F-actin-like ATPase Activity in a Polymerization-defective Mutant Yeast Actin (V266G/L267G)*

Xiaoyi Yao and Peter A. RubensteinDagger

From the Department of Biochemistry, University of Iowa College of Medicine, Iowa City, Iowa 52242

Received for publication, December 29, 2000, and in revised form, April 2, 2001


    ABSTRACT
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Polymerization increases a low level G-actin ATPase activity yielding ADP-Pi F-actin and then ADP F-actin following release of Pi. By monitoring Pi release, we explored the relationship between the ATPase activity and polymerization characteristics of a mutant yeast actin, GG. In this mutant, two hydrophobic residues at the tip of a proposed hydrophobic plug between actin subdomains 3 and 4, Val266 and Leu267, were mutated to Gly. Although GG-actin does not polymerize by itself in vitro, GG cells are viable. We show that GG-actin ATPase activity increases under normal polymerization conditions, although stable filaments do not form. A plot of Pi release rate versus actin concentration yields an apparent critical concentration, like that seen for actin polymerization, of ~8 µM for Mg2+ GG-actin and 11 µM for Ca2+ GG-actin. In contrast to WT-actin, Pi release from GG-actin is cold-sensitive, reflecting the temperature sensitivity associated with mutations that decrease hydrophobicity in this region. Thus, under polymerization conditions, GG-actin exhibits a continuous F-actin-like ATPase activity resulting from the temperature-sensitive formation of unstable cycling F-actin oligomers. Tropomyosin limits the extent and rate of this activity and restores polymerization by capturing and stabilizing these oligomers rather than enhancing filament nucleation.


    INTRODUCTION
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

G-actin, in the presence of Mg2+, slowly catalyzes the hydrolysis of ATP that is bound at a high affinity site at the base of a deep cleft separating the two major domains of the protein. This activity is greatly enhanced by polymerization of the actin (1). For those actins studied to date, hydrolysis occurs shortly after the incorporation of the actin monomer into the filament producing an ADP-Pi species, which slowly loses its Pi to yield an ADP-monomer. Because ATP and ADP-Pi F-actin are both more stable than ADP-F-actin, this Pi release is believed to play a major role in the treadmilling of actin filaments that occurs within the cell.

Actin polymerization is a multiple-step process that includes a salt-induced G to F conformational change, rate-determining nucleation, and filament elongation until the monomer actin concentration reaches a limiting value called the critical concentration. Prior to incorporation of the actin monomer into the filament, it has been hypothesized that the actin proceeds through an F-monomer state (2). Evidence for such a species derives from experiments such as comparing protease digestion patterns of the actin in the absence and presence of polymerization-inducing salts at actin concentrations below the critical concentration of actin needed for formation of filaments. Using muscle actin, Shu et al. (3) determined that the F-monomer exhibits a low ATPase activity similar to that observed with G-monomer, suggesting that the enhanced ATPase activity associated with actin polymerization requires the conformation and inter-monomer contacts formed within the context of the actin filament.

We have previously created a mutant actin (GG-actin) in which we simultaneously converted Val266 and Leu267 to glycines (4, 5). These residues along with Leu269 reside in the tip of a loop between actin subdomains 3 and 4. Holmes and co-workers (6) proposed that one major interstrand force stabilizing the actin filament was a "plug-pocket" interaction in which the tip of this loop interacts with a hydrophobic surface formed by the interface of two monomers on the opposing strand. In agreement with the predictions of this model, we have demonstrated that, as assessed by a change in light scattering, purified GG-actin alone fails to polymerize under normal polymerization conditions. The actin binding proteins tropomyosin (7) and fimbrin (8) can rescue GG-actin polymerization. However, this rescue is temperature-sensitive. In the presence of tropomyosin or fimbrin, polymerization of GG-actin occurs only at a temperature higher than 15 °C. Furthermore, when the temperature is lowered after polymerization reaches the steady state, depolymerization of actin filaments occurs.

