Role of Charged Residues in the Catalytic Sites of Escherichia coli ATP Synthase

Here we describe the role of charged amino acids at the catalytic sites of Escherichia coli ATP synthase. There are four positively charged and four negatively charged residues in the vicinity of of E. coli ATP synthase catalytic sites. Positive charges are contributed by three arginine and one lysine, while negative charges are contributed by two aspartic acid and two glutamic acid residues. Replacement of arginine with a neutral amino acid has been shown to abrogate phosphate binding, while restoration of phosphate binding has been accomplished by insertion of arginine at the same or a nearby location. The number and position of positive charges plays a critical role in the proper and efficient binding of phosphate. However, a cluster of many positive charges inhibits phosphate binding. Moreover, the presence of negatively charged residues seems a requisite for the proper orientation and functioning of positively charged residues in the catalytic sites. This implies that electrostatic interactions between amino acids are an important constituent of initial phosphate binding in the catalytic sites. Significant loss of function in growth and ATPase activity assays in mutants generated through charge modulations has demonstrated that precise location and stereochemical interactions are of paramount importance.


Introduction
A typical 70 kg human generates approximately 2.0 million kg of ATP, the cell's energy currency, in a 75-year lifespan by converting food into useable energy by oxidation. ATP is generated by ATP synthase from ADP and inorganic phosphate (Pi) [1,2]. ATP synthase is not only the essential means of cellular energy production in animals but also in plants and almost all microorganisms. ATP synthase is the final enzyme in the oxidative phosphorylation pathway and is responsible for ATP synthesis by oxidative or photophosphorylation in the membranes of bacteria, mitochondria, and chloroplasts. It is the smallest known biological nanomotor. In order to synthesize ATP, a mechanical rotation mechanism is used where subunits rotate at approximately 100 times per second. Basic [3] functional aspects of ATP synthase remain the same in both prokaryotes and eukaryotes [4].
Membrane bound F 1 F o ATP synthase enzyme is structurally identical and highly conserved among different species. ATP hydrolysis and synthesis occur in the F 1 sector, whereas proton transport occurs through the membrane embedded F o [2,5]. ATP synthesis is the result of proton gradient-driven clockwise rotation of γ (as viewed from the outer membrane), while ATP hydrolysis occurs from anticlockwise rotation of γ-sub unit. Detailed reviews of ATP synthase structure and function may be found in [6][7][8][9][10][11][12][13][14][15][16].
A number of diseases such as Leigh syndrome, ataxia, Batten's diseases, Alzheimer's, angiogenesis, hypertension, cancer, heart disease, mitochondrial diseases, immune deficiency, cystic fibrosis, diabetes, ulcers, and tuberculosis that affect both human and animals have been associated with ATP synthase ( [1,17] and references therein). The presence of ATP synthase on the surfaces of multiple cell types, and its involvement in a number of cellular processes, makes this enzyme an attractive molecular target in the development of treatments for numerous diseases. [18][19][20][21]. One particular way in which ATP synthase can be used as a therapeutic target is to inhibit it and thereby deprive 2 Journal of Amino Acids abnormal cells of required energy leading to cell death [1,17,21,22].
The polyphenol piceatannol is one of the most portent inhibitors of ATP synthase [19,22]. The binding site for polyphenols is at the interface of α-, β-, and γ-subunits of the F 1 sector. X-ray structure shows that the following polyphenol binding pocket residues γGln274, γThr-277, βAla-264, βVal-265, γAla-270, γThr-273, γGlu-278, γGly-282, and αGlu-284, are highly conserved among different species and are within 4Å of the bound polyphenol compounds. Consequently, piceatannol and other inhibitory polyphenols can form both hydrophobic and nonpolar interactions with the above residues [22,36,37]. We hypothesize that molecular modulation of both polyphenol-binding pocket residues and polyphenol structures may synergistically affect ATP synthase activity and provide additional clues to catalytic site function.
