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BIOENERGETICS AND PHOTOSYNTHESIS

The Catalytic Properties of Hybrid Rubisco Comprising Tobacco Small and Sunflower Large Subunits Mirror the Kinetically Equivalent Source Rubiscos and Can Support Tobacco Growth^1,[W],[OA]

Molecular Plant Physiology Group, Research School of Biological Sciences, Australian National University, Canberra, Australian Capital Territory 0200, Australia (R.E.S., S.v.C., S.M.W.); and Waksman Institute, Department of Plant Biology and Pathology, Rutgers, The State University of New Jersey, Piscataway, New Jersey 08854–8020 (P.M.)

	ABSTRACT

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

 
Plastomic replacement of the tobacco (Nicotiana tabacum) Rubisco large subunit gene (rbcL) with that from sunflower (Helianthus annuus; rbcL^S) produced tobacco^Rst transformants that produced a hybrid Rubisco consisting of sunflower large and tobacco small subunits (L^sS^t). The tobacco^Rst plants required CO₂ (0.5% v/v) supplementation to grow autotrophically from seed despite the substrate saturated carboxylation rate, K_m, for CO₂ and CO₂/O₂ selectivity of the L^sS^t enzyme mirroring the kinetically equivalent tobacco and sunflower Rubiscos. Consequently, at the onset of exponential growth when the source strength and leaf L^sS^t content were sufficient, tobacco^Rst plants grew to maturity without CO₂ supplementation. When grown under a high pCO₂, the tobacco^Rst seedlings grew slower than tobacco and exhibited unique growth phenotypes: Juvenile plants formed clusters of 10 to 20 structurally simple oblanceolate leaves, developed multiple apical meristems, and the mature leaves displayed marginal curling and dimpling. Depending on developmental stage, the L^sS^t content in tobacco^Rst leaves was 4- to 7-fold less than tobacco, and gas exchange coupled with chlorophyll fluorescence showed that at 2 mbar pCO₂ and growth illumination CO₂ assimilation in mature tobacco^Rst leaves remained limited by Rubisco activity and its rate (approximately 11 µmol m^–2 s^–1) was half that of tobacco controls. ³⁵S-methionine labeling showed the stability of assembled L^sS^t was similar to tobacco Rubisco and measurements of light transient CO₂ assimilation rates showed L^sS^t was adequately regulated by tobacco Rubisco activase. We conclude limitations to tobacco^Rst growth primarily stem from reduced rbcL^S mRNA levels and the translation and/or assembly of sunflower large with the tobacco small subunits that restricted L^sS^t synthesis.

Genetic manipulation of Rubisco in crop plants is hindered by several factors that are particularly complicated by the disparate location of the genes coding for the approximately 54 kD large subunit (L, coded by a single rbcL gene in the plastome) and the approximately 14 kD small subunits (S, coded by multiple RbcS gene copies in the nucleus). Assembly of the cytosolically synthesized S with the stromally synthesized L that contain the catalytic active sites into hexadecameric enzyme (L₈S₈) within the stroma occurs via a complex, highly organized chaperone-assisted mechanism that further restrains genetic manipulation of Rubisco in higher plants (Whitney and Andrews, 2001a; Zhang et al., 2002). It has been shown the preferred position of rbcL is in the chloroplast genome (plastome; Kanevski and Maliga, 1994), while an appropriate means for the engineering changes to the native (or inserting a foreign) RbcS in higher plants have remained elusive. Directly transplanting in catalytically more efficient Rubiscos from nongreen algae by transplastomic insertion of their genes for L and S into the tobacco (Nicotiana tabacum) plastome was frustrated by folding incompatibilities that precluded productive assembly of the foreign enzyme in tobacco chloroplasts (Whitney et al., 2001). Directed manipulation of RbcS in higher plants is complicated by the multiple copies that essentially precludes them from targeted mutagenic or replacement strategies. The difficulty with engineering changes to S via transplastomic manipulation is further compounded by an apparent preferential assembly of cytosolically synthesized S with the L subunits (Whitney and Andrews, 2001a; Zhang et al., 2002). Only by reducing the level of cytosolic S by >90% by antisensing RbcS and inserting a copy of rbcS in a highly transcribed region of the tobacco chloroplast genome could sufficient quantities of plastid synthesized S be incorporated into assemble tobacco Rubisco hexadeamers (Dhingra et al., 2004).

The generation of fully autotrophic and reproductive transplastomic tobacco-rubrum lines where the native L₈S₈ tobacco Rubisco has been replaced by the structurally simple L₂ form from the bacterium Rhodospirillum rubrum demonstrated the feasibility of replacing Rubisco in higher plants (Whitney and Andrews, 2001b). These lines were produced via homologous replacement of the tobacco rbcL gene with the R. rubrum Rubisco gene, rbcM. Importantly, the CO₂ response of photosynthesis in the tobacco-rubrum transformants was consistent with the content and kinetic properties of R. rubrum Rubisco (Whitney and Andrews, 2003). Earlier attempts to replace tobacco rbcL with the comparable gene from a cyanobacterium (Synechococcus PCC6301) or sunflower (Helianthus annuus) produced transformants that were nonautotrophic since they produced either no Rubisco (those containing the PCC6301 rbcL) or assembled a hybrid Rubisco hexadecamer (L^sS^t) comprising sunflower L and tobacco S (Kanevski et al., 1999). In the leaves of the latter transformant (line Nt-pIK83-1; Kanevski et al., 1999) grown in tissue culture the amount of hybrid enzyme was reduced by approximately 70%. The impeded autotrophic growth of line Nt-pIK83-1 in air necessitated grafting of the tissue onto wild-type tobacco to procure T₀ seed (Kanevski et al., 1999).

In this study we show that line Nt-pIK83-1 can be grown photoautotrophycally at elevated CO₂ levels and demonstrate that the kinetic properties of the hybrid L^sS^t mirror those of the source Rubiscos and that the hybrid enzyme is regulated appropriately by tobacco activase in vivo. We show the inability of juvenile Nt-pIK83-1 plants to grow in air and their delayed development at high pCO₂ is likely due to inadequate amounts of hybrid L^sS^t enzyme in the young vegetative tissue to provide sufficient source strength for development.

	RESULTS

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

 

Tobacco^Rst Variants Grown in Soil at High CO₂ Have Abnormal Phenotypic Features

Successful replacement of the plastome rbcL copy in tobacco with sunflower rbcL (rbcL^S) by Kanevski et al. (1999) produced tobacco transformants that produced a hybrid Rubisco comprising eight sunflower large subunits (L^s) and eight tobacco small subunits (S^t). We identify the transformed line Nt-pIK83-1 (Kanevski et al., 1999) as tobacco^Rst (tobacco with a hybrid Rubisco comprising sunflower L and tobacco S) and its hybrid hexadecameric Rubisco as L^sS^t. Limitations in the catalytic properties and content of L^sS^t were proposed to perturb autotrophic growth in air of tobacco^Rst plants grown in soil. Analogous to other tobacco transgenic lines expressing less Rubisco (Rodermel et al., 1988; Hudson et al., 1992) or catalytically perturbed foreign or mutated Rubiscos (Whitney et al., 1999; Whitney and Andrews, 2001b), the T₁ generation of the tobacco^Rst line Nt-pIK83-1 (Kanevski et al., 1999) could be grown in soil in air enriched with CO₂. The phenotype of the T₁ progeny was different to wild-type tobacco (see figure 2 in Andrews and Whitney, 2003) and to ensure the phenotype was not a consequence of unwanted nuclear mutations the tobacco^Rst flowers were repeatedly backcrossed with wild-type pollen. No change in the phenotype of multiple plants screened in the T₂ or T₃ progeny have been found and sequencing of the rbcL^S and flanking plastome sequence (approximately 0.2 kb either side) showed no unwanted mutations.

