HOME HELP FEEDBACK SUBSCRIPTIONS ARCHIVE SEARCH TABLE OF CONTENTS		QUICK SEARCH:   [advanced] Author: Keyword(s): Year:  Vol:  Page:

J. Biol. Chem., Vol. 282, Issue 51, 36782-36789, December 21, 2007

This Article Abstract Full Text (PDF) Supplemental Data All Versions of this Article: 282/51/36782    most recent M707007200v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via Google Scholar Google Scholar Articles by Wu, G. Articles by Ort, D. R. Search for Related Content PubMed PubMed Citation Articles by Wu, G. Articles by Ort, D. R. Related Collections Papers Of The Week Social Bookmarking                      What's this?

A Point Mutation in atpC1 Raises the Redox Potential of the Arabidopsis Chloroplast ATP Synthase -Subunit Regulatory Disulfide above the Range of Thioredoxin Modulation^*

Guosheng Wu¹, Guadalupe Ortiz-Flores², Adriana Ortiz-Lopez³, and Donald R. Ort⁴

From the Department of Plant Biology, University of Illinois, and the Photosynthesis Research Unit, United States Department of Agriculture Agricultural Research Service, Urbana, Illinois 61801

Received for publication, August 21, 2007 , and in revised form, October 19, 2007.

	ABSTRACT

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
The light-dependent regulation of chloroplast ATP synthase activity depends on an intricate but ill defined interplay between the proton electrochemical potential across the thylakoid membrane and thioredoxin-mediated redox modulation of a cysteine bridge located on the ATP synthase -subunit. The abnormal light-dependent regulation of the chloroplast ATP synthase in the Arabidopsis thaliana cfq (coupling factor quick recovery) mutant was caused by a point mutation (G to A) in the atpC1 gene, which caused an amino acid substitution (E244K) in the vicinity of the redox modulation domain in the -subunit of ATP synthase. Equilibrium redox titration revealed that this mutation made the regulatory sulfhydryl group energetically much more difficult to reduce relative to the wild type (i.e. raised the E_m,7.9 by 39 mV). Enzymatic studies using isolated chloroplasts showed significantly lower light-induced ATPase and ATP synthase activity in the mutant compared with the wild type. The lower ATP synthesis capacity in turn restricted overall rates of leaf photosynthesis in the cfq mutant under low light. This work provides in situ validation of the concept that thioredoxin-dependent reduction of the -subunit regulatory disulfide modulates the proton electrochemical potential energy requirement for activation of the chloroplast ATP synthase and that the activation state of the ATP synthase can limit leaf level photosynthesis.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
The chloroplast ATP synthase complex catalyzes the synthesis of ATP from ADP and free phosphate by coupling anhydride bond formation with the proton transmembrane electrochemical potential (µ_H⁺) across the thylakoid membrane and is one of the light-regulated enzymes of chloroplasts. In the light, the enzyme complex can be fully activated to achieve high capacity of ATP synthetic activity, whereas in the dark, it is converted to a catalytically inactive state, thereby preventing the dissipative cleavage of stromal ATP that would otherwise occur. The regulatory mechanisms governing the activity of this enzyme have been intensely investigated over the past several decades, revealing that regulation of the chloroplast ATP synthase catalytic activity is more intricate than that of its counterparts in mitochondria and bacteria.

There are at least three components involved in the regulation of chloroplast ATP synthase: µ_H⁺ formation across the thylakoid membrane, nucleotide binding and release to the catalytic and regulatory sites, and thiol modulation of disulfide bridge-forming cysteine residues on the -subunit (1). µ_H⁺ plays a central role in the regulation of chloroplast ATP synthase. In the light, the generation of µ_H⁺ induces conformational changes within the ATP synthase complex causing the release of bound ADP, activating the ATP synthase. As µ_H⁺ dissipates in the dark, these conformational changes and ADP release are reversed, inactivating the enzyme (2). These simple but subtle control devices avoid energy losses in the dark (3).

Redox modulation of the -subunit also plays an important role in regulating chloroplast ATP synthase activity and represents a level of regulation that is absent in the bacterial and mitochondrial homologs. In plants and green algae, the -subunit contains an extra domain of 40 amino acids (3) in which there is nested a unique sequence motif of nine amino acid residues, including two cysteines (4). Reversible disulfide bridge formation between the two cysteines enables regulation of the enzyme via redox thiol modulation. In vitro reduction can be achieved by dithiothreitol (DTT)⁵ addition, whereas in vivo reduction is through thioredoxin f that is reduced by photosystem I via ferredoxin-thioredoxin reductase (5). Unsurprisingly, deletion of the nine-amino acid motif containing the disulfide bridge-forming cysteines or replacement of the cysteines with alanine makes the enzyme insensitive to thiol modulation (6, 7). Redox modulation of the -subunit likely affects binding of the -subunit, which acts with the -subunit to repress activity (6, 8, 9).

