal structures of alpha 3beta 3gamma of the bovine mitochondrial F1 show that three alpha s and beta s are alternatively arranged in a hexamer ring forming a large central cavity in which half of the long coiled-coil structure of gamma  is inserted (3). According to the recently reported structure of the F1-F0c complex of yeast ATP synthase (4), the other half of the coiled-coil of gamma  extends to touch the F0c subunits. The epsilon  subunit binds to the side surface of the lowest part of the coiled-coil. In ATP synthase, epsilon  also has close contact with F0c. The delta  subunit, the last subunit whose atomic structure is not known, is likely to sit on top of the alpha 3beta 3 ring (5). Three catalytic sites on the beta s are different in nucleotide binding states; the first is occupied by Mg·AMP-PNP1 (an analog of ATP), the second is occupied by Mg·ADP, and the third is empty (no bound nucleotide); these sites are termed beta T, beta D, and beta E, respectively. These structural features are quite consistent with what the binding change mechanism predicted; the three catalytic sites should be in three different nucleotide states at a given moment, and cooperative interconversion of the states causes the rotation of gamma .


    Observing the Rotation
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

To visualize the rotation, F1 molecules from a thermophilic bacterium (Bacillus strain PS3) were fixed on the glass surface of a coverslip, and a large marker, a fluorescently labeled actin filament, was attached to gamma  (Fig. 2A) (6). Dependent on ATP, the rotation of the actin filaments with a length of 1-4 µm at 0.2-10 revolutions per s was seen under an optical microscope. The rotation continued for several minutes with hundreds of revolutions. The direction of the rotation was always anti-clockwise viewed from the F0 side, consistent with the crystal structure in which one beta  undergoes transition from beta T to beta D to beta E. The F1s from Escherichia coli (7, 8) and the chloroplast (9) are also shown to be a rotary motor by applying the same technique. No obvious difference among the gamma  rotations was observed. The mechanical properties of the F1 motor described below seem to be conserved among species.



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Fig. 2.   The direct observation of the gamma  rotation in the F1 motor. A, experimental system for the observation of the gamma  rotation using an optical microscope. The F1 motor tagged with 10 His residues at the N terminus of the beta  subunit was immobilized upside down on a coverslip coated with nickel-nitrilotriacetic acid (Ni-NTA). An actin filament (green) labeled with fluorescent dyes and biotins was attached to the biotinylated gamma  subunit (gray) through streptavidin (blue). B, rotary movement of an actin filament observed from the bottom, the membrane side, with an epifluorescent microscope. Length from the axis to tip, 2.6 µm; rotary rate, 0.5 revolution per s; time interval between images, 133 ms.



    One ATP Drives 120° Step Rotation
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

Because of the hydrodynamic friction, at high ATP concentrations the rotation of an actin filament is the slowest step in the catalytic turnover. The rates of rotation of the filaments with the same length were, therefore, leveled off above 2 µM ATP. At ATP concentrations below 600 nM, the slowest step is the ATP binding and actin filaments showed a stepwise rotation; F1 waits for ATP at the fixed position, makes a 120° rotation upon arrival of the ATP, and waits for the next ATP (10). Obviously, a 120° step is a reflection of the 3-fold arrangement of the catalytic beta  subunits in the alpha 3beta 3 hexamer. The histogram of the duration time between 120° steps obeys an exponential function, and the estimated apparent rate constant of ATP binding to F1 agrees well with the rate obtained in a bulk F1 solution. This confirms that the hydrolysis of one ATP molecule suffices for making one 120° step. Interestingly, F1 occasionally makes a backward step as fast as forward steps and too fast to be ascribed to a thermal fluctuation. Presumably, the molecular machine makes a mistake in the order of ATP binding or product release.