The βDELSEED-loop of E. coli ATP synthase is known to be the binding site for several basic amphiphilic α-helical peptide inhibitors of ATP synthase. Examples are melittin, melittin-related peptide (MRP), bacterial/chloroplast ATP synthase ε-subunit, and SynA2 (the synthetic derivative of cytochrome oxidase). The α-helical basic peptide, melittin, is composed of 26 residues and is the primary component of honey bee venom (Apis mellifera). MRP is a 23-residue long peptide derived from frog skin (Rana tagoi). Both melittin and MRP are potent inhibitors of ATPase activity of E. coli ATP synthase [1,21,38,39].
Most ATP synthase inhibitory peptides studied so far are from anuran (frogs) sources. These antimicrobial peptides (AMPs) are cationic, between 10 and 50 residues in length, and frequently include a C-terminal amide group [1,[40][41][42]. Previous mode of action studies indicate that AMPs appear to interact with negatively charged phospholipids and then insert into the bacterial cell membrane or that they may also move across the cell membrane by passive transport and there disrupt a number of cellular processes [43].
Lately, it was observed that some of the antimicrobial effects of amphibian AMPs may be through their inhibitory effects on ATP synthase [1,21]. Melittin and other peptide inhibitors inhibit ATPase activity in a reversible and noncompetitive fashion [38,39,[44][45][46][47]. It is hypothesized that relatively short antibacterial or anticancer cationic peptides of approximately 10-30 amino acid residues with α-helical secondary structure may inhibit ATP synthase through their binding to the βDELSEED loop. For example, lysine-induced three positive charges of dermaseptin or four positive charges of magainin II interact with the five negative charges of βAsp-380, βGlu-381, βGlu-384, βGlu-385, or βAsp-386 and result in the inhibition of ATPase activity.
Of nearly 60 anuran-derived potential antimicrobial/ anticancer peptides, only 13 have been tested for their inhibitory effects on ATP synthase [1,21]. It was shown that MRP (melittin-related peptide) and MRP-amide strongly inhibited the ATPase activity of ATP synthase and that the presence of an amide group at the c-terminus of MRP caused a ∼16% increase in inhibition of ATP synthase ATPase activity. Whether or not negative charges in the βDELSEED motif play any role in the structural stability of the catalytic sites through electrostatic interactions with site residues remains to be seen.

Structural and Functional Aspects of Charged Residues in the Catalytic Sites of ATP Synthase
Recent studies have illuminated the role of charged residues in Pi binding at the catalytic sites. Binding of inorganic phosphate (Pi) is an important step in the ATP synthase mechanism which has been extensively studied by biochemical approaches and may be directly coupled to subunit rotation [2,11,25,[48][49][50][51][52][53]. ATP synthase is the terminal enzyme of oxidative phosphorylation and photophosphorylation that synthesizes ATP from ADP and Pi. The energy for ATP synthesis comes from the transmembrane movement of protons down an electrochemical gradient that is generated by substrate oxidation or by light capture. As protons move through the interface between the a and c subunits in the membrane-bound F o -sector of the enzyme, the free energy is transduced into mechanical rotation of a group of subunits (γεc 10−14 ) which comprise the "rotor". The helical coiled coil domain of the γ-subunit projects into the central region of the α 3 β 3 hexagon in the membrane extrinsic F 1 -sector. The α 3 β 3 hexagon contains three catalytic sites at α/β interfaces. The "Stator" subunits b 2 and δ function to prevent corotation of α 3 β 3 with the rotor [6,[54][55][56][57][58]. In this paper we present a detailed description of the catalytic site charged amino acids, their role in Pi binding, their effects on the spatial orientation, and effect of their modulation on one another. Figure 1 represents the simplest form of ∼530 kDa Escherichia coli ATP synthase containing eight different subunits, namely, α 3 β 3 γδεab 2 c 10−15 , divided into two sectors Two of these helices form a coiled coil that extend into the central space of the α 3 β 3 hexagon. In recent nomenclature, the rotor consists of γεc n , and the stator consists of α 3 β 3 δab 2 . Current understanding of the F 1 F o ATP synthase structure, function, catalytic mechanism, and its role in human health and disease has been thoroughly reviewed by Senior's group and others [1,2,7,8,17,20,59]. Based on the binding of ATP, ADP, and Pi, the three catalytic sites located on the F 1 sector of ATP synthase are designated βTP, βDP, and βE by X-ray crystallographers [60,61]. βE is the empty site into which Pi (inorganic phosphate) must initially bind for initiation of ATP synthesis. It has been proposed that the synthesis reaction in the three catalytic sites do not occur independently but in a consecutive manner [51]. In this "binding change mechanism", the three catalytic sites