Although the redox regulation of chloroplast ATPase and ATP synthase activity has been extensively studied, the in planta physiological function remains unclear in that redox modulation is not a prerequisite for either activation or deactivation of the chloroplast ATP synthase. Activation of the ATP synthase is a rapid process that normally precedes the thioredoxin-dependent reduction of -subunits following a dark-to-light transition (10). It has been shown that reduction of the -subunit lowers the µ_H⁺ threshold for activation of the chloroplast ATP synthase (11–13) and increases the efficiency of ATP formation as a function of µ_H⁺ (14, 15), likely by stabilizing the activated conformational state of the enzyme complex (16, 17). This makes it possible to sustain activated ATP synthase in low light. Additionally, the physiological significance of the oxidation, which results in disulfide bridge formation within the -subunit, is also uncertain because deactivation of the ATP synthase following a light-to-dark transition is normally more rapid than -subunit oxidation (10, 18, 19).

To investigate the physiological significance of the thiol modulation, we adopted a genetic approach to study the in situ regulation of ATP synthase in Arabidopsis thaliana. We previously developed a two-step screening strategy for the selection of ATP synthase activation mutants in Arabidopsis and chose several candidates in which redox responses of chloroplast ATP synthase differed compared with the wild type (20, 21). In one mutant, cfq, the energetic threshold for activation of the ATP synthase was insensitive to pre-illumination, behaving as though the -subunit regulatory disulfide was not reduced in the light. In the work reported here, we investigated the activity of the ATP synthase in the cfq mutant and discovered a point mutation in the cfq mutant atpC1 gene that resulted in an amino acid substitution (E244K) in the vicinity of the redox modulation domain in the -subunit of ATP synthase. Redox titration revealed that the midpoint potential of the regulatory sulfhydryl group on the cfq -subunit was nearly 40 mV more reducing than that of the wild type. The more negative midpoint potential resulted in a higher energetic threshold (i.e. higher µ_H⁺) for sustaining the activation of ATP synthase and thus lowered ATP synthase activity in the mutant under limiting light conditions. Photosynthetic rates of the mutant were lower than those of the wild type under the low light, consistent with the higher energy requirement for sustained activation of the ATP synthase and a lower capacity of ATP synthesis in the mutant.

	EXPERIMENTAL PROCEDURES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Plant Materials and Growth Conditions—The M₃ generation of the cfq mutant (20) was back-crossed three times with wild-type Col-0, and a homozygous line was chosen from the F₃ generation. Wild-type and mutant plants were grown at 20 °C on soil at 70–80% humidity under a 12/12-h light/dark photo-period with a photon flux density of 150 µmol m^–2 s^–1.

Measurement of A₅₁₈ Relaxation Kinetics—Plants 45 days old were initially dark-adapted for 12 h to ensure that -subunits of ATP synthase within the leaves were fully oxidized. A kinetic spectrophotometer was used to monitor the flash-induced absorbance change at 518 nm with detached leaves as described previously (20) with the exception that 7 s of continuous red light (65 µmol m^–2 s^–1) was used to induce -subunit reduction. A₅₁₈ relaxation kinetics were analyzed, and the relaxation time constants were calculated by fitting the initial 600 ms of the decay to a first-order exponential using an iterative nonlinear least-squares program (OriginLab Corp., Northampton, MA). The r² values of the fits were all 0.93.

Equilibrium Redox Titrations—Fully expanded detached leaves were infiltrated with varying ratios of oxidized and reduced 20 mM DTT solutions in 10 mM Tricine/NaOH (pH 7.9) containing 1% (v/v) Tween 20 (22). After 4 h of incubation in the dark, A₅₁₈ kinetic measurements were carried out. The equilibrium redox potential for DTT at pH 7.9 was calculated according to the following equation: E_m,7.9 = E_m,7 – 0.059(pH 7.9 – pH 7). E_m,7.9 is equal to –380 mV when using the E_m,7 value of –327 mV at 25 °C (23). The redox potentials (E_h) were calculated according to the Nernst equation: E_h = E_m,7.9 + (59/n)log([DTT^ox]/[DTT^red]), where n is equal to 2 for the two electrons involved in the thioredoxin-mediated thiol/disulfide exchange. The pH value of 7.9 mimics the stromal pH in the light (24).

DNA Sequencing of atpC1 of the cfq Mutant—Genomic DNA from cfq leaves was isolated; the entire atpC1 coding region for the -subunit of chloroplast ATP synthase was amplified by PCR using primers gama-1 (5'-TGTTTCACCACTCCAAGCGTCTC-3') and gama-2A (5'-TCAAAGAGGGTTCAAAACAAATCAAAC-3'); and the product was sequenced (25).