The polymerization defect exhibited by GG-actin and the cold-sensitive rescue of GG-actin polymerization are consistent with the Holmes model. If the model is correct, removal of two hydrophobic residues at the tip of the plug should greatly decrease the proposed hydrophobic cross-strand interaction, leading to polymer instability of the mutant actin. Tropomyosin or fimbrin binding may strengthen intermonomer contacts along one strand partially compensating for the loss of cross-strand stabilization to the point that polymerization at 25 °C is restored. However, hydrophobic interactions are destabilized by colder temperatures (9). Thus, at low temperatures, the residual cross-strand interaction of the mutant actin is reduced to such an extent that the extra stabilization can no longer compensate, and filament formation cannot occur.

Although GG-actin has been used as a model system for examining the filament-stabilizing abilities of actin-binding proteins (7, 8), the specific mechanism responsible for the polymerization defect associated with GG-actin is unclear. For example, it is not known whether GG-actin remains in its G form under normal polymerization conditions, is converted to an F-actin monomer, or actually forms transient unstable F-actin oligomers. To understand the mechanisms by which this rescue of GG-actin polymerization occurs, it is necessary to first understand the nature of the polymerization defect. To explore these alternatives, we have assessed in this paper the effect of F buffer1 on the ATPase activity exhibited by GG-actin and the dependence of this activity on actin concentration and temperature. We have also determined the effect of temperature on the ATPase activity of WT yeast actin under polymerizing conditions.

    MATERIALS AND METHODS
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Actin Purification and Polymerization-- Purification of wild-type and GG-actins from Saccharomyces cerevisiae was done by a combination of DNase I affinity chromatography and DEAE-cellulose chromatography as previously described (10). Affinity columns were made with DNase I purchased from Worthington and Affi-Gel 10 obtained from Bio-Rad Laboratories. Purified Ca2+/G-actin was stored at 4 °C in Ca2+/G buffer (10 mM Tris-HCl, pH 7.5, 0.2 mM CaCl2, 0.2 mM ATP, and 0.5 mM DTT) and used within 4 days.

Actin polymerization was induced by the addition of 2 mM MgCl2 and 50 mM KCl to a G-actin solution in G buffer (F buffer). Reactions of a total volume of 120 µl were followed in the thermostatted cuvette chamber of a fluorescence spectrometer. The increase in light-scattering caused by polymerization was monitored with the excitation and emission wavelengths set at 360 nm. For studies with the Mg2+ form of actin, purified Ca2+-actin was converted into the Mg2+ form by treatment with 0.2 mM EGTA in the presence of 0.1 mM MgCl2 at 4 °C for 10 min using a modification of a previously published procedure (11). Mg2+-G-actin was used immediately after the conversion from Ca2+/G-actin.

Enzchek Phosphate Assay-- Release of inorganic phosphate from actin was quantitated by the Enzchek phosphate assay. This assay employs a kit obtained from Molecular Probes and is based on the Pi-dependent liberation of 2-amino-6-mercapto-7-methylpurine from methyl-thioguanine, a nucleoside derivative of this base, by a purine nucleoside phosphorylase. The product base has a characteristic UV spectrum, not evident when part of a nucleoside, which can be utilized to monitor its phosphate-dependent rate of release by the enzyme. Each reaction mixture contained actin at the desired concentration as specified by the manufacturer, 2 units/ml purine nucleoside phosphorylase, and 200 µM methyl-thioguanine riboside. Pi release from actin in F buffer (10 mM Tris-HCl, pH 7.5, 0.2 mM ATP, 0.5 mM DTT, 2 mM MgCl2, and 50 mM KCl) or in Mg2+-G buffer (10 mM Tris-HCl, pH 7.5, 0.2 mM ATP, 0.5 mM DTT, and 0.1 mM MgCl2) was monitored continuously by the increase in absorbance at 360 nm. Phosphate standard curves were generated for each assay.

Tropomyosin Purification-- Bovine cardiac tropomyosin was purified from cardiac acetone powder according to the procedure of Butters et al. (12).