have different affinities for nucleotides at any given moment. Each catalytic site undergoes conformational transitions that lead to the following sequence: substrate binding (ADP and Pi) → ADP phosphorylation → ATP release. Experimental observations of rotation verified the predication made by Boyer [4,51,62] that catalysis requires the sequential participation of the three catalytic sites, with changing affinity for substrates and products, as it proceeds through the recurring mechanism, hence the term "binding change mechanism." Proton motive force is converted by F o to a mechanical rotation of the rotor shaft, which drives conformational changes of the catalytic domains of F 1 causing synthesis of ATP by phosphorylation of ADP. Conformational changes in the catalytic sites are connected to γ-subunit rotation. γ-Subunit rotation in isolated α 3 β 3 γ subcomplex has been observed directly by Yoshida and Kinosita with colleagues in Japan and subsequently by several other labs [12,[63][64][65][66][67][68]. The focus of this paper, the role of charged residues at the catalytic sites of E. coli ATP synthase, is a fundamental issue, because catalytic site charged residues are also relevant to many other ATPases, GTPases, and their potential application to nanotechnology and nanomedicine [1,11,18,69].

Catalytic and Motor Function of ATP Synthase
Determination of catalytic site Pi-binding residues has allowed a better understanding of the reaction mechanism of ATP synthesis and hydrolysis, and their relationship to the mechanical rotation of the γ-subunit. Characterization of catalytic site-charged residues can provide essential understanding in the following possible applications (1) development of effective modulator (inhibitory/stimulatory) molecules of ATP synthase catalytic function and (2) development of catalytic site mutants for biotechnological applications.
The analysis of charged catalytic sites residues involved in Pi binding has also helped answer the primary question of how the enzyme binds ADP and Pi rather than ATP at the catalytic sites? This is an often overlooked but crucial question in the mechanism of ATP synthesis. In active cells, the cytoplasmic concentrations of ATP and Pi are approximately in the 2-5 mM range, whereas that of ADP is at least 10-50-fold lower. Equilibrium-binding assays have established that both ADP and ATP bind to catalytic sites of purified F 1 and detergent solubilized F 1 F o with relatively similar binding affinities [71][72][73][74]. Obviously, a specific mechanism must have evolved for selectively binding ADP into catalytic sites while simultaneously preventing ATP binding during proton driven rotation and ATP synthesis. One hypothesis is that during ATP synthesis, the proton gradient-driven rotation of subunits impels an empty catalytic site to bind Pi tightly, thus stereochemically precluding ATP binding and, therefore, selectively favoring ADP binding [7]. A second fundamental question is how does subunit rotation affect Pi binding [49][50][51]? It was shown that Pi binding appears to be "energy linked", which entails a linkage to subunit rotation [56,75,76]. Therefore, for formulating a mechanism of ATP synthesis, it is of paramount importance to understand the features that determine Pi binding. Moreover, in the near future, it may be possible to use molecular features of Pi binding, derived from mutational and biochemical The βDP site in the AlF 4 − -inhibited enzyme structure is taken from [61]. E. coli residue numbering is used. Four positively and four negatively charged residue in close proximity to the bound phosphate analog AlF 4 − are identified. Rasmol software [70] was used to generate this figure using PDB file 1H8E [61].
studies, in the development of potent and novel molecular modulators of ATP synthase.

Characterization of Charged Residues at the Catalytic Sites
X-ray structural studies and mutagenic analyses of F 1 sector, the catalytic segment of ATP synthase, have so far identified four basic residues critical for catalysis, namely, αβLys-155, βArg-182, Arg-376, and βArg-246. Figure 2 shows the spatial orientation of these amino acids in close proximity to bound phosphate analog AlF 4 − . E. coli residue numbers are used throughout. Figure 2 also shows the spatial relationship between positive and negative charged residues. Initial studies employed the MgATP-and MgADPbinding parameters in mutant enzymes βK155Q, βR182K, βR182Q, βR246A, βR246Q, βR246K, αR376K, and αR376Q. These studies used fluorimetric analysis with introduced βTrp-331 as a specific catalytic site probe, while analysis of the transition state formation was done using MgADPfluoroaluminate and MgADP-fluoroscandium as transition state analogs [77][78][79][80][81]. Absent from these analyses was a direct measurement of Pi binding in the mutant enzymes. The above residues were clearly demonstrated to be involved in Pi binding with the subsequent application of Pi protection against NBD-Cl inhibition assays [11,48,[82][83][84][85].