View larger version (20K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 2. CO2 assimilation rates in tobaccoRst and wild-type tobacco plants and their Rubisco kinetics. A, Gas-exchange measurements of CO2 assimilation rates in response to intercellular pCO2 measured at an irradiance of 350 (white symbols) or 950 (black symbols) µmol quanta m–2 s–1 and leaf temperature of 25°C. Measurements were made on attached leaves from two wild-type plants (wt1, 13.5 cm leaf diameter; wt2, 15 cm leaf diameter containing 33.2 and 30.6 µmol Rubisco sites m–2, respectively) and two tobaccoRst plants (tobRst1 and tobRst2; both 12 cm leaf diameters with 5.8 and 4.9 µmol Rubisco sites m–2, respectively). The Rubisco limited CO2 assimilation rates for wt1 () and tobRst2 () were modeled according to Farquhar et al. (1980) using estimates of maximal ribulose-P2 dependent carboxylase activity. B, Vcmax, Km for CO2 under ambient O2 levels (Kc21%O2), and CO2/O2 specificity (Sc/o) measured using leaf protein extracts and purified Rubisco preparations. See "Materials and Methods" for further details. Vcmax measurements in bold italics are those made using leaf tissue from tissue culture grown plants; see Supplemental Figure S3 for details. Superscript a indicates data from Whitney et al. (1999) and superscript b indicates data from Kanevski et al. (1999).

View larger version (64K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 1. Growth and phenotype of tobaccoRst plants compared with wild-type tobacco grown in air containing 0.5% (v/v) CO2 (see "Material and Methods" for further details). A, Phenotype of wild-type and tobaccoRst (B and C) plants (tobRst1 and tobRst4, both germinated from the same seed stock of a T2 plant derived from previous generations only backcrossed with wild-type pollen) at the juvenile (top sections) and mature growth stage. The number of days since cotyledon emergence is shown. The white arrows indicate the normal oblanceolate leaves (A and B) and irregular oblanceolate leaves (C) analyzed in Figure 7. D, Change in height of the primary axial shoot for wild-type (, n = 6) and tobaccoRst plants with one (tobRst1, , n = 1), two (, n = 2), or four (tobRst4, , n = 1) primary axial shoots. The exponential growth rates (black lines) were modeled to the height data according to the equation where A1 is the amplitude, t1 the time constant (calculated values are shown), and Y0 is the offset. E, Comparison of a mature wild-type and tobRst leaf (F) with the marginal dimpling phenotype in the tobRst lines not evident when grown in Suc containing tissue culture medium (G; Svab and Maliga, 1993).

View larger version (45K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 7. Comparison of Rubisco activase content and Rubisco production in juvenile wild-type tobacco and tobaccoRst (tRst) leaves grown in air containing 0.5% (v/v) CO2. Total and soluble protein from 0.3 cm2 of normal ovate wild-type leaves (n = 6) and the strappy oblanceolate tRst leaves (n = 4; refer to white arrows in Fig. 1, A–C) were separated by SDS-PAGE and stained with Coomassie Blue (A) or replicate samples (B) blotted and probed with antibodies raised against spinach Rubisco (Rubisco L antibody) and tobacco Rubisco activase (activase antibody). For comparison, the content of Rubisco active sites measured in the soluble leaf protein by [14C]CABP binding are shown. C, The abundance of rbcLS (black) and rbcLS-aadA (white) transcripts in the tRst samples relative to the average amount of rbcL message in wild type measured from RNA blots probed with 5'rbcL (see Fig. 6B for example). The RTE was obtained by dividing Rubisco content by transcript abundance. For tobaccoRst, the RTE in parentheses is calculated from the sum of the abundances of the rbcLS and rbcLS-aadA transcripts.

Photosynthesis in Tobacco^Rst Leaves Corresponds to the Content and Catalytic Properties of the Hybrid Rubisco

Photosynthetic gas-exchange CO₂ response measurements in young fully expanded tobacco^Rst leaves showed CO₂ assimilation rates were largely independent of light intensity below 2 mbar CO₂, consistent with assimilation remaining Rubisco activity limited below this CO₂ concentration (Fig. 2A ). This was confirmed by simultaneous chlorophyll fluorescence measurements that showed electron transport rate continued to increase above 1,600 µbar CO₂ while nonphotochemical quenching remained high (Supplemental Fig. S2). In wild-type controls assimilation was limited by light-dependent regeneration of ribulose-P₂ at approximately 300 to 600 µbar CO₂, depending on the illumination intensity. The maximum assimilation rates for tobacco^Rst (approximately 11 µmol m^–2 s^–1) were half of wild type (approximately 22 µmol m^–2 s^–1) at growth illumination (350 µmol quanta m^–2) with CO₂ compensation points of 97 and 49 µbar CO₂, respectively. Simultaneous measurements of stomatal conductance showed little difference between tobacco^Rst (0.21 ± 0.02 µmol m^–2 s^–1) and wild-type leaves (0.26 ± 0.02 µmol m^–2 s^–1) under growth light. Likewise, the measured F_v/F_m, chlorophyll content, and chlorophyll a/b ratio in the same tobacco^Rst leaves mirrored the wild-type controls, indicating no apparent perturbation in photochemical efficiency or elevated photoinhibition in tobacco^Rst under the growth conditions (Table I).

After taking into consideration the reduced Rubisco content, the initial slope of the assimilation curves for the tobacco^Rst leaves were inconsistent with the hybrid L^sS^t having a 5-fold higher K_m for CO₂ (K_c) and 4-fold lower substrate-saturated carboxylase activity (V_c^max) as reported previously (Kanevski et al., 1999). When limited by carboxylase activity, the slope of the CO₂ assimilation rate in response to changing pCO₂ is dependant on Rubisco content, V_c^max, and K_c^21%O₂ (K_m for CO₂ at ambient pO₂ and equals K_c[1+O/K_o] where K_o is the K_m for O₂ and O is the O₂ concentration; Farquhar et al., 1980; von Caemmerer et al., 1994). Both K_c^21%O₂ and V_c^max were measured for the tobacco^Rst, tobacco, and sunflower Rubiscos in vitro using rapidly sampled soluble protein extracts from mature leaves (Fig. 2B). The measured values for wild-type tobacco Rubisco matched those measured previously and were comparable to that measured for the sunflower and tobacco^Rst Rubiscos, indicating all three enzymes show similar kinetics and, most importantly, that the catalytic turnover and substrate CO₂ affinity of the hybrid enzyme was not impaired. Comparable rates of catalytic turnover were measured using leaf protein extracts from tobacco^Rst and tobacco plants grown in tissue culture (Fig. 2B) even when extracted and assayed in the extraction buffer used by Kanevski et al. (1999; Supplemental Fig. S3).