PDM Cross-linking-- G-actin in G buffer was centrifuged through a micro Bio-Spin chromatography column (Bio-Rad) pre-equilibrated with DTT-free G buffer to remove remaining DTT, and the eluted G-actin was diluted to 20 µM with DTT-free G buffer. 20 µl of 20 µM actin was then incubated at 25 °C for 10 min with or without the addition of 2 mM MgCl2 and 50 mM KCl. A stock solution of 5 mM N,N'-1,4-phenylenedimaleimide (PDM) in dimethylformamide was freshly diluted 10 times with DTT-free G buffer, and 1 µl of PDM was added into the 20-µl actin solution followed by an additional 8-min incubation. The final ratio of PDM to actin was about 1:1. The cross-linking was quenched by the addition of 20 µl of 2× SDS sample buffer containing 20% beta -mercaptoethanol. The presence of cross-linked actin oligomers was analyzed by 10% SDS-PAGE.

    RESULTS
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Pi Release by GG-actin in F Buffer Is Significantly Faster Than in G Buffer-- We first determined whether increasing the ionic strength to that normally used to induce actin polymerization enhances the ATPase activity of GG-actin by comparing Pi release from GG-actin under polymerization (F buffer) and monomeric (G buffer) conditions. Fig. 1 shows the time-dependent release of Pi from GG-actin with or without the addition of 2 mM MgCl2 and 50 mM KCl. Monomeric GG-actin exhibited a Pi release curve similar to that of WT actin. Addition of 2 mM MgCl2 and 50 mM KCl, which induces polymerization of WT-actin, did not do so with GG-actin as judged by a lack of change in light scattering and the absence of filaments in samples examined by electron microscopy (5). Interestingly, however, the rate of Pi release from GG-actin in F buffer increased 4-fold compared with that in G buffer.


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Fig. 1.   Phosphate release from GG-actin in G buffer and F buffer. Mg2+-GG-actin (10 µM) in G buffer (open circle ) or F buffer (), and 10 µM Mg2+ WT-actin in G buffer (asterisks) were incubated at 25 °C. The rate of Pi release was quantitated by the Enzchek phosphate assay. This is a representative example of an experiment that was repeated with three different actin preparations.

Pi Release by GG-actin Is Greatly Increased Above a Certain Actin Concentration-- To explore the mechanism behind this enhanced GG-actin ATPase activity in the presence of F buffer, we first measured the continuous release of Pi from WT-actin to which F salts had been added. Our results demonstrate (see Fig. 6) that Pi release from WT-actin closely mirrors its polymerization curve reaching a plateau when F-actin formation reaches equilibrium. We next measured Pi release by Mg2+-GG-actin at different concentrations under polymerization conditions (Fig. 2A). At low concentrations, a continuous slow monophasic Pi release occurred. However, at higher actin concentrations, Pi release by GG-actin appeared to be biphasic: a lag phase and a linear fast release phase with no plateau. We observed the same behavior with Ca2+/GG-actin, showing that this behavior, at least qualitatively, was independent of the nature of the tightly bound divalent cation (Fig. 2B).


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Fig. 2.   Effect of actin concentration on GG-actin ATPase activity. To different concentrations of GG-actin in G buffer were added 2 mM MgCl2 and 50 mM KCl, and Pi release was monitored continuously by the Enzchek phosphate assay. A, Mg2+-GG-actin; B, Ca2+-GG-actin. , 16 µM GG-actin; -, 14 µM GG-actin; ×, 12 µM GG-actin; open circle , 10 µM GG-actin; *, 8 µM GG-actin; +, 4 µM GG-actin. This experiment was repeated with two different preparations of actin with essentially similar results.

This type of concentration-dependent Pi release by GG-actin resembles a critical concentration curve determination for actin polymerization, suggesting that GG-actin might form unstable oligomers leading to abortive polymerization. For both cations, we thus plotted the rate of Pi release by determining the slopes of the linear second phase of each curve as a function of actin concentration (Fig. 3). This plot exhibited two linear phases as a function of actin concentration, and the intersection of the two lines yielded an apparent critical concentration for enhancement of ATPase activity of ~8 µM for Mg2+-GG-actin. A duplicate experiment with a second actin preparation yielded an apparent critical characterization of 7 µM (data not shown). Both determinations using Ca2+-actin yielded a critical concentration value of 11 µM. This distinction in apparent critical concentration for enhancement of Pi release is consistent with the divalent cation-dependent difference in critical concentration for polymerization determined earlier for muscle actin (13), although the difference is smaller than that reported in this previous study. Our results therefore indicate that the enhanced ATPase activity we observed for GG-actin in F buffer results not merely from conversion of a G- to an F-monomer but derives from the formation of unstable oligomers of F-actin.