The βLys-155 is part of the Walker A sequence in the catalytic sites of ATP synthase. X-ray structures of native F 1 with bound MgAMPPNP and MgADP [5], of MgADP-BeFx inhibited F 1 [87], of MgADP-AlF 4 -inhibited F 1 representing the transition state [61], and of MgADP-AlF 3 inhibited F 1 representing the late transition state/early ground state [88] all show the ε-amino group of βLys-155 very close (≤3Å) to the γ-phosphate position. The βK155Q mutant lacks ATP synthesis and has very low F 1 -ATPase activity (Table 1). Previous work had shown that βLys-155 plays a major role in binding MgATP, particularly at catalytic sites of high and medium nucleotide affinity, but not in binding MgADP [77]. βLys-155 is also critical for transition state formation [79,80]. The earlier hypothesis that βLys-155 was important for Pi binding in ATP synthesis [2] was experimentally confirmed by Pi protection against NBD-Cl inhibition where Pi binding in the βE catalytic site is abolished in βK155Q. Therefore, residue βLys-155 is involved at all stages of ATP synthesis from Pi binding, to the transition state, to MgATP formation [84]. βArg-182 is another important positively charged phosphate-binding residue in the catalytic sites of ATP synthase [84]. Mutants βR182Q and βR182K lack ATP synthesis activity and have low F 1 -ATPase activity (Table 1). Residue βArg-182 had been shown to be involved in MgATP binding at the site of highest affinity but not in MgADP binding. Transition state formation is abolished by βR182Q but retained in βR182K [78]. In this regard, it should be noted that βR182K F 1 does have somewhat higher ATPase activity (Table 1). βArg-182 was also hypothesized to be required for Pi binding in ATP synthesis [2], and this confirmed that both βR182Q and βR182K mutations abolished Pi binding in the βE site. Therefore, residue βArg-182 is also involved in all stages of ATP synthesis from Pi binding through ATP formation [84].
The αArg-376 residue of E. coli ATP synthase has been described as the "arginine finger" based on G-protein literature and was thought to be a required ligand for the catalytic transition state. Nonetheless, this residue was not shown to be involved in MgATP or MgADP binding despite its apparent proximity to the γ-phosphate of MgAMPPNP in X-ray structures [65,81]. Movement of this residue in and out of the catalytic site was inferred and was postulated to produce the rate acceleration ("positive catalytic cooperativity") linked to subunit rotation and full ("tri-site") catalytic site occupancy that is a hallmark of the mechanism [2]. Significant spatial displacements of residue αArg-376 have been noted in X-ray structures representing different reaction intermediates [5,33,61,75,87,88]. Consequently, it was hypothesized that conformational freedom of this residue likely contributes to its importance in catalysis [87]. The previously hypothesized importance of this residue in catalysis [2] was confirmed by Pi protection against NBD-Cl inhibition in which Pi failed to protect αR376Q F 1 from NBD-Cl inhibition. However, just as the αR376K mutant was able to form the transition state [81], it was also able to support Pi binding. It is nevertheless strongly impaired in both ATP synthesis and hydrolysis, which suggests that this residue has other required function(s) such as in conformational movements or in H-bonding to other side chains that are specific to Arg and not supported by Lys [11,84].