    Torque and Energy of Rotation
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

The rotational rate became slower with an increasing filament length because of the increased viscous friction. However, when the rotary torque is calculated from the frictional drag coefficient and the rotation rate, it becomes clear that the F1 motor generates a constant torque of 40 pN·nm irrespective of the length of the actin filament (10). If the torque is produced at the beta -gamma interface at a radius of ~1 nm from the central axis of the alpha 3beta 3 hexamer, the force would amount to 40 pN. This is the highest value among reported nucleotide-driven motor proteins (3-5 pN for myosin/actin, 5 pN for kinesin/microtubule, and 14 pN for RNA polymerase/DNA) (11). The torque of 40 pN·nm × 2pi /3 radians (120°) or 80 pN·nm is the work done in a step against the viscous load. To define the free energy of the ATP hydrolysis, we purposely included 10 µM ADP and 10 mM Pi in addition to 2 mM ATP and measured the rotation rates (10). The free energy of the ATP hydrolysis under the condition is 90 pN·nm per one ATP molecule, and the energy for the observed rotation was 80 pN·nm per 120° step. Therefore, F1 works with almost perfect efficiency. The high efficiency accords with the fully reversible nature of this motor.


    Rotation without Load
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

As another probe to visualize the F1 rotation, a single fluorophore was attached to gamma , and its orientation was monitored (12). With this small marker, F1 can rotate almost without a load. Under this condition, F1 showed the 120° stepwise rotation at low ATP concentrations as seen in the experiment using an actin filament. Furthermore, the apparent rate of ATP binding is the same as that observed with actin filaments. This suggests that the torque-generating step in the ATPase catalytic cycle of F1 is not the ATP binding but step(s) after it, including the interconversion of the beta  subunit that initially accommodates ATP from the "loose" binding state to the "tight" one.


    Kinetic Framework; Bi-site or Tri-site?
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

Knowledge of the exact kinetic sequence in the catalytic turnover of F1 is the prerequisite for any models of the rotation mechanism. Three catalytic modes are recognized when F1 hydrolyzes ATP. At extremely low ATP (less than 1 nM) or a stoichiometric amount of ATP, only one ATP binds to the first catalytic site, and the hydrolyzed products are only released slowly (uni-site catalysis) (13). Uni-site catalysis is not inhibited by the cross-link between gamma  and beta  (14) and is probably, if not exclusively, a process that does not couple with rotation. Binding of a second ATP to the next catalytic site significantly promotes the release of the products at the first site (13). The apparent Km for this process is in the micromolar range (bi-site catalysis). Boyer's binding change mechanism has adopted the bi-site catalysis. We observed rotation in this ATP concentration range. It has been proposed that the third catalytic sites bind ATP to attain the maximum hydrolysis rate (tri-site catalysis). Actually, the ATPase activity of F1 is usually saturated above 100 µM ATP. Using the fluorescence of tryptophan introduced near the catalytic site of E. coli F1 as the signal of nucleotide binding, Senior's group (15) found that the change was saturated at an ATP concentration above ~100 µM and suggested that all three catalytic sites were filled by nucleotides. A similar observation has been made for the thermophilic F1 (16). However, the interpretation has been complicated by the "Mg-ADP-inhibited form," a state observed for F1s from any sources in which one of the catalytic sites is stuck with a tightly bound Mg-ADP. F1 exerting the steady state catalysis is a dynamic mixture of the inhibited and active forms, and this equilibrium is dragged to the active form by the Mg-ATP binding to the noncatalytic alpha  subunit of which the affinity is below 100 µM (17). Boyer has raised a question of whether deviation from simple kinetics at high ATP concentrations could be because of the Mg-ADP-inhibited form rather than the tri-site catalysis (18). Contrary to this, a mutant whose alpha  subunits lost the nucleotide binding ability still showed kinetics best interpreted by tri-site catalysis (19). The current results favor the tri-site catalysis as a physiological mode, but exclusive evidence is still needed to settle the argument. Noticeably, no obvious shift in the properties of the gamma  rotation was observed from 2 µM to 2 mM ATP where the transition from the bi- to tri-site catalysis should occur (10).