Complementation Analysis—C31 (26) containing the Arabidopsis Col-0 atpC1 gene was used as the PCR template, and a 1456-bp insert spanning the coding region was subcloned into the multicloning XbaI site of the pBI-121 binary vector (Clontech, Mountain View, CA). The insert was positioned downstream of the cauliflower mosaic virus 35S promoter and used for transformation of cfq mutant plants using the infiltration method (27). Transformants (T₁ generation) were selected on Murashige-Skoog medium containing 0.8% agar and 50 mg/liter kanamycin. Resistant plants were transferred to soil. The homozygous lines (T₃) were further selected on the same medium.

DNA Gel Blot Analysis—The genomic DNA was extracted from 3-week-old plants. Approximately 8 µg of DNA/lane was digested with EcoRV overnight, resolved on 0.7% (w/v) agarose gel, and transferred onto a Hybond-N nylon membrane (Amersham Biosciences). The blots were probed with [-³²P]dCTP-labeled XbaI fragment (Megaprime DNA labeling system, Amersham Biosciences) from C31 containing the whole atpC1 coding region. The blots were hybridized at 60 °C in hybridization solution (6x SSC (3 M NaCl and 3 M sodium citrate), 0.01 M EDTA (pH 8.0), 5x Denhardt's solution, 0.5% (w/v) SDS, and 100 mg/ml sheared denatured salmon sperm DNA) overnight; washed repeatedly for 15 min in a solution containing 30 mM NaCl, 3 mM Na₃C₆H₅O₇, and 0.1% (w/v) SDS; and then exposed to x-ray film (Kodak X-Omat AR) for 1 day.

RNA Gel Blot Analysis—Total RNA was isolated from fully expanded leaves using TRIzol reagent (Invitrogen). 10 µg of RNA was resolved on formaldehyde-containing 1% (w/v) agarose gel and transferred to a Hybond-N nylon membrane. Preparation of the atpC1 probe, hybridization, and washing were carried out essentially as described above for DNA gel blotting.

Immunoblot Analysis—Chloroplast thylakoid membranes were isolated following a published protocol (28). The membrane pellet was washed three times with ice-cold 10 mM NaCl and centrifuged at 7000 x g. The resulting thylakoid pellet was resuspended in 0.75 mM EDTA to a concentration of 50 µM chlorophyll. The suspension was shaken (200 rpm) for 10 min and centrifuged at 10,000 x g for 15 min. Coupling factor 1 (CF₁) was precipitated with ammonium sulfate at 50% saturation at 4 °C and collected by centrifugation at 10,000 x g for 5 min. The pellet was resuspended in 0.1 M Tris-HCl (pH 8.0) and desalted using Micro Bio-Spin columns (Bio-Gel P-6, Bio-Rad). Proteins were separated by SDS-PAGE on 12% acrylamide gels and transferred onto Immobilon-P transfer membrane (Millipore Corp., Bedford, MA). Immunoblot analyses were performed using an Immun-Blot assay kit (Bio-Rad). Antiserum raised against the spinach chloroplast ATP synthase β-subunits was used for detection of CF₁ β-subunits. The membrane was incubated with 1000-fold diluted rabbit antiserum and then with 5000-fold diluted alkaline phosphatase-conjugated goat anti-rabbit antibodies (Bio-Rad). Protein was detected colorimetrically using the 5-bromo-4-chloro-3-indolyl phosphate/nitro blue tetrazolium liquid substrate system (Sigma). Band intensities were analyzed using Adobe Photoshop 6.0.

View larger version (20K): [in this window] [in a new window]   FIGURE 1. A518 relaxation kinetics in wild-type and cfq Arabidopsis leaves. A518 relaxation kinetics were measured in >20 leaves using a flash kinetic spectrophotometer, and some representative responses are shown. Wild-type (A) and cfq (B) plants were dark-adapted for 12 h (Dad traces) and then illuminated with 65 µmol m–2 s–1 red light for 7 s and dark-adapted for 4 min (Lad traces). Wild-type (C) and cfq (D) plants were dark-adapted for 12 h (Dad traces), and leaves were then infiltrated with 1 mM DTT for 20 min (DTT traces).

Measurement of ATP Synthesis—Photophosphorylation was determined at various light intensities in reaction mixtures containing 20 mM Tricine/NaOH (pH 8.0), 25 mM NaCl, 5 mM MgCl₂, 3 mM ADP, 4 mM KH₂PO₄, 30 µM phenazine methosulfate, and chloroplasts equivalent to 0.22 µM chlorophyll in a total volume of 0.4 ml. ATP synthesis was initiated by illuminating the reaction mixtures with white light. After 10 min of incubation at 30 °C, the reaction was stopped by the addition of 0.4 ml of 8% trichloroacetic acid, and the amount of phosphate depleted from the medium was determined colorimetrically (29).