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Fig. 3.   Relationship of the rate of Pi release to GG-actin concentration. The slope of the linear portion of each curve from Fig. 2 was determined and plotted as a function of actin concentration. A, Mg2+-GG-actin; B, Ca2+-GG-actin.

It has previously been shown (14) that, for a polymerization process like that of actin, a plot of ln (lag phase) versus ln (actin) will produce a line with a slope equal to one-half of the number of monomers in the nucleus. Using the data in Fig. 2 for Mg2+-actin, we calculated the lag phase by determining the point at which the second linear part of the curve intersected the first section of the plot for the 10, 12, and 16 µM curves. The plot of ln (lag phase) versus ln (actin) shown in Fig. 4 is a straight line with a slope of 2.1. This experiment was repeated with a second preparation of actin, and a slope of 1.85 was obtained (data not shown). This result, consistent with the data of Tobacman and Korn for muscle actin (14), indicates that the increase in ATPase activity following addition of salt depends on formation of a nucleus with three or four monomers, further demonstrating that it results from abortive F-actin formation.


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Fig. 4.   Estimation of nucleus size for Mg2+-GG-actin oligomerization. The lag times for the fast release phase of 10, 12, and 16 µM Mg2+-GG-actin were determined by the intersection of the two phases. The ln (lag time) was plotted versus ln [actin], yielding a straight line with a slope of 2.1 and a correlation coefficient of 0.99. A repetition of this experiment with a second preparation of actin yielded a slope of 1.85 with a correlation coefficient of 1.

Pi Release by GG-actin under Polymerization Conditions Is Cold-sensitive-- Our previous work demonstrated that the ability of beryllium fluoride, BeFx (5), tropomyosin (7), or Sac6p (8) to rescue GG-actin polymerizability was cold-sensitive. We therefore determined whether or not the F-actin-like ATPase activity associated with GG-actin displayed a similar temperature sensitivity. Control experiments to determine the temperature sensitivity of the Enzchek assay system showed a peak activity at 20 °C, which decreased to between 85% and 90% of this activity as the temperature was decreased to 4 °C or increased to 25 °C. As an indication of ATPase activity, we assessed the release of Pi from 12 µM Mg2+-GG-actin at temperatures ranging from 15 °C to 25 °C following the addition of 2 mM MgCl2 and 50 mM KCl. Results were then adjusted to reflect the small temperature-dependent differences in the efficiency of the Enzchek system. As shown in Fig. 5A, at 15 °C, minimal Pi release was observed. Increasing the temperature above this point resulted in a corresponding increase in the rate of Pi release. The biphasic nature of these plots is similar to what is observed when one studies the polymerization of actin at different temperatures and suggests that the lag phase is due to nucleation whereas the faster second phase is associated with the unstable addition of monomers to the nuclei. To further analyze the dependence of Pi release on temperature, we plotted the slopes of both the first and second phases of the plots shown versus temperature in Fig. 5, B and C. Fig. 5D shows that both sets of data points produce the same line when the points in each curve are normalized to the slope at 25 °C for each curve. In each case, the intercept on the temperature axis is about 15 °C. When the experiment was reproduced with another preparation of actin, the onset of polymerization was 15.5 °C. Actin polymerization follows nucleation/elongation kinetics, and if nucleation is rate-limiting, the number of nuclei will dictate the rate of oligomerization. Our data therefore suggest that a threshold for nucleation for 12 µM Mg2+-GG-actin is 15 °C and that, over the temperature range tested, the increase observed in Pi release results primarily from an increase in the number of nuclei present as a function of temperature.