    Bending Motion of beta  May Drive the gamma  Rotation
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

The source of energy for the gamma  rotation is ATP hydrolysis on the beta  subunits. The conformation changes occurring in beta  during the ATPase cycle should then be responsible for (or at least closely related to) the torque generation. In the crystal structure of the mitochondrial F1, both beta T and beta D are in the closed conformation in which the C-terminal domain is lifted to the nucleotide-binding domain (3). The beta E employs the open conformation with a wide crevice between the two domains. The crystal of the isolated beta  subunit takes the open conformation,2 and the addition of a nucleotide caused the transition from the open to closed conformation (NMR) (20). The binding energy of ATP to the beta  subunit facilitates an energetically unfavorable transition from the empty to closed conformation of the beta  subunit. When beta  in F1 is fixed in the closed conformation by cross-linking, ATP hydrolysis stops (21). Thus, beta  appears to undergo a bending motion upon binding and the release of the nucleotide during catalysis. Like an automobile engine, the reciprocal motion of beta  in F1 is converted to the rotary motion of gamma . For this to occur, three beta s in F1 coordinate the motion, pushing and pulling the eccentric gamma  (22). A real time recording of the motion of the beta s simultaneously with ATP hydrolysis and gamma  rotation is a challenge to prove the above contention. Residues playing key roles in the torque generation have been sought by mutagenesis (23, 24). However, the F1 motor seems fairly robust against the mutations of the beta  subunit at the "hinge region" of the bending motion (23) and the conserved "DELSEED region" that has a contact surface with gamma  in the closed conformation (24).


    Structure of F0
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

F0 conducts proton movement across a membrane. F0a is embedded in the membrane by five transmembrane helices. A dimer of F0b is anchored to the membrane by a single transmembrane helix (25). F0c is a small hydrophobic protein with a hairpin structure, two transmembrane helices connected by a short polar loop (26). The F0c subunits are arranged in a ring structure, but agreement has not been established for the number of subunits in a ring; 10, 12, 14, and variable copies have been proposed (4, 27-29). F0a and F0b2 most likely exist outside of the F0c ring. A carboxyl group located in the middle of the C-terminal helix of F0c (glutamate in most cases but aspartate (Asp-61) in the case of E. coli) is proven to be essential for proton translocation (30). This carboxyl group is specifically labeled with dicyclohexylcarbodiimide (DCCD), and the labeled ATP synthase loses the activity of the ATP hydrolysis/synthesis coupled with proton movement (31). Genetic studies indicated that several charged residues of F0a are also essential and assumed to be components of a putative proton path of F0 (reviewed in Ref. 32).


    Is the F0c Ring a Rotor?
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

Although the assumption is widely accepted that the F0c ring rotates together with gamma  and epsilon , it has not been proven yet by experiment. Actually, we observed the ATP-driven rotation of the actin filaments attached to the F0c ring of the immobilized ATP synthase (33). However, the detergent used in the experiments impaired the integrity of the enzyme, and the DCCD-labeled enzyme showed uninhibited rotation and ATP hydrolysis. The F0c ring of the detergent-impaired ATP synthase could simply rotate by being dragged by the rotating gamma  without regard to whether the F0c ring works as a stator in the native enzyme. Other groups also reported the same results using DCCD-insensitive preparations, but they thought that the rotation of the F0c ring was proven (34). The loss of structural integrity of the ATP synthase in the detergent was unambiguously shown by the structure of the yeast ATP synthase crystals grown in detergent; the enzyme lost at least F0a and F0b2. Whether the F0c ring is a rotor or stator will be decided by demonstration of, for example, the DCCD-sensitive rotation of F0c or by a clear biochemical result such as DCCD-sensitive proton translocation by ATP synthase containing a gamma -epsilon -F0c cross-link.3


    Hints and Problems of F0 Motor
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

A monomer structure of F0c in a water-saturated organic solvent, which mimics well the native structure, was determined by NMR (26). Using this method, a large conformational change of F0c induced by deprotonation of essential Asp-61 was detected; the C-terminal helix rotates 140° as a unit with respect to the N-terminal helix, and the conformation of the loop region between two helices significantly changes (35). If a deprotonated F0c subunit is sandwiched by protonated F0c subunits in the F0c ring, the deprotonated Asp-61 comes close to the protonated Asp-61 of the adjacent F0c subunit, and proton transfer among the F0c subunits and essential Arg of F0a will occur. Although the details are unknown, the process by which the protons drive the F0 motor may be more mechanical than a simple rotational diffusion of the rigid F0c ring driven by electrostatic forces.