βArg-246 is the fourth positively charged residue within the Pi-binding subdomain of catalytic sites identified in the X-ray crystallographic structure ( Figure 2) that is involved in Pi binding. βArg-246 is equivalent to βArg-260 in mitochondrial F 1 and is conserved among all species. Early random mutagenesis experiments revealed that mutations βR246H and βR246C impaired oxidative phosphorylation drastically and reduced ATPase activity in purified F 1 to ∼1% of wild type [89,90]. Further work showed that these mutations caused the unisite catalysis parameter K d Pi to change by 4 orders of magnitude, whereas the K d ADP was largely unaltered by βR246C, and the ATP hydrolysis reaction equilibrium constant changed to favor ATP over ADP plus Pi [91]. Computer simulations have drawn attention to βArg-246, where movement of the residue during rotation, conformational change of the sites [92], and a role in binding Pi in the transition state were predicted [93,94]. Sitedirected mutagenesis of βR246 to Gln, Lys, and Ala was used to examine the effects of each mutation on function. A variety of inhibitors and ligands known to bind or react in the catalytic sites close to the Pi-binding subdomain were utilized in combination with the mutant enzymes to establish the role of the βArg-246 side chain. Substitutions of the Arg side chain to Gln (removes charge and preserves bulk), to Lys (preserves positive charge), and to Ala (removes side chain and charge) were all examined. All three substitutions severely impeded growth by oxidative phosphorylation and reduced ATPase activity of purified F 1 to ∼1% of wild type.
Finally, as shown in Figure 3 Pi protection against NBD-Cl inhibition clearly demonstrated that βArg-246 residue side chain is an important constituent in binding Pi and in forming the transition state [48].
Pi binding assays using Pi protection against NBD-Cl were devoid of any nucleotide and enzymes were prepared so as to have all three catalytic sites essentially empty. Therefore, the sites were in βE conformation. In this conformation αArg-376 and βArg-246 lie 2.6 and 4.0Å from βArg-182, whereas βLys-155 lies 9.5, 7.3, and 6.3Å from αArg-376, βArg-182, and βArg-246, respectively [88]. In essence, the X-ray structure [87] showed that bound MgADP-BeFx mimicked bound MgATP. In assays of F 1 -ATPase, it was shown that wild type and αR376Q were fully inhibited by MgADP-BeFx, whereas βK155Q and βR182Q were fullyresistant (Z. Ahmad, and A. E. Senior, unpublished work). These results supported the hypothesis that βLys-155 and βArg-182 are MgATP ligands, but that αArg-376 is not, and that the involvement of stringent stereochemical orientation factors plays a role in determining the functional interactions of αArg-376 [11,84].
The four positively charged residues form a tetrahedral structure with βLys-155 at the apex and αArg-376, βArg-182, and βArg-246 on the base [11,25]. A potential Pibinding pocket can readily be envisaged at the center of this tetrahedron (see Figure 2). In ATP synthesis, the βE site will change to the βADP + Pi ("half-closed") site in association with γ-rotation [2,61]. The X-ray structure of this conformation [61] shows that the residues αArg-376, βLys-155, and βArg-182 are each located ≤3.0Å from the nearest oxygen atom of bound SO 4 2− ) anion (modeling Pi), whereas βArg-246 is 4.5Å from the sulfate. Thus, as the reaction proceeds, the three residues αArg-376, βLys-155 and βArg-182 close around the Pi and move it away from βArg-246 toward the site of transition state formation [11,12,48,95].