Purified Rubisco from tobacco^Rst, tobacco, and sunflower was used to measure their CO₂/O₂ selectivity, which again were highly similar (Fig. 2B). As evident in Figure 2A, the modeled assimilation rate of tobacco^Rst using the in vitro kinetic (V_c^max, 3.3 s^–1:K_c^21%O₂, 20.8 µM) and Rubisco content measurements (determined by [¹⁴C]carboxyarabinitol-P₂ binding, see below) closely matched that measured by whole leaf gas exchange supporting the validity of the measured kinetic parameters.

Even in air containing 0.5% (v/v) CO₂ the growth of tobacco^Rst remains Rubisco activity limited. Ribulose-P₂ content in young fully expanded tobacco^Rst leaves was approximately 50% higher and the 3-PGA content approximately 3-fold lower compared to wild-type controls, resulting in a 9-fold increase in the ribulose-P₂ to 3-PGA ratio (Table I). Both the dry weight and starch content of tobacco^Rst leaves were similarly reduced one-third while the fresh weight of the tobacco^Rst leaves matched wild type, indicating the leaves of the mutants were highly hydrated.

Rubisco and Rubisco Activase Content in Mature Leaves

As Rubisco content varies considerably with leaf age (Rodermel, 1999; Miller et al., 2000) significant care was made to undertake all biochemical measurements on the expanding fifth leaf from plants of similar height during the fast growth phase. In both wild-type and tobacco^Rst the width of the fifth leaf was 10% to 15% less than the widest seventh leaf and positioned at similar heights in the canopy. The binding affinity of the hybrid L^sS^t enzyme for carboxyarbinitol-P₂ was tested using the [¹⁴C]/[¹²C]-carboxyarabinitol-P₂ exchange method (Schloss, 1988; Whitney and Andrews, 2001b). Over a 24 h period there was no displacement of [¹⁴C]carboxyarabinitol-P₂ bound to either purified L^sS^t or tobacco Rubisco when incubated with a 500-fold excess of [¹²C]carboxyarabinitol-P₂, validating its use for quantifying Rubisco content. Indeed, Coomassie staining, immunoblot analyses, and [¹⁴C]carboxyarabinitol-P₂ showed the Rubisco content in fully expanded tobacco^Rst leaves was approximately one-quarter that of the wild-type controls (Fig. 3, A–C ; Table I). To partially compensate for the reduced content, the carbamylation status (i.e. the number of activated sites that have activator CO₂ bound to Lys 201 and coordinated with Mg²⁺) of L^sS^t under the high-CO₂ growth conditions was twice that of wild type (Fig. 3D). However, despite the difference in Rubisco content there was little difference in the leaf activase content (Fig. 3B), indicating an approximately 4-fold increase in the activase:Rubisco stoichiometry in tobacco^Rst leaves. Notably, the approximately 1 g m^–2 reduced Rubisco content within tobacco^Rst leaves did not account for the approximately 3 g m^–2 reduction in leaf protein that was approximately 40% lower than the wild-type controls (Table I).

View larger version (33K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 3. Rubisco activase abundance and Rubisco content and carbamylation status in comparable young, fully expanded leaves from wild-type tobacco (wt, n = 4) and tobaccoRst (tRst, n = 3) plants of similar physiological age (approximately 35 cm in height) grown in air containing 0.5% (v/v) CO2. Soluble protein from 2.7 mm2 of leaves was separated by SDS-PAGE and stained with Coomassie blue (A) or replicate samples (B) blotted and probed with antibodies raised against spinach Rubisco (Rubisco L antibody), tobacco Rubisco activase (tobacco activase antibody), or tobacco Rubisco S subunit (Rubisco S antibody; Whitney and Andrews, 2001a). C, The content of Rubisco active sites and their carbamylation status (D) measured by [14C]carboxyarabinitol-P2 binding/[12C]carboxyarabinitol-P2 exchange under the high-CO2 growth conditions. See "Materials and Methods" for further details.

Light transient CO₂ assimilation measurements, identical to those described by Hammond et al. (1998), were performed using the flow-through LI-6400 gas-exchange system to ascertain whether tobacco Rubisco activase could correctly regulate L^sS^t in tobacco^Rst leaves. Changes in assimilation rates were measured following the sudden transition from low to high light (110 and 1,200 µmol quanta m^–2 s^–1, respectively) at pCO₂ of 250 µbar where assimilation remained Rubisco activity limited under the high light. Both tobacco^Rst and wild-type controls showed the typical biphasic increase in CO₂ assimilation rate (Woodrow and Mott, 1989) where assimilation rate rapidly increased initially due to an upsurge in energy production by the photosynthetic light reactions that concomitantly increases ribulose-P₂ synthesis, stimulating assimilation rates to saturating levels, resulting in the stabilized second phase of assimilation (Fig. 4 ). The gradual rise in assimilation rate to a final steady state (A*_f) is dependant on the ability of Rubisco activase to activate Rubisco active sites that, under the low light, had bound sugar phosphates (primarily ribulose-P₂), rendering them unable to participate in catalysis (Hammond et al., 1998). By plotting the natural log of the difference between the corrected assimilation rate (A*) from A*_f, the apparent rate constants for Rubisco activation (k_a) were calculated from the regression of the linear part of the second phase. The k_a for tobacco^Rst (0.16 ± 0.01 min^–1, n = 3) was less than wild type (0.21 ± 0.02 min^–1, n = 3), indicating a faster rate of activation of L^sS^t by tobacco Rubisco activase (Fig. 4).

View larger version (18K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 4. Measurement of the activation constant for tobacco and tobaccoRst Rubisco. Representative whole leaf gas-exchange measurements of the CO2 assimilation response for physiologically analogous leaves (12 cm leaf width, 35 cm plant height) from a wild-type tobacco (A) and a tobaccoRst (B) before and after leaf irradiance was suddenly increased from 110 to 1,200 µmol quanta m–2 s–1 (time zero). The chamber CO2 concentration and leaf temperature were set at 250 µbar and 25°C, respectively. Bottom panels show the data replotted as the natural logarithm of the final assimilation rate (A*f) minus the adjusted assimilation rate (A*) as described (Woodrow and Mott, 1989). See "Materials and Methods" for further details. The rate constant for Rubisco activation (ka) was calculated from the gradients of the linear second phase fitted to the wild-type (white dashed line) and tobaccoRst (black dashed line) measurements.

Pulse-chase labeling with [³⁵S]-Met was used to compare the turnover of the L^sS^t and native tobacco Rubisco in detached leaf discs. Following separation of the [³⁵S]-labeled leaf soluble proteins by nondenaturing PAGE, Rubisco hexadecamers were identified as the prominent protein by Coomassie staining and autoradiography in both wild type and tobacco^Rst (Fig. 5A ). Band densitometry analysis of the autoradiographs showed that the stability of the L^sS^t hexadecamer was comparable to wild-type Rubisco, indicating the reduced Rubisco content in tobacco^Rst leaves is unlikely to be due to increased turnover of the hybrid enzyme (Fig. 5B).