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Fig. 5.   Effect of temperature on the salt-induced ATPase activity of Mg2+-GG-actin. A, Pi release from 12 µM Mg2+-GG-actin at various temperatures was monitored by the Enzcheck assay following the addition of 2 mM MgCl2 and 50 mM KCl. , 25 °C; open circle , 20 °C; ×, 17.5 °C; +, 15 °C. B, the slope for the fast release phase at each temperature was replotted as a function of temperature. C, the slope for the slow release phase at each temperature was replotted as a function of temperature. D, the release rate at each temperature relative to that at 25 °C for each phase was plotted. , slow phase; open circle , fast phase. This experiment was repeated with two different actin preparations with same results.

Temperature Dependence of Pi Release by Polymerizing WT Actin-- It is possible that the temperature sensitivity of Pi release by GG-actin reflects an inherent sensitivity of the ATPase reaction per se rather than temperature-sensitive actin oligomerization. We thus assessed both the extent of polymerization and the Pi release of WT yeast actin as a function of temperature following induction of polymerization by the addition of salts. Fig. 6 shows that decreasing the temperature results in a concomitant decrease in both the rate of polymerization and Pi release. ATPase activity is present at all temperatures, and the extent of Pi release from WT actin is governed solely by the extent of actin polymerization. These results suggest that the decrease in ATPase activity observed reflects a decrease in the rate of polymerization and not an inherent temperature-sensitive decrease in the ATPase activity per se. At 15 °C, where Pi release from GG-actin had disappeared, WT actin exhibited significant Pi release with its rate dependent solely on the rate of polymerization of the actin. Therefore, the lack of Pi release, and thus ATPase activity, seen with GG-actin at 15 °C most likely results from the inability of this actin to nucleate and form transient F-actin oligomers.


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Fig. 6.   Effect of temperature on polymerization of and Pi release from WT yeast actin. A, polymerization of 4.5 µM Mg2+ WT-actin induced by the addition of 2 mM MgCl2 and 50 mM KCl at different temperatures is shown using light scattering as an assay. B, Pi release under the same conditions, as monitored by the Enzcheck assay, is shown. , 25 °C; ×, 20 °C; *, 15 °C; open circle , 10 °C; +, 7 °C. C, the data from light scattering and Pi release at 25 °C were normalized and plotted together. , light scattering; open circle , Pi release. This experiment has been repeated three times with different preparations of actin with essentially the same results.

Although it has been demonstrated that muscle actin slowly releases its bound Pi after ATP hydrolysis (15), it is not known whether or not yeast actin has the same behavior. To address this question, we normalized the data from light scattering and Pi release at 25 °C and plotted them together (Fig. 6C). The concentration of yeast actin we used, 4.5 µM, polymerized as rapidly as 10 µM muscle actin (data not shown) under the same conditions, in agreement with the results of Buzan and Frieden (16) that yeast actin polymerizes substantially faster than muscle actin. Although we observed a significant lag phase in the rate of Pi release following polymerization for muscle actin, no apparent lag phase was seen in the case of the yeast actin.

Tropomyosin Limits the Extent of Pi Release by GG-actin-- We have previously shown that tropomyosin (7) restores the polymerizability of GG-actin. If the continuous ATPase activity observed with GG-actin alone in F salts is due to the continuous turnover of oligomers, this activity should be greatly curtailed in the presence of tropomyosin after polymerization reaches a steady state. We therefore determined the rate of Pi release when polymerization-inducing salts were added to mixtures of actin in the presence of tropomyosin. Fig. 7 demonstrates that, as predicted, the linear increase in Pi is greatly inhibited when polymerization approaches the steady state.


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Fig. 7.   Tropomyosin limits the extent of ATP hydrolysis by GG-actin in F buffer. A, Mg2+-GG-actin, 20 µM, was mixed with 6 µM cardiac tropomyosin, and 2 mM MgCl2 and 50 mM KCl was added to the mixture. This amount of tropomyosin is sufficient to saturate the tropomyosin binding sites on the F-actin. Polymerization under such conditions was monitored by the increase in light scattering. B, Pi release under the same conditions as in A or by GG-actin in the absence of tropomyosin was monitored by the Enzcheck assay. , GG-actin with tropomyosin; open circle , GG-actin by itself. This experiment was performed twice with different preparations of actin with essentially the same result.