Photosynthetic Gas Exchange Measurements—Leaf gas exchange measurements were conducted on single rosette leaves at the bolting stage using an open gas exchange system (LI-6400, LI-COR Biosciences, Lincoln, NE). Prior to measurements, plants were dark-adapted for 1 h. The conditions were set at 21 °C and 60–70% relative humidity, and the CO₂ partial pressure was set to 370 µmol/mol (30). Each experimental treatment was performed with five replications.

Measurement of Growth Rate and Chlorophyll Content—For growth rate analysis, plants with four true leaves were moved to growth chambers at light intensities of 50, 100, and 150 µmol m^–2 s^–1 for 30 days. Shoot fresh weights were then measured.

For chlorophyll analysis, chlorophyll was extracted with 80% acetone from 0.1 g of rosette leaves. Chlorophyll contents were measured, and chlorophyll a/b ratios were determined according to the method of Graan and Ort (31).

	RESULTS

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 
Light-dependent Reduction of the Chloroplast ATP Synthase -Subunit Cysteine Disulfide Bond Is Impaired in the Arabidopsis cfq Mutant—Chloroplast ATP synthase activity can be monitored in intact leaves by taking advantage of the fact that the amplitude of light-induced electrochromic absorbance change with a peak at 518 nm (A₅₁₈) is closely linear to the amplitude of the electrical component of µ_H⁺ that is formed across the thylakoid membrane in the light (e.g. Refs. 10, 19, and 20). Fig. 1A shows that a single flash of light, strong and brief enough to excite all of the photosystem reaction centers in unison, generated a large µ_H⁺ across the thylakoid membrane. The slow first-order decay of A₅₁₈ (time constant of A₅₁₈ decay () = 257 ms) in dark-adapted wild-type leaves (Fig. 1A, D_ad trace) indicated that the catalytically inactive form of the ATP synthase predominated (20) and that the decay was due mainly to slow depolarization by ion movement across the thylakoid membrane rather than proton efflux through the ATP synthase. In wild-type leaves, 7 s of pre-illumination with 65 µmol m^–2 s^–1 red light was sufficient to fully activate the ATP synthase and to bring about the thioredoxin-dependent reduction of the -subunit. As we (20) and others (32) have shown, a subsequent 4-min dark adaptation results in deactivation of the ATP synthase but not oxidation of the -subunit. Under this condition, a single flash was sufficient to activate the ATP synthase, and the decay of A₅₁₈ was accordingly accelerated ( = 73 ms) because of the increased conductance of protons through the ATP synthase associated with ATP formation (Fig. 1A, L_ad trace). In cfq, the dark-adapted leaves exhibited the same slow decay of A₅₁₈ ( = 248 ms) (Fig. 1B, D_ad trace) seen in the wild type. However, in the mutant, the pre-illumination and subsequent 4-min dark adaptation caused only modest acceleration of the decay of A₅₁₈ ( = 161 ms) (Fig. 1B, L_ad trace), indicating substantially less activation of the ATP synthase.

To determine whether the lower activation of the ATP synthase in cfq was caused by impaired reduction of the -subunit, we pretreated leaves for 20 min with 1 mM DTT, which normally has the ability to at least partially reduce CF₁ -subunits (14). Fig. 1C illustrates that although 1 mM DTT pretreatment was not as efficient as pre-illumination, the reductant pretreatment substantially accelerated the decay of A₅₁₈ ( = 120 ms) in wild-type leaves. In contrast, there was no effect of 1 mM DTT pretreatment on the decay of A₅₁₈ in cfq (Fig. 1D), indicating that the -subunit of ATP synthase in cfq was still in the oxidized form after DTT pretreatment.

View larger version (21K): [in this window] [in a new window]   FIGURE 2. Equilibrium redox titrations of thiol/disulfide regulatory groups in the -subunit of the chloroplast ATP synthase. Leaves of the wild type (WT), the cfq mutant, and cfq mutants transformed with wild-type atpC1 (T3-2, T3-3, and T3-4) were infiltrated with 20 mM DTT at various reduced/oxidized ratios for 4 h at pH 7.9. The A518 relaxation kinetics were then measured and used to calculate the equilibrium midpoint potential of ATP synthase -subunit regulatory cysteines. The 95% confidence limits were calculated and are presented rounded to the nearest whole number.