Historically, many attempts to measure Pi binding in purified E. coli F 1 using [ 32 P] Pi [50] or by competition with ATP or AMP-PNP in fluorescence assays of nucleotide binding [72,96] failed to detect appreciable Pi binding at physiological Pi concentration. An assay devised by Perez et al. [97] in which the protection afforded by Pi against the inhibition of ATPase activity was induced by covalent reaction with 7-chloro-4-nitrobenzo-2-oxa-1, 3,-diazole (NBD-Cl) provided a measure of Pi binding. Orriss et al. [98] showed by X-ray crystallography that the covalent adduct formed by NBD-Cl is specifically in the βE catalytic site. Hence, protection afforded by Pi indicates that binding of Pi DVSAFVPTNV I S I TDGQ IFLETNLFNAG I RPAVNPG I SVSRVGGAAQTK IMKKL SGG I RTALAQYRE LAAF SQFASDLD  DVSAFVPTNV I S I TDGQ IFLE SNLFNAG I RPAVNPG I SVSRVGGAAQTK IMKKL SGG I RTALAQYRE LAAF SQFASDLD  DVSAY I PTNV I S I TDGQ IFLEAE LFYKG I RPA I NVGL SVSRVGSAAQVKAL KQVAGS LKL F LAQYREVAAFAQFGSDLD  DVSAYVPTNV I S I TDGQ IFLE S E LFYKGF RPAVN I GL SVSRVGSAAQLKSVKKVAGS I KL S LAQYRE L EDFAKFGSDLD  DVSAYVPTNV I S I TDGQ IFLE S E LFYKGF RPAVN I GL SVSRVGSAAQLKSVKKVAGS I KL S LAQYRE L EDFAKFGSDLD  DVSAY I PTNV I S I TDGQ IFLETE LFYKG I RPA I NVGL SVSRVGSAAQTRAMKQVAGTMKL E LAQYREVAAFAQFGSDLD  DVSAY I PTNV I S I TDGQ IFLETE LFYKG I RPA I NVGL SVSRVGSAAQTRAMKQVAGTMKL E LAQYREVAAFAQFGSDLD  DVSAY I PTNV I S I TDGQ IFLETE LFYKG I RPA I NVGL SVSRVGSAAQTRAMKQVAGTMKL E LAQYREVAAFAQFGSDLD  DVSAY I PTNV I S I TDGQ IFLETE LFYKG I RPA I NVGL SVSRVGSAAQTRAMKQVAGTMKL E LAQYREVAAFAQFGSDLD  DVSAY I PTNV I S I TDGQ IFLETE LFYKG I RPA I Figure 3: Sequence alignment of α and β-subunit residues. α and β-subunit amino acids from different species are aligned. Conserved positively charged residues are shown in blue color, and negatively charged residues are identified by red color. E. coli starting residue for α-subunit is αD336 and for β-subunit is βK155.
It may be noted that [ 32 P]Pi binding was detected with a Kd(Pi) in the range of 0.1 mM using an alternative, pressure ultrafiltration method, and this result is consistent with data obtained from the NBD-Cl protection assay [99]. It is apparent that Pi dissociates more rapidly from E. coli F 1 than it does from mitochondrial F 1 , undesirably, rendering the convenient centrifuge assay incompatible with the E. coli enzyme.
The story goes on with the presence of many charged/uncharged residues in close proximity to the Pi binding subdomain in the catalytic sites. These residues have been shown to exert either a direct or an indirect role in Pi binding. One of these residues is the charged αAsp-350 of the VISIT-DG sequence. αAsp-350 is part of the α-subunit VISIT-DG sequence, which is a highly conserved motif in this enzyme [25]. VISIT-DG sequence residues are of special interest in general and negatively charged αAsp-350 in particular, because of the close proximity to the known positively charged phosphate-binding residues. αAsp-350 is ∼3Å from αArg-376. It would be imperative to understand three specific aspects of αAsp-350 residue. First, is residue Asp-350 directly or indirectly involved in phosphate binding through αArg-376? Second, is αAsp-350 important for function through its role in maintaining the structural integrity of the Pi binding subdomain but not involved in Pi binding per se? Third, is the carboxyl side chain of αAsp-350 involved in the transition state at the catalytic site? Our hypothesis is that αAsp-350 interacts electrostatically with αR376. Such an interaction may provide proper orientation of αArg-376 side chain towards Pi.

Modulation of Charge in the Catalytic Sites
Understanding the role of charged residues and the effects of modifying them is important in understanding the molecular mechanism of ATP synthesis. NBD-Cl inactivation assay described earlier have shown that positively charged residues are functionally essential for Pi binding in the βE catalytic site of E. coli ATP synthase [11,48,83,84]. The introduction Journal of Amino Acids of charged residues in place of uncharged residues in the vicinity of catalytically important residues has been shown to affect Pi binding by resulting in a loss or gain of ATPase activity [82,83,86]. Earlier work [82,83] indicated that the introduction of negative charge in the Pi-binding pocket in the form of βN243D close to βArg-246 prevented Pi binding ( Figure 5). Also, introduction of positive charge in the form of βN243R restored Pi binding in βR246A mutants. Similarly, the introduction of negative or positive charge in the form of αF291D/E/R with βR246 or βR246A resulted in a loss or gain of Pi binding (Figures 4 and 5) [83,86]. These results suggested that modulation of charge in the Pi binding site could be used to understand the molecular mechanism of Pi binding. It is established that Arg residues occur particularly commonly in the Pi binding sites of proteins [100]. Therefore, varying the number of Arg residues in the Pi binding site of ATP synthase can be an instructive approach.