Pi Release by GG-actin under F-monomeric Conditions-- Although Shu et al. (3) reported that the F-monomer did not exhibit enhanced ATPase activity over the G-monomer, their study was performed for very short times following addition of salt to actin solutions above the critical concentration, which might have led to inaccuracies in their measurements. Second, in a number of instances dealing with polymerization rates and nucleotide exchange, yeast and muscle actins have been shown to behave quantitatively quite differently (4, 16). Fig. 3 shows that oligomerization of GG-actin only occurs when its concentration is above the critical concentration. This suggests that we could possibly gain a population representing F-monomeric actin when we induce the conformational switch by F salts with GG-actin at concentrations below the critical concentration. Thus, we determined whether, below the critical concentration, GG-actin in F buffer would display an enhanced ATPase activity over that seen in G buffer. We incubated 5 µM Mg2+-GG-actin at 25 °C with or without the addition of salts and determined the rate of Pi release by the Enzchek phosphate assay. No difference could be seen between these two salt conditions in agreement with the results of Shu et al.

Probing GG-actin Oligomer Formation by Cross-linking-- N,N'-1,4-Phenylenedimaleimide (PDM) has been used to probe the oligomeric state of actin polymerization. Millonig and Aebi (17) have demonstrated the time-dependent appearance of two cross-linked species during polymerization, a lower dimer (LD) with an apparent molecular mass of 86 kDa and an upper dimer (UD) with an apparent molecular mass of 115 kDa by SDS-PAGE. The LD, a Cys374-Cys374 cross-linked species (18), appears immediately after salt induction and is not compatible with the structure of the actin filament. The UD forms between Lys191 on one subunit and Cys374 on another subunit along the helical filament and reflects the structure of a dimer in the actin filament. The LD is consumed during polymerization probably via two pathways (19). In one path, the LD is in equilibrium with a G-actin pool and indirectly involved in polymerization. In a second pathway, during polymerization LD directly incorporates into actin filaments to form LD-decorated F-actin. The unincorporated actin subunits are then released during filament maturation probably due to an F-conformational change resulting in smooth-looking filaments.

We monitored GG-actin oligomerization by PDM cross-linking. 20 µM Ca2+-GG-actin in G or F buffer was incubated at 25 °C for 10 min during which phosphate release is linear, and cross-linking by PDM was initiated as described under "Materials and Methods." WT actin from rabbit skeletal muscle was treated in the same way as a control. Fig. 8 shows that muscle actin yielded all upper dimer, consistent with what was previously reported and what we observed with yeast WT actin (20). In contrast, a significant amount of LD was observed with GG-actin along with a fainter UD band demonstrating that GG-actin could form F-actin like assemblies. The Mg2+ form of GG-actin gave essentially the same result (data not shown).


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Fig. 8.   PDM cross-linking demonstrates GG-actin oligomerization. 20 µM Ca2+ actin in DDT-free G or F buffer was incubated for 10 min at 25 °C. PDM was added at a 1:1 ratio to actin and incubated at 25 °C for 8 more min. The cross-linking reaction was stopped by SDS sample buffer containing 20% beta -mercaptoethanol, the products were analyzed by 10% SDS-PAGE, and the bands were visualized by staining with Coomassie Blue. UD, upper dimer with apparent molecular mass of 115 kDa; LD, lower dimer with apparent molecular mass of 86 kDa. The identity of these species was based on the migration of a series of molecular weight markers not shown. This experiment was repeated with two preparations.


    DISCUSSION
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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We previously demonstrated that, in agreement with Holmes' model of the actin filament, eliminating hydrophobicity in a subdomain 3/4 loop in yeast actin (GG) resulted in a nonpolymerizing protein (5). However, we showed that polymerizability could be restored by incubation with phalloidin (5), Sac6p (8), or tropomyosin (7). Whether the polymerization defect lay in the nucleation or elongation phase could not be determined. The demonstration that BeFx, a phosphate analogue, also restored polymerization (5) suggested that the protein could still hydrolyze ATP. However, BeFx-dependent rescue of polymerization could have resulted from stabilization of labile oligomers following nucleation or by generation of ADP-BeFx actin, which then polymerized due to an altered conformation.