View larger version (20K): [in this window] [in a new window]   FIGURE 3. Alignment of amino acid sequences of chloroplast -subunits. The amino acid sequence of the -subunits of ATP synthase encoded by A. thaliana atpC1 (AT4G04640) is aligned with those of Spinacia oleracea (CAA68727) and Chlamydomonas reinhardtii (1808328A) as described previously (26). Shaded boxes indicate sequence identity. The E244K substitution in atpC1 of the cfq mutant is shown above the alignment. The two regulatory cysteine residues are shown at positions 199 and 205.

Identification of a Point Mutation in the -Subunit Encoding the atpC1 Gene of cfq—In A. thaliana, there are two nuclear genes encoding the -subunit of the chloroplast ATP synthase, atpC1 (At4G04640) and atpC2 (At1G15700). atpC1 is a light-regulated gene with a GT-1-binding site upstream of the coding region (26). The expression of atpC2 is negligible (26) and was found not to be sufficient to compensate for the lack of atpC1 in the dpa1 null mutant (34), implying the -subunit of the Arabidopsis chloroplast ATP synthase to be exclusively the product of the atpC1 gene. The entire coding region of the cfq mutant atpC1 gene was amplified by PCR and sequenced. Comparison of the mutant sequence with the wild-type sequence identified a point mutation (G to A) located at position 2447 in the coding region of the gene. The substitution resulted in a change in the amino acid sequence from negatively charged Glu to positively charged Lys at position 244 within a region of the protein sequence that is highly conserved among photosynthetic eukaryotes (Fig. 3). This conserved region is located close to the C-terminal end of the protein and 38 amino acids from the second cysteine residue in the redox regulatory domain, strongly suggesting that this substitution caused the specific alteration in the redox properties of -subunits present in cfq.

To obtain conclusive evidence that alteration of the atpC1 gene led to the abnormal A₅₁₈ relaxation kinetic phenotype and midpoint redox potential of cfq, a Pro35S::atpC1 construct was introduced into cfq plants. Several kanamycin-resistant transformants were isolated, and the presence of the transgene construct was confirmed by DNA gel blot analysis (supplemental Fig. 1A). RNA blot analysis demonstrated that atpC1 was highly expressed in the transgenic lines compared (supplemental Fig. 1B).

View larger version (17K): [in this window] [in a new window]   FIGURE 4. Rescue of the cfq phenotype in transgenic lines by transformation with wild-type atpC1. Leaves were dark-adapted for 12 h to fully deactivate and oxidize the chloroplast ATP synthase. Leaves were then illuminated for 7 s with 65 µmol m–2 s–1 red light. The A518 relaxation kinetics were measured before (white bars) and after (black bars) pre-illumination. A518 relaxation time constants were calculated from five to seven independent measurements.

It was a possibility that the cfq -subunit mutation resulted in assembly or stability problems and that the mutant phenotype was the result of a decrease in the ATP synthase content in the thylakoid membrane of the mutant. Additionally, the overexpression of wild-type atpC1 in the transgenic plants may have driven an increase in the content of the ATP synthase in the thylakoid membrane, accounting for the observed acceleration of the decay of A₅₁₈. To investigate this possibility, immunoblotting was performed to determine the ATP synthase β-subunit content. Each ATP synthase contains three β-subunits, and quantifying the β-subunits enables the determination of the total chloroplast ATP synthase content. The immunoblot of the β-subunits revealed that the chloroplast ATP synthase in cfq and overexpression lines accumulated normally and to the same level as in the wild type (supplemental Fig. 2), indicating that the mutation in the -subunit of the cfq mutant and overexpression of the wild-type atpC1 gene in the cfq background had no significant influence on the content of ATP synthase. An increased expression of several or all genes of the ATP synthase appears to be necessary to regulate the abundance of the complex. Thus, the cfq and transgenic phenotypes were caused by the differences in the function of the -subunit of ATP synthase rather than a change in the ATP synthase content in the thylakoid membrane.

View larger version (22K): [in this window] [in a new window]   FIGURE 5. A518 relaxation time constant as a function of pre-illumination time. A, leaves were dark-adapted for 12 h and then pre-illuminated with 65 µmol m–2 s–1 red light for the times indicated. After a 4-min dark re-adaptation, A518 relaxation kinetics were measured, and A518 relaxation time constants were calculated. B, leaves were dark-adapted for 12 h, illuminated with 65 µmol m–2 s–1 red light for 7 s, and dark-readapted for the times indicated. A518 relaxation kinetics were measured, and A518 relaxation time constants were calculated. A518 relaxation time constants were calculated from five to seven independent measurements.

View larger version (23K): [in this window] [in a new window]   FIGURE 6. Dependence of ATP synthase/hydrolyase activity on illumination intensity. A, ATP hydrolyase activity was measured as inorganic phosphate released by thylakoid membranes exposed to various light intensities for 2 min. Each data point represents the mean ± S.E. of four individual samples. B, ATP synthase activity was measured as inorganic phosphate depletion by thylakoid membranes as a function of light intensity. Each data point represents the mean ± S.E. of four individual samples. chl, chlorophyll.