View larger version (54K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 5. Rubisco turnover in tobacco and tobaccoRst leaves. Multiple leaf discs from the same leaf were infiltrated with 35S-Met and chased with 10 mM unlabeled Met for the times shown and the soluble protein from 18 mm2 of leaf separated by nondenaturing PAGE. A, Hexadecameric Rubisco from wild-type tobacco (L8S8, black arrow) and tobaccoRst (LsSt, white arrow) leaves identified in the gels by Coomassie staining and autoradiography. B, Densitometry measurements of the 35S-labeled Rubiscos during the chase periods (±SD of three separate leaf samples for each time point).

The relative contents of rbcL and Rubisco in physiologically comparable expanding tobacco^Rst and tobacco leaves (the same leaves analyzed by gas exchange) were compared to examine to what extent rbcL^S transcription, its translational processing, or folding assembly of sunflower L with tobacco S impeded production of L^sS^t. The integration of the antibiotic resistance gene cassette (Prrn-aadA-Trps16) within the rbcL 3'-untranslated sequence within the plastome of tobacco^Rst (Fig. 6A ) resulted in the production of a monocistronic rbcL^S transcript and a similarly abundant bicistronic one containing rbcL^S and aadA (Fig. 6B). On a leaf area basis, the total RNA content in the tobacco^Rst expanding fifth leaf from plants during the fast growth phase were approximately 10% to 15% lower than the comparable leaves in wild-type controls. As the RNA blots contained similar amounts of total leaf RNA per lane, the equivalent leaf area sampled to obtain this amount of RNA was larger for the tobacco^Rst samples (Fig. 6B). When standardized on a leaf area basis, the steady-state pool of rbcL mRNA in wild-type leaves was 4-fold higher than the content of both rbcL^S mRNAs (Fig. 6C). This deficit indicated problems with transcription of the rbcL^S genes, problems with the stability of their mRNAs, and/or a difference in the developmental profiling of the rbcL^S transcripts during the ontogeny of tobacco^Rst leaves. Measurement of Rubisco content in these leaves by [¹⁴C]carboxyarabinitol-P₂ binding showed the L^sS^t content was reduced approximately 9-fold compared to wild type, corresponding to a 30% reduction in the relative translational efficiency (RTE; calculated as the amount of Rubisco divided by the relative mRNA abundance on a leaf area basis) of the rbcL^S mRNA relative to that seen in wild type (or 50% reduction if the rbcL^S and rbcL-aadA^S mRNAs are equally translated). This indicated that in addition to reduced steady-state levels of rbcL^S, production of the hybrid enzyme is further compromised by translation and/or assembly of the heterologous Rubscio subunits.

View larger version (50K): [in this window] [in a new window] [as a PowerPoint slide]   Figure 6. Plastome organization, transcript content, and translational efficiency of rbcL in comparable light adapted leaves of physiologically analogous tobacco (wt) and tobaccoRst (tRst) plants (approximately 60 cm in height). A, The tRst transformants have the tobacco rbcL gene replaced with the corresponding gene from sunflower (rbcLS) and contain a p-aadA-t gene cassette (p, 16S rDNA rrn promoter and 5' UTR; t, rps16 3' UTR; Svab and Maliga, 1993) inserted 174-bp downstream of the rbcL stop codon within the rbcL 3' UTR (T). The annealing positions of the 5'rbcL probe and the primers LsE and LsH are shown. The dotted lines and numbering (Shinozaki et al., 1986) refer to positioning of the homologously inserted foreign sequence into the tobacco plastome (GenBank accession no. Z00044). P, rbcL promoter and 5' UTR. B, Blot of total leaf RNA (the amount and relative leaf area used are shown) probed with 5'rbcL, showing the rbcL produced in wt and the mono- (rbcLS) and bi- (rbcLS-aadA) cistronic mRNAs produced in the tRst plants. Equivalent loading was confirmed by comparing the amount of 16SrRNA transcript (data not shown). C, The relative abundance of the rbcL and rbcLS mRNAs measured from B and the corresponding Rubisco content measured by [14C]CABP binding are expressed as a percentage to the average rbcL transcript and Rubisco content in the wt samples. The RTE was obtained by dividing Rubisco content by transcript abundance. For tRst, the RTE in parentheses is calculated from the sum of the abundances of the rbcLS and rbcLS-aadA transcripts.

At ambient pCO₂ (C_i of approximately 350 µbar) the CO₂ assimilation rates in the young fully expanded tobacco^Rst leaves were approximately 3 µmol m^–2 s^–1, indicating photoautotrophic growth should be supported in air. When grown from seed in air the leaf tissue that developed following normal cotyledon development was necrotic, consistent with Kanevski et al. (1999). However, when grown at elevated pCO₂ and then transferred to growth in air once a defined apical meristem had developed and shoot elongation was imminent, growth to fertile mature plants was possible, albeit 4-fold slower than a tobacco^Rst plant maintained in air with 0.5% (v/v) CO₂ (Supplemental Fig. S4). The leaves that developed in air were phenotypically distinct, being paler green, thinner, and consequently, extremely fragile.

Rubisco Content in Juvenile Leaves

The ability of more mature but not juvenile vegetative tobacco^Rst tissue to grow in air led us to investigate whether a paucity of hybrid enzyme or Rubisco activase in the juvenile tobacco^Rst oblanceolate leaves led to their demise in air. The levels of both enzymes in the total and soluble protein of juvenile leaves were examined (Fig. 7 ). Comparative immunoblot and [¹⁴C]carboxyarabinitol-P₂ binding analyses to wild-type controls showed no difference in leaf Rubisco activase levels while the level of hybrid Rubisco produced by tobacco^Rst were approximately 7-fold less than the wild-type controls and appeared entirely soluble (Fig. 7, A and B). On a leaf area basis, the RNA content in the juvenile tobacco^Rst leaves was reduced approximately 30% relative to wild type and the abundance of rbcL^S and rbcL^S-aadA transcripts (present in a ratio of approximately 9:1) reduced 5-fold relative to the levels of rbcL in wild type (Fig. 7C). This resulted in a 30% lower RTE for L^sS^t compared with wild-type Rubisco in the juvenile plants indicating that, analogous to the mature leaves, the paucity of hybrid enzyme appears influenced by limitations in both the steady-state levels of the rbcL^S transcripts, their translational processing, folding, and/or subunit assembly (Fig. 7C). Additional qualitative SDS-PAGE analyses showed even lower sunflower L content in juvenile tobacco^Rst leaves sampled earlier in development, suggesting juvenile tobacco^Rst vegetative tissue produce insufficient levels of the L^sS^t to support adequate levels of CO₂ assimilation for growth in air.

	DISCUSSION

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

 

Tobacco^Rst Can Grow Autotrophically

We have shown using tobacco^Rst and independently generated t^RstLA transplastomic lines that tobacco only expressing a hybrid L^sS^t enzyme comprising sunflower L and tobacco S subunits can be grown autotrophically past cotyledon emergence to fertile maturity in air when supplemented with CO₂ (Fig. 1; Supplemental Fig. S1). Both photosynthetic gas-exchange measurements on mature leaves and kinetic measurements made on extracted L^sS^t showed that the catalytic properties of the hybrid enzyme are comparable to the native sunflower and tobacco Rubiscos (Fig. 2B). However, even when supplied with 0.5% CO₂ (v/v) the tobacco^Rst line and the t^RstLA lines display atypical developmental phenotypes and slower growth.