We have addressed these questions by employing a continuous phosphate release assay to assess nucleotide hydrolysis by GG-actin. This assay provides a combined estimate of the hydrolysis of ATP and the subsequent release of the Pi from the actin, although it does not allow us to examine the ATP hydrolysis step per se. However, the virtual coincidence of the polymerization and Pi-release curves for yeast actin makes it very unlikely that Pi release is rate-limiting in comparison to ATP hydrolysis, thereby validating this approach.

Although GG-actin will not form stable filaments, our results demonstrate a substantial F buffer-dependent increase in GG-actin ATPase activity for both the Ca2+ and Mg2+ forms of the actin. In contrast with the case of WT actin, however, the ATPase activity of GG-actin is continuous. Theoretically, the continuous nature of this activity could result from an F-monomer ATPase, because previous work had presented evidence for the generation of such a species in solution (2). Alternatively, continuous activity could result from the formation and cycling of small oligomers, undetectable by light scattering. Our results demonstrate that the second alternative is the correct one. In the case of WT actin polymerization, continuous low level linear ATPase activity due to treadmilling occurs at the steady state. In response to the introduction of F salts into solution, GG-actin exhibits a biphasic ATPase activity, an initial low linear ATPase activity followed by a faster but still linear phase. The low ATPase activity is very likely due to a process involving nucleation. The second faster phase could not result from a typical net elongation phenomenon, because this would require the attainment of a steady-state level of filament formation that does not occur. Instead, the continuous activity probably reflects a steady state of exchange of monomers from unstable oligomers driven by the hydrolysis of ATP. In essence, the system is one in which, once an apparent critical concentration for GG-actin is reached, nuclei or short oligomers provide a surface catalyst for the hydrolysis of ATP by cycling monomers. Because this is a steady-state situation governed by the critical concentration of the system, as the actin concentration increases, the filament ends, but not the free monomers, increase concomitantly leading to the actin-dependent linear increase in ATPase activity we observe.

The apparent critical concentration of GG-actin, about 11 µM for Ca2+ actin and 7 or 8 µM for Mg2+ actin is ~50-60 times higher than it is for WT actin. Wen (7) had previously determined a critical concentration of 5.5 µM for the tropomyosin-dependent rescue of Mg2+-GG-actin polymerization by light scattering. The small difference (0.086 mg/ml) between the critical concentration of intrinsic oligomerization and tropomyosin-dependent polymerization may be due to different preparations of actin or small variations in carrying out the experiments. It is also possible that tropomyosin slightly decreases the critical concentration of GG-actin polymerization. However, the measurement of an intrinsic critical concentration for GG-actin oligomerization allows for the first time an estimate of the importance for filament stabilization of the hydrophobicity normally associated with Val266 and Leu267, which was eliminated in this mutant. Furthermore, this system provides us with a way of actually assessing nucleation and oligomerization of actin under conditions that do not permit formation of stable filaments.

Demonstration of an oligomerization-dependent ATPase coupled with our previous finding that BeFx allows formation of stable GG-actin filaments allows one to understand the underlying basis for the inability of GG-actin to form stable filaments alone. There is clearly an effect on the critical concentration of the ATP-actin. In other words, in terms of the Holmes model, in the ATP monomer, the residual hydrophobicity of the plug is oriented correctly enough to provide sufficient cross-strand stabilization for initiation of actin filament formation. However, ATP hydrolysis and subsequent release of the phosphate alters the conformation of either the plug or other monomer contacts enough so that this residual plug hydrophobicity is no longer sufficient for maintenance of the filament structure. In other words, the critical concentration of the ADP-actin monomer is so high that, under the conditions of the experiment, filaments cannot form.

Oligomerization of GG-actin was directly demonstrated by PDM cross-linking. Under conditions where steady ATPase activity is observed, GG-actin forms a significant amount of LD along with much less UD. Because the UD is the precursor for nucleus and filament formation, presumably it is the conformation responsible for the F-like ATPase activity. Taking into account the differences between the critical concentrations of WT- and GG-actin, there can be no more than half as much GG F-actin species as WT species at any point. The fact that the ratio for UD between these two actins is much greater than 2:1 can be attributed to the continuous cycling of the GG F species and a resulting reduction in the frequency with which they can react with the cross-linker and perhaps to an inherently less reactive conformation assumed by the GG-actin per se. This result substantiates our previous hypothesis that tropomyosin-dependent rescue of GG-actin polymerization depends initially on the capture of pre-formed actin oligomers and not on tropomyosin-dependent nucleation of filament formation.