The time course for the light-dependent activation of ATPase activity was determined in chloroplasts isolated from wild-type and cfq leaves (Fig. 6A). Illumination with low light increased the enzyme activity by 2-fold in the wild type, whereas the ATPase activity responded only slightly to the illumination in the cfq mutant. The ATP synthesis in isolated wild-type chloroplasts increased as light intensity was increased, responding to the rise of the proton gradient across the thylakoid membranes, and saturated at 600 µmol m^–2 s^–1 (Fig. 6B). Although the cfq mutant showed a similar trend compared with the wild type, the ATP synthase activities were lower at all intensities (Fig. 6B).

View larger version (17K): [in this window] [in a new window]   FIGURE 7. Effect of the cfq mutation on photosynthetic and growth parameters. A, CO2 assimilation rates of cfq and the wild type (WT) were compared at illumination intensities of 50, 100, and 200 µmol m–2 s–1. Error bars represent the mean ± S.E. of five or six individual plants. B, wild-type and cfq plants with two true leaves were moved to growth light intensities of 50, 100, and 150 µmol m–2 s–1. After 30 days, shoot fresh weights were measured. Error bars represent the mean fresh weight ± S.E. of five plants from three individual experiments. PFD, photon flux density.

	DISCUSSION

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

In an atpC1 null mutant missing the -subunit of chloroplast ATP synthase, the entire ATP synthase complex is destabilized, leading to a lethal phenotype (34) and highlighting the importance of this gene. The atpC1 gene in cfq was determined to carry a single base pair mutation changing the amino acid sequence within a highly conserved motif proximal to the cysteine residues (Cys¹⁹⁹ and Cys²⁰⁵) in the redox regulatory domain of the -subunit. Several studies confirmed the regulatory importance of the residues proximal to the dithiol-containing domain. Deletion from Glu²¹⁰ to Glu²¹² in the -subunit of the ATPase complex results in a mutant in which the complex is inactivated rather than activated by reduction of the disulfide bond (38). In contrast, deletion from Glu²¹² to Ile²³⁰ confers high ATPase activity independent of DTT treatment (38). In vitro study of assembled CF₁ with various mutant -subunits showed that deletion from Thr²²⁴ to Ile²⁴⁰ or from Glu¹⁹⁷ to Ile²⁴⁰ results in an active enzyme insensitive to redox control (6). All of these studies demonstrated an important role of the amino acid residue segment proximal to the regulatory dithiol. However, in the absence of redox titration data, it is not clear whether these mutations in the -subunit alter the redox properties of the enzyme complex.

On the basis of the modeled structure (6, 9) and the amino acid sequence (4, 39) of the chloroplast -subunit that placed the point mutation of cfq close to the thiol-modulated cysteine motif and within a conserved domain of the -subunit (Fig. 3), we hypothesized that the point mutation might change the redox property of the two cysteines. The midpoint redox potential (E_m,7.9) for the wild-type ATP synthase was –337 ± 4 mV, whereas that for the cfq mutant markedly shifted to a more reducing potential of –376 ± 5 mV (Fig. 2). The shift of the -subunit redox potential in cfq would make the ATP synthase more difficult to reduce by the natural reductant thioredoxin f, which has an equilibrium midpoint potential near –325 ± 10 mV at pH 7.9 (33). Indeed, under conditions in which the wild-type -subunit would be 75% reduced (i.e. when thioredoxin f is 90% reduced), the cfq -subunit would be only 10% reduced. The substitution of negatively charged glutamic acid (Glu²⁴⁴) with positively charged lysine represents a significant change in the local electrostatic environment of the protein. The electrostatic change alone or coupled with a charge-driven conformational change in the -subunit is a likely candidate for making the disulfide bond between the two cysteines more stable and difficult to reduce. Our results demonstrate that the conserved amino acid residue segment proximal to the regulatory dithiol bridge is necessary for maintaining the physiologically appropriate redox range for the cysteine thiol/disulfide equilibrium.

It is thought that four protons pass through the ATP synthase from the thylakoid lumen to the stroma to generate one ATP from ADP and phosphate. To investigate the possibility of impaired proton utilization efficiency in cfq, we also measured ATP hydrolysis and synthesis activity. The ATP synthase activity of cfq (monitored as the dissipation of µ_H⁺ following a light flash) could reach the same magnitude as that of the wild type after a longer pre-illumination period (Fig. 5), but the ATP hydrolysis and synthesis activity were lower than those of the wild type at all times and all intensities under continuous light (Fig. 6). This difference in behavior is explained by the fact that ATP synthesis following a flash of light is less limited by the amount of active ATP synthase than is ATP synthesis in continuous light (10, 14). Together, these results show that the -subunit point mutation lowered the efficiency of ATP formation.