Related to the above contention, evolutional variation of F0c family is worth noting. Members of the F0c family in V-type ATPases, found in membranes of archaebacteria, some eubacteria, and inside-acidic vacuolar systems in eukaryotic cells, are mostly a tandemly fused dimer of prototype F0c units composed of four transmembrane helices (reviewed in Ref. 36). Interestingly, the dimer contains only a single essential carboxylate in the second helix. Because the ring structure of these double-sized c subunits in V-type ATPases is made most likely using two helices as a unit, the question arises as to how these homologues make a rotary motion with essential carboxylates having two times longer intervals. This places the restraint on any models trying to explain the common function of the ATP synthase and V-type ATPases.

The Delta <A><AC>&mgr;</AC><AC>˜</AC></A> H+ value has two components; the concentration difference (Delta pH) and the transmembrane voltage (Delta psi ). Although they are energetically equivalent, they can be kinetically different. Each proton in F0 receives the force by Delta psi and can possibly drive the F0 motor. On the contrary, Delta pH does not apply any force to each proton in F0. Using the ATP synthase from Propionegenium modestum, which utilizes Na+ instead of H+ as a coupling ion, Dimroth's group (37, 38) indicated that a certain magnitude of Delta psi is always required for ATP synthesis even when Delta pNa is a major component of Delta <A><AC>&mgr;</AC><AC>˜</AC></A> Na+. They further suggested that the ATP synthesis in the classic acid-base transition experiment cannot exclude contribution of the induced Delta psi (39). It is possible to think that beta  subunits of F1 resist the torque by the F0 motor as a strong spring, and therefore only Delta psi can wind up the strong spring of the beta  as quickly as observed.


    Perspectives
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES

ATP synthase is a rotary motor enzyme. The decisive evidence for the F1 rotation has justified Boyer's prediction in the past few years. This is not the goal but the start of new exciting studies. The central questions are how the motor generates force and how the motor is regulated. Models have been proposed. However, we think more facts are required to develop a vivid model. We know relatively little about F0. The proton-driven F0 motor remains a matter of unproved rational prediction. The direct observation of proton-driven rotation in a membrane using the lipid bilayer membrane will be a challenge but probably is not an impossible task. Of course, more atomic structures are a prerequisite to understanding the F1 and F0 motors.


    FOOTNOTES

* This minireview will be reprinted in the 2001 Minireview Compendium, which will be available in December, 2001.

The on-line version of this article (available at http://www.jbc.org) contains a supplemental video.

To whom correspondence should be addressed: Chemical Resource Laboratory, Tokyo Institute of  Technology, Yokohama 226-8503, Japan. Tel.: 81 45 924 5233; Fax: 81 45 924 5277; E-mail: myoshida@res.titech.ac.jp.

Published, JBC Papers in Press, November 15, 2000, DOI 10.1074/jbc.R000021200

2 K. Miki and M. Yoshida, unpublished result.

3 Very recently, unequivocal evidence that F0c belongs to the rotor part was obtained by linking the gamma , epsilon , and F0c subunits by disulfide bridges between cysteine residues introduced genetically at the interfaces (Tsunoda, S. P., Aggeler, R., Yoshida, M., and Capaldi, R. A. (2001) Proc. Natl. Acad. Sci. U. S. A. 98, in press). This fixing of the three subunits together had no significant effect on ATP hydrolysis, proton translocation, or ATP synthesis, and each of these functions retained sensitivity to DCCD.


    ABBREVIATIONS

The abbreviations used are: AMP-PNP, adenosine 5'-(beta ,gamma -imino)- triphosphate; pN, piconewtons; DCCD, dicyclohexylcarbodiimide.


    REFERENCES
TOP
INTRODUCTION
ATP Synthase
Structure of F1
Observing the Rotation
One ATP Drives 120°...
Torque and Energy of...
Rotation without Load
Kinetic Framework; Bi-site or...
Bending Motion of beta ...
Structure of F0
Is the F0c Ring...
Hints and Problems of...
Perspectives
REFERENCES


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