Our temperature studies not only provide additional information concerning the effect of the GG mutation on actin function, but they also provide new insight into the ATPase of WT actin as well. The extent of polymerization of WT actin is minimally affected by cold temperatures, although, as the temperature drops, the rate of filament formation slows. Our demonstration that the rate and extent of Pi release during this process closely parallels the rate of formation of F-actin indicates, for the first time, that the F-actin ATPase activity per se is not cold-sensitive. This situation is contrary to what is found with many enzyme-substrate systems in which cold temperatures do not inhibit substrate binding but do inhibit catalysis.

With 12 µM Mg2+-GG-actin, F-actin-dependent ATPase activity was not observed unless the temperature was >15 °C. This cold-sensitive behavior of GG-actin alone allows us for the first time to compare the effects of this double mutation quantitatively with the less severe polymerization defects observed with other alterations in the hydrophobic plug. The L267D mutant, in which a negative charge was placed between the two remaining hydrophobic groups required >6 °C for polymerization, whereas little if any effect was observed when either Val266 or Leu267 was altered singly to G or when Val266 was substituted with D (21).

Pi release is the slow step in the nucleotide cycle that occurs during the polymerization of muscle actin (1), and the lag between ATP hydrolysis and Pi release has been proposed to be an important factor in the rate of actin filament turnover (22). In this light, our observation that such a lag did not exist with yeast actin was very surprising and suggests the possibility of a comparatively greater degree of instability of yeast actin filaments compared with those of higher eukaryotic actins. We previously observed that nucleotide exchange in yeast actin is faster than in higher eukaryotic actins (4, 23). Furthermore, when we compared the rate of release of Pi by monomeric yeast and muscle actins (data not shown), the rate constant for the reaction in yeast G-actin (2.8 × 10-4 s-1) is faster than that exhibited by muscle actin (9 × 10-5 s-1). These findings reinforce the suggestion of an inherently less stable yeast actin filament in comparison with that of higher eukaryotic actins.

Systematically studying the ATPase activity that accompanies actin polymerization is inherently difficult because of the self-limiting nature of the reaction. Its rate slows drastically as polymerization reaches the steady state requiring that large amounts of actin be employed if reasonable signals are to be obtained. This problem can be circumvented somewhat by employing continuous sonication to make the ATPase reaction continuous. However, the awkwardness of this approach coupled with artifacts arising from the heat generated by the sonic probe makes this approach less than desirable. The continuous ATPase activity exhibited by GG-actin in F buffer potentially provides us with a means for experimentally addressing the mechanism of the actin-dependent hydrolysis of ATP under polymerizing conditions.

    ACKNOWLEDGEMENTS

We are grateful to Dr. Larry Tobacman for the muscle actin and his suggestions concerning the analysis of the data and the writing of the manuscript and to Kuo-Kuang Wen for preparing the tropomyosin used in this work.

    FOOTNOTES

* The work was supported by National Institutes of Health Grant GM-33689 (to P. A. R.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

Dagger To whom correspondence should be addressed: Dept. of Biochemistry, University of Iowa College of Medicine, Iowa City, IA 52242. Tel.: 319-335-7911; Fax: 319-335-9570; E-mail: peter-rubenstein@uiowa.edu.

Published, JBC Papers in Press, April 27, 2001, DOI 10.1074/jbc.M011797200

    ABBREVIATIONS

The abbreviations used are: F buffer, 2 mM MgCl2 and 50 mM KCl to G buffer; G buffer, 10 mM Tris-HCl, pH 7.5, 0.2 mM CaCl2, 0.2 mM ATP, and 0.5 mM DTT; WT, wild-type; PDM, N,N'-1,4-phenylenedimaleimide; PAGE, polyacrylamide gel electrophoresis; DTT, dithiothreitol; BeFx, beryllium fluoride; LD, lower dimer; UD, upper dimer.

    REFERENCES
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
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