That lower photosynthetic rates in cfq were observed only under low light conditions (Fig. 7A) is in agreement with predictions of the well validated biochemical model of leaf photosynthesis (40) that, in limiting light, photosynthesis is primarily limited by the rate of ATP formation and NADPH production. As light intensities approach saturation, photosynthesis is increasingly ribulose-bisphosphate carboxylase/oxygenase-limited, and thus, the difference in net CO₂ reduction between wild-type and cfq leaves would be expected to disappear. The cfq plants grown under low light intensity (50 µmol m^–2 s^–1) showed substantially slower shoot growth rates compared with the wild-type plants, almost certainly due to the lower photosynthetic rate of cfq at low light (Fig. 7B), suggesting that plants may benefit from the thiol modulation system under low light conditions. That cfq but not wild-type plants growing under low light accumulated less chlorophyll than those growing under normal light conditions (Table 1) is likely another manifestation of lower rates of ATP formation due to the cfq mutation in the -subunit.

	FOOTNOTES

 
^* The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

The on-line version of this article (available at http://www.jbc.org) contains supplemental Figs. 1 and 2.

This article was selected as a Paper of the Week.

¹ Present address: Dept. of Botany, University of Wisconsin, Madison, WI 53706.

² Present address: Agriculture School, Universidad de Guanajuato, Irapuato, Guanajuato 36500, México.

³ Present address: Joslin Diabetes Center, Harvard University, One Joslin Place, Boston, MA 02210.

⁴ To whom correspondence should be addressed: Dept. of Plant Biology, 1406 Inst. of Genomic Biology, 1206 West Gregory Dr., University of Illinois, Urbana, IL 61801. Tel.: 217-333-2093; Fax: 217-244-2057; E-mail: d-ort{at}uiuc.edu.

⁵ The abbreviations used are: DTT, dithiothreitol; Tricine, N-[2-hydroxy-1,1-bis(hydroxymethyl)ethyl]glycine; CF₁, coupling factor 1.

	ACKNOWLEDGMENTS

 
We are most grateful to M. L. Richter for providing antiserum against the spinach chloroplast ATP synthase β-subunits and M. Futai for providing the C31 construct. We acknowledge Dr. Aleel Grennan for expert assistance with the manuscript and Dr. Carl Bernacchi for assistance with curve fitting.

	REFERENCES

TOP ABSTRACT INTRODUCTION EXPERIMENTAL PROCEDURES RESULTS DISCUSSION REFERENCES

 