The Sustained Kinetics of the Hybrid L^sS^t Enzyme Is Unique

Previous mutagenic studies using cyanobacterial and Chlamydomonas Rubiscos have clearly shown the S subunits are required for catalytic competency, have a pervasive influence on the kinetic properties of Rubisco, and that the L subunits are catalytically impaired when assembled with heterologous or structurally altered S subunits (Spreitzer, 2003; Karkehabadi et al., 2005). This is not the case for L^sS^t, invalidating the canonical belief that the assembly of heterologous Rubisco L and S subunits will unfavorably influence catalytic efficiency. Indeed, although only sharing 76% sequence identity we can only assume from the sustained kinetics of L^sS^t that there is sufficient similarity in the quaternary structure of the assembled tobacco S subunits so as to retain the normal active site geometry of the assembled sunflower L subunits. This raises the interesting possibility that there may be greater structural flexibility between heterologous Rubisco S and L peptides from higher plants that enables their assembly with little or no kinetic perturbation to the hybrid enzyme. Addressing this possibility will necessitate comparable tranplastomic studies focused on replacing the tobacco rbcL with other plant rbcL variants.

Our in vitro measurements of V_c^max were made using rapidly isolated protein extracts from leaves from both tissue-culture and autotrophically grown L^sS^t plants using different extraction buffers containing different protease inhibitor additives without appreciable decline in activity after 30 min incubation at 25°C (Supplemental Fig. S3). This use of rapidly isolated leaf protein extract is now commonplace within this laboratory and gives accurate, and reproducible, estimates of V_c^max (Whitney et al., 2001; Ghannoum et al., 2005) and also K_c whose values match those obtained previously using freshly purified Rubisco (Fig. 2B). Possibly the purified L^sS^t used by Kanevski et al. (1999) to measure its kinetics had been compromised by partial proteolysis of terminal residues during the extended purification process. Proteolysis of N- and/or C-terminal residues may explain their lower V_c^max (Fig. 2B) and high K_c (60 µM) measurements for L^sS^t as these kinetic parameters (and to a much lesser extent S_c/o) have also been strongly compromised in R. rubrum, cyanobacteria, and spinach (Spinacia oleracea) Rubiscos upon removal of residues from their L subunit termini by partial proteolysis or mutagenesis (Gutteridge et al., 1986a; Kettleborough et al., 1987; Ranty et al., 1990).

Rubisco Activity Limits Tobacco^Rst Growth

Our results indicate the efficiency of the photosystems was uncompromised in tobacco^Rst at their growth illumination as their chlorophyll content, a/b ratio, and F_v/F_m ratio mirrored that observed for wild type. It is more likely the primary basis for the developmental differences resulted from limitations in L^sS^t production. Development was particularly perturbed during juvenile growth when L^sS^t levels were reduced more than 7-fold, resulting in the production of unique oblanceolate leaf clusters not seen previously in anti-RbcS tobacco lines where Rubisco production was reduced 5-fold (Tsai et al., 1997), suggesting greater limitations to source strength in tobacco^Rst. With maturation, the leaf L^sS^t content improved to levels approximately 20% that of Rubisco in wild-type tobacco, however, the photosynthetic capacity of tobacco^Rst remained Rubisco activity limited despite CO₂ supplementation (Fig. 3). This limitation was substantiated by an approximately 2-fold lower content of nonstructural carbohydrate, an approximately 9-fold higher ribulose-P₂ to P-glycerate ratio, and high nonphotochemical quenching up to a intracellular pCO₂ (C_c) of 2 mbar (Supplemental Fig. S2), and the ineffectual response of CO₂ assimilation rate to illumination above the growth intensity of 350 µmol quanta m^–2 s^–1 for tobacco^Rst (Fig. 2A). Consistent with the differences in their exponential growth rates (Fig. 1D) the predicted Rubisco limited CO₂ assimilation rate at the growth pCO₂ (approximately 5 mbar) in fully expanded tobacco^Rst leaves (containing 5 µmol Rubisco active sites m^–2) modeled according to Farquhar et al. (1980) is 14 µmol CO₂ m^–2 s^–1, which is approximately two-thirds that of the light limited assimilation rate in wild-type tobacco (23 µmol CO₂ m^–2 s^–1; Fig. 2A). Also consistent with leaf gas-exchange measurements was the capacity for tobacco^Rst to grow without CO₂ enrichment, albeit only once source strength and leaf L^sS^t content were adequate. This necessitated the development of normal ovate leaves before growth through to reproductive maturity could be supported in air, albeit approximately 4-fold slower than if maintained at high pCO₂ (Supplemental Fig. S4).

What Is Limiting the Content of L^sS^t in Tobacco^Rst Leaves?

While the comparable stability of the tobacco^Rst and wild-type tobacco Rubiscos indicated little or no perturbations to turnover of the assembled L^sS^t hexadecamer (Fig. 4), reductions in the relative RNA content per leaf area and in the steady-state pool of the sunflower rbcL^S and rbcL^S-aadA mRNAs contributed to the paucity of L^sS^t produced. Compared with the rbcL pool in tobacco, the abundance of both the rbcL^S and dicistronic rbcL^S-aadA transcripts in juvenile and mature tobacco^Rst leaves were approximately 5- and 4-fold lower, respectively. The stability of chloroplast transcripts are strongly influenced by appropriate endo- and exonucleolytic maturation of the 5'- and 3'-untranslated regions (UTRs; Bollenbach et al., 2004). The sequence of these regions, and that of the juxtaposed coding sequence, strongly influence appropriate mRNA folding and interaction with nucleus encoded chloroplast RNA-binding complexes that maintain the integrity of the transcript by correctly processing the 5' and 3' ends to prevent degradation by nucleases (Monde et al., 2000; Bollenbach et al., 2004; Zicker et al., 2007). As rbcL^S expression in tobacco^Rst is controlled by the same promoter and 5' UTR as tobacco rbcL it is likely changes to the 3' UTR and rbcL^S coding sequences perturbed proper maturation and stabilization of the transcripts making them more susceptible to degradation by plastid ribonucleases. The importance of the tobacco rbcL 3' UTR for maintaining steady-state levels of rbcL mRNA has been shown previously (Whitney and Andrews, 2003). In tobacco^Rst the aadA cassette is inserted at the equivalent position 178-bp downstream of the rbcL stop codon after nucleotide 59251 in the tobacco plastome (GenBank accession no. Z00044). Intriguingly in subsequent RNA blots using fully denaturing formaldehyde gels we find the rbcL^S mRNA is smaller than the native rbcL mRNA, indicating the mature 3' UTR of rbcL extends further downstream (data not shown). In support of this, insertion of a promoterless aadA gene a further 91-bp 3' to that in tobacco^Rst does not perturb rbcL abundance or Rubisco production and still enables transcription of an additional, less abundant (approximately 20% of the rbcL mRNA) rbcL-aadA transcript (Whitney et al., 1999; Whitney and Andrews, 2003). Clearly, the 3' UTR does have a pervasive influence on the steady-state levels of chloroplast mRNAs and to what extent lengthening the 3' UTR would improve rbcL^S transcript abundance, and reduce transcriptional read through of the rbcL^S-aadA message, remains to be examined.