Residue βAsn-243 lies 3.2Å from βArg-246 in both AlF 3 and SO 4 2− )-containing catalytic sites (nearest atom distances quoted) [83]. One experimental approach used was to introduce the mutation βN243R in a wild-type background (with βArg-246) and in presence of the βR246A mutation. Residue αPhe-291, located at the end of the Pi-binding pocket across the catalytic α/β interface, with its side-chain pointing toward the bound Pi analogs, is also a suitable location for introducing a new Arg. This residue lies at a distance of 3.2Å from βArg-246 in the AlF 3 -containing catalytic site and 7.5Å in the SO 4 2− -containing catalytic site [61,83,88]. Arginine was introduced in the form of an αF291R mutation in the wild-type background and in the presence of the βR246A mutation. The actual distances of residues βArg-246, βAsn-243 and αPhe-291 were obtained from bound AlF 3 and SO 4 2− as determined by X-ray crystallography [61,88], while speculative distances (in brackets) were calculated for mutant residues βAla-246, βArg-243 and αArg-291 using the "Deep View Swiss-Pdb Viewer" [101]. Apparently, mutations placed extra positive charge relatively close to Pi, and the βAla-246 mutation left a relatively large space into which a new Arg fits nicely.

Synergistic Stereochemical Interactions at the Catalytic Sites
The introduction of one or two extra positively charged Arg residues in the wild-type background at either β-243 or α-291, or both, has proven to inhibit Pi binding ( Figure 4). Introduction of a new Arg at β-243 or α-291 in the βR246A background provided a significant compensatory effect on ATPase. ATP-driven proton pumping was also reinstated in the case of the αF291R/βR246A mutant. But these new arginines did not restore function to full normal [83]. The βR246A mutant did not show Pi binding, but both βN243R and αF291R mutations "rescued" Pi binding in combination with βAla-246 ( Figure 4). Since neither βArg-243 nor αPhe-291 could be expected to assume the exact same stereochemical interactions that βArg-246 achieves, electrostatic interaction appears to be a significant factor. Presence of at least one positive charge at this general location is a requisite determinant of initial Pi binding in the catalytic site βE. βN243R or αF291R in the wild-type background (representing one extra positive charge) did not prevent Pi binding, but the combination of αF291R/βN243R (two extra charges) abrogated Pi binding (Figure 4). Presumably the local concentration of charge in the latter becomes too disruptive and distorts the Pi-binding site [83].
A similar pattern of effects has been reported when transition state stabilization was assessed by assaying inhibition of ATPase activity by the transition state analogs MgADPfluoroaluminate and MgADP-fluoroscandium. Previously, it was shown that [48] that both inhibitors are potent against wild-type ATP synthase but that each inhibit βR246A mutant only to small extent, which indicates that βArg-246 is intimately involved in transition state stabilization. It was found that either mutant residue βArg-243 or αArg-291 partly "rescued" transition state stabilization when present with βAla-246 [83]. Raising the number of positively charged residues to two (βN243R and αF291R mutants in wild-type background) had an adverse effect as reflected by a lesser inhibition of ATPase activity. Raising the number of local positive charges to three reduced transition state stabilization right back to where it was in βR246A. Interestingly, even in the best cases among the mutants (βN243R/βR246A or αF291R/βR246A) transition state stabilization was incomplete as compared to wild-type, which suggests the importance of stereochemical interactions [83].
In summary, all the results showed that Pi binding is notably affected by the local positive charges in catalytic site βE of ATP synthase. Positive charge in the vicinity of the natural βArg-246 is important because its removal in βR246A mutant can be compensated partially by introduction of one Arg at either β-243 or α-291. Thus, electrostatic interaction is an important determinant of Pi binding. The presence of two arginines by introduction of either βArg-243 or αArg-291 in the presence of βArg-246 does not prevent Pi binding, but the presence of all three arginines eliminates Pi binding. Effects on transition state stabilization followed a parallel pattern, but the restoration of Pi binding in βE catalytic sites by charge compensation was not sufficient by itself to restore full function [83].