1. Ort, D. R., and Oxborough, K. (1992) Annu. Rev. Plant Physiol. Plant Mol. Biol. 43, 269–291[CrossRef]
2. Kleefeld, S., Lohse, D., Mansy, A. R., and Strotmann, H. (1990) Biochim. Biophys. Acta 1019, 11–18
3. Richter, M. L. (2004) Photosynth. Res. 79, 319–329[CrossRef][Medline] [Order article via Infotrieve]
4. Miki, J., Maeda, M., Mukohata, Y., and Futai, M. (1988) FEBS Lett. 232, 221–226[CrossRef][Medline] [Order article via Infotrieve]
5. Wolosiuk, R. A., and Buchanan, B. B. (1977) Nature 266, 565–567[CrossRef]
6. Samra, H. S., Gao, F., He, F., Hoang, E., Chen, Z., Gegenheimer, P. A., Berrie, C. L., and Richter, M. L. (2006) J. Biol. Chem. 281, 31041–31049[Abstract/Free Full Text]
7. Gao, R., Lipscomb, B., Wu, I., and Richter, M. L. (1995) J. Biol. Chem. 270, 9763–9769[Abstract/Free Full Text]
8. Hightower, K. E., and McCarty, R. E. (1996) Biochemistry 35, 4847–4851
9. Richter, M. L., Samra, H. S., He, F., Giessel, A. J., and Kuczera, K. K. (2005) J. Bioenerg. Biomembr. 37, 467–473[CrossRef][Medline] [Order article via Infotrieve]
10. Kramer, D. M., Wise, R. R., Frederick, J. R., Alm, D. M., Hesketh, J. D., Ort, D. R., and Crofts, A. R. (1990) Photosynth. Res. 26, 213–222[CrossRef]
11. Davenport, J. W., and McCarty, R. E. (1981) J. Biol. Chem. 256, 8947–8954[Abstract/Free Full Text]
12. Mills, J. D., and Mitchell, P. (1982) FEBS Lett. 144, 63–67[CrossRef]
13. Nalin, C. M., and McCarty, R. E. (1984) J. Biol. Chem. 259, 7275–7280[Abstract/Free Full Text]
14. Hangarter, R. P., Grandoni, P., and Ort, D. R. (1987) J. Biol. Chem. 262, 13513–13519[Abstract/Free Full Text]
15. Ketcham, S. R., Davenport, J. W., Warncke, K., and McCarty, R. E. (1984) J. Biol. Chem. 259, 7286–7293[Abstract/Free Full Text]
16. Richter, M. L., and McCarty, R. E. (1987) J. Biol. Chem. 262, 15037–15040[Abstract/Free Full Text]
17. Komatsu-Takaki, J. (1992) J. Biol. Chem. 267, 2360–2363[Abstract/Free Full Text]
18. Noctor, G., and Mills, J. D. (1988) Biochim. Biophys. Acta 935, 53–60
19. Ortiz-Lopez, A., Ort, D. R., and Boyer, J. S. (1991) Plant Physiol. 96, 1018–1025[Abstract/Free Full Text]
20. Gabrys, H., Kramer, D. M., Crofts, A. R., and Ort, D. R. (1994) Plant Physiol. 104, 769–776[Abstract]
21. Gong, P., Wu, G., and Ort, D. R. (2006) Photosynth. Res. 88, 133–142[CrossRef][Medline] [Order article via Infotrieve]
22. Hutchison, R. S., and Ort, D. R. (1995) Methods Enzymol. 252, 220–228[Medline] [Order article via Infotrieve]
23. Lees, W. J., and Whitesides, G. M. (1993) J. Org. Chem. 58, 642–647[CrossRef]
24. Werda, K., Heldt, H. W., and Milovancev, M. (1975) Biochim. Biophys. Acta 396, 276–292[Medline] [Order article via Infotrieve]
25. Chung, D. W., Pruzinska, A., Hortensteiner, S., and Ort, D. R. (2006) Plant Physiol. 142, 88–97[Abstract/Free Full Text]
26. Inohara, N., Iwamoto, A., Moriyama, Y., Shimomura, S., Maeda, M., and Futai, M. (1991) J. Biol. Chem. 266, 7333–7338[Abstract/Free Full Text]
27. Clough, S. J., and Bent, A. F. (1998) Plant J. 16, 735–743[CrossRef][Medline] [Order article via Infotrieve]
28. Whitmarsh, J., and Ort, D. R. (1984) Arch. Biochem. Biophys. 231, 378–389[CrossRef][Medline] [Order article via Infotrieve]
29. Chifflet, S., Torriglia, A., Chiesa, R., and Tolosa, S. (1988) Anal. Biochem. 168, 1–4[CrossRef][Medline] [Order article via Infotrieve]
30. Leakey, A. D. B., Uribelarrea, M., Ainsworth, E. A., Naidu, S. L., Rogers, A., Ort, D. R., and Long, S. P. (2006) Plant Physiol. 140, 779–790[Abstract/Free Full Text]
31. Graan, T., and Ort, D. R. (1984) J. Biol. Chem. 259, 14003–14010[Abstract/Free Full Text]
32. Kramer, D. M., and Crofts, A. R. (1989) Biochim. Biophys. Acta 976, 28–41
33. Hutchison, R. S., Groom, Q., and Ort, D. R. (2000) Biochemistry 39, 6679–6688[CrossRef][Medline] [Order article via Infotrieve]
34. Bosco, C. D., Lezhneva, L., Biehl, A., Leister, D., Strotmann, H., Wanner, G., and Meurer, J. (2004) J. Biol. Chem. 279, 1060–1069[Abstract/Free Full Text]
35. Schumann, J., Richter, M. L., and McCarty, R. E. (1985) J. Biol. Chem. 260, 11817–11823[Abstract/Free Full Text]
36. Moroney, J. V., and McCarty, R. E. (1982) J. Biol. Chem. 257, 5910–5914[Abstract/Free Full Text]
37. McCarty, R. E. (2005) J. Bioenerg. Biomembr. 37, 289–299[CrossRef][Medline] [Order article via Infotrieve]
38. Konno, H., Yodogawa, M., Stumpp, M. T., Kroth, P., Strotmann, H., Motohashi, K., Amano, T., and Hisabori, T. (2000) Biochem. J. 352, 783–788[CrossRef][Medline] [Order article via Infotrieve]
39. Moroney, J. V., Fullmer, C. S., and McCarty, R. E. (1984) J. Biol. Chem. 259, 7281–7285[Abstract/Free Full Text]
40. Farquhar, G. D., von Caemmerer, S., and Berry, J. A. (1980) Planta 149, 78–90[CrossRef]

CiteULike

Complore

Connotea

Del.icio.us

Digg

Reddit

Technorati

This Article Abstract Full Text (PDF) Supplemental Data All Versions of this Article: 282/51/36782    most recent M707007200v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via Google Scholar