Problems with translation and/or assembly also contributed to the paucity of L^sS^t produced in the tobacco^Rst leaves. Frequently in plastome transformation studies the equipping of foreign gene sequences with nonnative UTR sequences can perturb mRNA folding and slow translational processing of transgenes (Maliga, 2002). This necessitates the trialing of different UTR combinations to optimize expression (Maliga, 2003). The RTE of both rbcL^S mRNAs in both the juvenile and mature tobacco^Rst leaves was reduced 30% to 50%. One possible reason for this difference is the levels of rbcL and Rubisco holoenzyme during leaf ontogeny may differ between tobacco^Rst and wild type. That is, despite sampling expanding leaves from a comparable position in the canopy from wild type and tobacco^Rst of similar heights, their apparent developmental differences (Fig. 1) might extend to variations in the patterns of rbcL and Rubisco contents during leaf development that are otherwise generally correlated in tobacco (Miller et al., 2000) but not in all plants (see Suzuki et al., 2001 and refs. therein). Clearly this needs to be examined more comprehensively in the future by profiling the variation in plastome copy number, rbcL, RbcS, and Rubisco contents, and the rates of subunit translation (using rapid ³⁵S-Met pulse methods; Rodermel et al., 1996) in both tobacco and tobacco^Rst leaves during their development.

The reduced RTE of rbcL^S mRNAs in tobacco^Rst might otherwise arise from problems related to translational processing of the transcripts due to the introduced NheI cloning site in codons 9 and 10. This introduces changes to nucleotides 27 and 30 in rbcL^S that otherwise shows absolute homology to tobacco rbcL for the first 56 nucleotides (GenBank accession no. AF097517). Unfortunately these nucleotide changes may potentially hamper translational processing of rbcL^S since the translational control region of rbcL includes both the 5' UTR and N-terminal coding sequence (approximately 42 nucleotides; Kuroda and Maliga, 2001). By examining the sedimentation behavior of the polysomes associated with the rbcL^S mRNA it should be possible to identify whether translation initiation or translation elongation is impeded (Kim and Mullet, 1994). Alternatively, truncation of the mRNA 3' UTR may affect interactions between the 5' UTR and 3' UTR that are required for efficient recycling of mRNAs during translation (Kawaguchi and Bailey-Serres, 2002).

The lower RTE of the rbcL^S transcripts in mature tobacco^Rst leaves may also stem from limitations on the functional assembly of the L^sS^t hexadecamer. This limitation may arise from incompatibilities between tobacco chloroplast chaperone complexes and the folding and assembly requirements of sunflower L, or be indicative of reduced chaperone availability in response to elevated metabolic stress. Indeed chaperone incompatibility problems preclude assembly of functional form I Rubiscos from nongreen algae in tobacco chloroplasts (Whitney et al., 2001). However, unlike nongreen algal Rubisco subunits, no misfolded, unassembled sunflower L were detected, possibly due to their rapid removal along with the unassembled tobacco S by chloroplast proteases. Improvements in foreign Rubisco assembly might therefore be attained by cotransplanting in appropriate chaperones with their cognate Rubisco L subunits. In favor of this, the production of correctly folded cuboid crystals of the insecticidal Bacillus thuringiensis Cry protein in tobacco plastids required cotransplanting of a complementary chaperone (De Cosa et al., 2001). Despite the complexity of Rubisco assembly in chloroplasts, candidate chaperones that specifically interact with Rubisco L subunits have been identified and may provide useful starting points. These chaperones include the BSDII chaperone protein that shares homology with DnaJ chaperones (Brutnell et al., 1999) and RbcX-like homologs that play an important role in promoting assembly of cyanobacterial L₈ cores in E. coli by forming dynamic intermediate complexes with L subunits after having undergone folding by the chaperonins (Saschenbrecker et al., 2007).

The Hybrid Rubisco Is Adequately Regulated by Tobacco Rubisco Activase

The compatibility problems that can potentially limit the regulatory capacity of a Rubisco activase to Rubiscos from related species (Wang et al., 1992) did not affect the capacity of tobacco activase to adequately regulate L^sS^t. This was initially evident from the approximately 2-fold higher carbamylation status of the hybrid Rubisco. As seen in transplastomic tobacco lines producing 50% less Rubisco (Whitney and Andrews, 2003) or a kinetically inferior mutant (Whitney et al., 1999), the high carbamylation status presumably compensates for the lower carboxylation potential. Light transient gas-exchange analyses also showed the activation constant for L^sS^t was 25% faster than wild-type tobacco Rubisco, indicating the hybrid enzyme was adequately regulated by tobacco Rubisco activase (Fig. 4). Possibly this faster activation occurred as a consequence of the 4- to 7-fold (depending on leaf age) higher stoichiometry of activase to Rubisco in the tobacco^Rst leaves that resulted from a concomitant reduction in L^sS^t levels but no discernable change in activase production. This higher stoichiometry might also conceal regulatory incompatibilities between L^sS^t and tobacco Rubisco activase that will need to be resolved using appropriate in vitro enzyme assays (Wang et al., 1992), particularly if efforts are undertaken to increase production of L^sS^t in tobacco chloroplasts.

Reasons for the Abnormal Tobacco^Rst Leaf Phenotype Are Unclear

As the developmental phenotype of tobacco^Rst leaves has been maintained over three generations after backcrossing with wild-type pollen and is repeated in the independently generated tob^RstLA7 and tob^RstLA13 transplastomic lines (Supplemental Fig. S1), the phenotype is not caused by pleiotropic effects and results from the replacement of tobacco L with the sunflower L. More comprehensive developmental studies on tobacco^Rst and the tob^RstLA lines are needed to uncover the underlying cause(s) of its aberrant phenotypic features. While sharing developmental similarities to anti-RbcS and other Calvin cycle antisense mutants with reduced carbon assimilation capacity (Tsai et al., 1997; Raines and Paul, 2006), the unique production of leaf clusters and multiple shoots early in tobacco^Rst development and the marginal dimpling of mature leaves indicate their development process is more severely perturbed. Interestingly, juvenile tobacco-rubrum plants do not show this phenotype when grown in air containing 1% or 2.5% CO₂ (v/v), suggesting their rates of carbon assimilation are sufficiently nonlimiting at these high pCO₂. However, at 1% CO₂ some tobacco-rubrum leaves display slight marginal dimpling early in development that disappears as the leaves age and accumulate more Rubisco (data not shown). Whether the developmental anomalies of tobacco^Rst can be circumvented by growth under non-Rubisco limiting conditions (i.e. higher pCO₂, lower light) have yet to be examined. Nevertheless, it is important to note that when grown in tissue culture on media containing Suc, tobacco^Rst only produces normal leaves consistent with limitations in carbon assimilation being the primary cause of the developmental differences during autotrophic growth.

Possibly the developmental differences of tobacco^Rst arise from greater limitations in carbohydrate production than in other anti-Calvin cycle mutants, particularly in the juvenile tissue where survival past cotyledon emergence necessitates CO₂ supplementation. Very low Rubisco levels would impose significant limitations on the acquisition of sufficient source strength, explaining the lengthy duration of the juvenile phase in tobacco^Rst (30–40 d) and phenotypic abnormalities that possibly arise from alterations in the developmental program of the shoot apical meristems in response to developmental delay. As shoot apical meristems regulate the development of lateral organs such as leaves and branches (Piazza et al., 2005), it is possible some (or all) of the multiple apical shoots produced by tobacco^Rst may really be lateral branches. Clearly a more thorough growth comparison of tobacco^Rst with anti-RbcS tobacco (‘Petit Havana’) with comparable Rubisco reductions (particularly in juvenile leaves) is needed to identify differences in their development, carbon-nitrogen status, and metabolite profiles (Fritz et al., 2006) and improve our understanding of the regulatory signals derived from changes in leaf metabolism that influence a plant's developmental program (Raines and Paul, 2006).

Future Considerations for Rubisco Engineering in Tobacco Chloroplasts

While many unresolved problems associated with transplanting foreign Rubiscos into higher plant plastids remain to be addressed, our discovery that L^sS^t is not catalytically impaired should motivate further plastomic replacement studies with foreign Rubisco L subunits, particularly those from other higher plants. As highlighted in this study, success will necessitate the introduced rbcL to be stably transcribed, efficiently translated, and the folding and assembly requirements of the L be sufficiently compatible with the tobacco chaperone complexes and the tobacco S and suitably regulated with the endogenous Rubisco activase. Only needing to engineer rbcL would be advantageous as it would negate the need for cotransplanting in the complementary RbcS and evade further obstacles with needing to silence the endogenous S or genetically manipulate it as this is complicated by the multiple RbcS copies in the nuclear genome (Andrews and Whitney, 2003). Candidate rbcL genes for testing would include those of the kinetically superior Rubiscos from C₃ plants growing in hot arid conditions (Galmes et al., 2005), such as Limonium gibertii (Parry et al., 2007) whose L shows 92% identity to tobacco L. A wider examination might also include rbcL genes from C₄ Rubiscos that characteristically have higher k_c^cat values relative to C₃ species, albeit at the expense of higher K_c values (Yeoh et al., 1981; Seemann et al., 1984).

	MATERIALS AND METHODS

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

 

Materials

Substrate ribulose-P₂ (both 1 ³H labeled and unlabeled) was synthesized according to Kane et al. (1998). Unlabelled ([¹²C]) and carboxyl-¹⁴C-labeled ([¹⁴C]) carboxypentitol-P₂ (an isomeric mixture of carboxyarabinitol-P₂ and carboxyribitol-P₂) were synthesized as described in Pierce et al. (1980). The carboxyarabinitol-P₂, that binds stoichiometrically to CO₂-Mg²⁺ activated Rubisco active sites almost irreversibly (Schloss, 1988) was purified from these preparations by ion exchange (Zhu and Jensen, 1991).

Plant Growth

Tobacco (Nicotiana tabacum L. ‘Petit Havana’ [N,N]) and transplastomic tobacco^Rst (line Nt-pIK 83-1; Kanevski et al., 1999; T₀ seed obtained from Pal Maliga) were germinated and grown in soil in a controlled environment cabinet with a 14 h light (25°C) and 10 h dark (20°C) photoperiod in air supplemented with 0.5% (v/v) CO₂ during the light period where the artificial illumination was 350 µmol quanta m^–2 s^–1 and the humidity set at 65%. Each generation of tobacco^Rst was artificially pollinated with wild-type pollen and the T₂ seed used for all analyses. The plants were grown in 5-L pots of soil and provided with Hoagland nutrient mix (Hoagland and Snyder, 1933) every 2 d. The height of the plants was measured every 2 to 3 d from the soil surface to the apical meristem of the primary axial shoot until the emergence of the first floral apertures.

Leaf Gas Exchange

Whole leaf photosynthetic gas exchange was measured using the portable, flow-through LI-6400 gas-exchange system (Li-COR). Tobacco^Rst and wild-type tobacco controls (approximately 30–35 cm tall) were brought from the high-CO₂ growth cabinet to the laboratory for gas-exchange analysis and measurements made on the still expanding fifth leaf whose width was typically approximately 85% that of the largest seventh leaf. CO₂ assimilation rates were measured using the 2 x 3 cm chamber fitted with a red/blue (10%) LED light source (Li-COR 6400-02B) with the leaf temperature set at 25°C. Transient light assays were performed similar to those described by Hammond et al. (1998). The plants were brought from the growth chamber early in the light period into the laboratory to ensure that the nocturnal inhibitor of tobacco Rubisco, 2-carboxyarabinitol-1-P (Gutteridge et al., 1986b) was absent from the Rubisco active sites. The plants were maintained under dim light (<60 µmol quanta m^–2 s^–1) before gently clamping into the LI-6400 system and equilibrating the leaf at 110 µmol quanta m^–2 s^–1 and approximately 200 µbar CO₂ (to encourage stomata opening and ensure the conductance was >0.15 µmol m^–2 s^–1) for 45 min. The CO₂ concentration was then raised to 250 µbar (where CO₂ assimilation is still Rubisco activity limited) for 20 min before suddenly increasing the irradiance to 1,200 µmol quanta m^–2 s^–1. The flow rate of air into the chamber was set at 500 µmol s^–1. At this flow rate, it takes 7 s for 63% of the air in the LiCOR chamber (83 cm³) to be refreshed. Assimilation measurements were continued until a final steady-state rate was reached (A_f). Photosynthetic CO₂ assimilation rates were normalized to a constant C_i by assuming linear relationship between the CO₂ compensation point () and each assimilation rate measurement (A; Brooks and Farquhar, 1985; Woodrow and Mott, 1989). Calculation of was achieved by measuring assimilation rates, in replicate, at intercellular pCO₂ (C_i) of approximately 50, 100, 150, and 250 µbar at an illumination of 350 µmol quanta m^–2 s^–1 (the growth irradiance). Using a linear fit, was calculated for tobacco^Rst (97 ± 6.6 µbar) and wild type (49 ± 3.0 µbar) as the C_i where A was zero. A corrected assimilation rate (A*) was calculated for each 10 s time point using the equation:

where C_i* represents a C_i value (170 µbar) chosen to normalize the varying C_i against.

Leaf Sampling, Metabolite, and Biochemical Measurements

Biochemical measurements were made on leaf samples taken 8 h into the 14 h photoperiod from either developing juvenile leaf tissue or from young expanding mature leaves at comparable positions in the canopy (typically the fifth leaf below the apical meristem) from plants during the fast growth phase that were either approximately 35 or 60 cm tall. For the mature leaves, samples were taken from the same leaf and frozen immediately in liquid nitrogen and stored at –80°C or dried at 80°C for elemental nitrogen and carbon content analysis as described in Whitney et al. (2001b). Stored leaf samples were used to measure Rubisco content and carbamylation status using the [¹⁴C]carboxyarabinitol-P₂ binding/[¹²C]carboxyarabinitol-P₂ exchange procedure (Ruuska et al., 1998; Whitney and Andrews, 2001b) and the content of nonstructural starch, chlorophyll, soluble protein, ribulose-P₂, and P-glycerate measured according to Whitney and Andrews (2003).

The substrate saturated turnover rate (V_c^max) and K_m for CO₂ at ambient pO₂ (K_c^21%O₂) for Rubisco were measured using the soluble protein rapidly extracted on ice from 1 cm² leaf discs using glass homogenizors (Wheaton) into 0.8 mL CO₂-free extraction buffer (50 mM Hepps-NaOH, pH 8.0, 1 mM EDTA, 2 mM dithiothreitol, 1% [v/v] plant protease inhibitor cocktail [Sigma-Aldrich], and 1% [w/v] polyvinylpolypyrrolidone). A sample of lysate was taken for SDS-PAGE analysis as described (Whitney et al., 2001) and the remainder centrifuged (14,000g, 1 min, 4°C) and samples of the soluble protein taken for SDS-PAGE or incubated (activated) with NaHCO₃ and MgCl₂ (15 mM each) for 10 min and used to: measure Rubisco content in duplicate aliquots incubated with 10 or 30 µM of [¹⁴C]CABP and the amount of Rubisco-bound [¹⁴C]CABP recovered by gel filtration (Ruuska et al., 1998; Whitney and Andrews, 2001b), or used to measure K_c^21%O₂ at 25°C, pH 8.0 using ¹⁴CO₂ fixation assays as described in Whitney and Sharwood (2007). The K_c assays were initiated by adding the activated soluble protein extract into septum capped scintillation vials containing CO₂-free air equilibrated assay buffer (100 mM Hepps-NaOH, 15 mM MgCl₂, 0.6 mM ribulose-P₂, 0.1 mg mL^–1 carbonic anhydrase) containing 0 to 44 µM ¹⁴CO₂. The assays were stopped after 1 min with 0.5 volumes of 25% (v/v) formic acid and processed for scintillation counting (Whitney and Sharwood, 2007). Measurements of V_c^max were calculated using comparable ¹⁴CO₂ fixation assays containing 15 mM NaH¹⁴CO₃ and dividing the rate by the concentration of Rubisco active sites measured by [¹⁴C]carboxyarabinitol-P₂ binding (see above).

Rubisco Purification and CO₂/O₂ Specificity

Rubisco was rapidly purified from approximately 50 g of freshly harvested leaves of tobacco, tobacco^Rst, and sunflower (Helanthus annuus) plants grown at high CO₂. The leaves were homogenized in 40 mL ice cold extraction buffer, filtered through five layers of miracloth, centrifuged (30,000g, 10 min, 2°C), and the soluble protein chromatographed on a 5 mL Q-sepharose column equilibrated with column buffer (50 mM Hepps-NaOH, pH 8.0, 1 mM EDTA). Proteins were eluted over a 0 to 400 mM NaCl gradient over 150 mL (5 mL min^–1 flow rate) and the two fractions (5 mL) containing peak Rubisco activities (measured by ribulose-P₂-dependent ¹⁴CO₂ fixation) were pooled and dialyzed for 16 h at 4°C against 1 L of storage buffer (25 mM Hepps-NaOH, pH 8.0, 1 mM EDTA, 20% [v/v] glycerol). This concentrated the samples approximately 3-fold before they were frozen in liquid nitrogen and stored at –70°C. The purified Rubisco preparations were used to measure their CO₂/O₂ specificity (S_c/o) using the method of Kane et al. (1994).

SDS-PAGE and Immunoblots

Leaf protein samples were separated by SDS-PAGE (Bis-Tris-buffered 4%–12% NuPAGE gels, Invitrogen), blotted onto nitrocellulose, probed with appropriate antibodies, and the immunoreactive bands visualized using AttoPhos (Promega) as described previously (Whitney and Andrews, 2001a).

³⁵S-Pulse Chase Labeling

Pulse chase labeling of leaf proteins was performed at 25°C using a modified protocol described by Whitney and Andrews (2001a). Thirty leaf discs (1 cm²) were collected in the growth chamber from young fully expanded leaves and transferred to the laboratory in covered dishes onto prewetted Whatman paper. Within 5 min the discs were layered abaxial side down onto pulse solution (Murashige and Skoog nutrient solution [pH 7.2]; Murashige and Skoog, 1962) containing 10 mM NaHCO₃, 0.25% (v/v) silwet, and 2% (v/v) [³⁵S]Met (10.5 mCi/mL; ICN Biomedicals) and vacuum infiltrated at 200 mbar for 4 min before slowly releasing the vacuum. After 20 min illumination (600 µmol quanta m^–2 s^–1) the discs were quickly rinsed with three 100 mL washes of chase solution (pulse solution containing 10 mM Met) with intermittent blotting on Whatman paper to remove excess solution. Three leaf discs were snap frozen in liquid nitrogen (0 h chase samples) and the remainder layered onto 50 mL chase solution, vacuum infiltrated, and illuminated a further 0.5, 1, or 2 h before freezing in liquid nitrogen. The frozen discs were extracted in 0.5 mL extraction buffer on ice in Wheaton glass homogenizors then centrifuged (35,000g, 10 min, 4°C) and the supernatant diluted 9:1 with native load buffer (60% [v/v] glycerol, 1% [w/v] bromphenol blue) and the proteins loaded onto Tris-Glycine buffered 4% to 20% NuPAGE gels and separated at 60 V for 18 h at 4°C in nondenaturing running buffer (19.2 mM Gly, 2.4 mM Tris, pH 8.3). The separated proteins were fixed in the gels and stained with Gel Code Blue Coomassie stain (Pierce) according to manufacturer instructions before vacuum drying the gels and exposing them to a storage phosphor screen for 21 d. The radioactive signals were detected using a Molecular Dynamics 400-B 2D PhosphorImager and the banding quantified by densitometry analysis using ImageQuant software.

Leaf DNA, RNA, and PCR Analyses

Total leaf DNA and RNA was extracted, separated by agarose gel electrophoresis, and blotted onto membranes as described previously (Whitney et al., 1999, 2001). The membranes were prehybridized at 55°C for at least 1 h in hybridization buffer supplied in the AlkPhos Direct Labeling kit (Promega) before hybridizing with DNA probes labeled with -[³²P]dATP using the MegaPrime Labeling kit (GE Biosciences). For RNA blots the 575-bp tobacco 5'rbcL probe (Fig. 6A), which spans the tobacco rbcL promoter, 5' UTR, and the first 42 nucleotides of the tobacco rbcL gene, was amplified from tobacco DNA using the primers LsH (5'-CTATGGAATTCGAACCTGAACTT-3') and NdeHis-15 (5'-CCATATGTTTGAATCCAACACTTGCTTTA-3'). The DNA blots were hybridized with the 1,856-bp DNA rbcL probe as described (Whitney and Andrews, 2001b; Supplemental Fig. S1). The autoradiograph signals were detected on storage phosphor screens as described above.

Total leaf DNA from tobacco^Rst transplastomic plants was used as template for PCR amplification using primers LsE (Whitney and Andrews, 2001b) and LsH (Fig. 6A). The 2.6 kb amplified product was cloned into pGEM-T Easy (Promega) and fully sequenced using BigDye terminator sequencing (Applied Biosystems) on an ABI 3730 sequencer (Biomolecular Resource Facility, John Curtin School of Medical Research, Australian National University).

Supplemental Data

The following materials are available in the online version of this article.

Supplemental Figure S1. The genotype and phenotype of new t^RstLA (tobacco^Rst-Lox-aadA) transplastomic lines.

Supplemental Figure S2. Measurement of electron transport rate, nonphotochemical quenching (NPQ), and CO₂ assimilation rate in response to change in intercellular pCO₂ using simultaneous leaf chlorophyll fluorescence and CO₂ assimilation measurements.

Supplemental Figure S3. Change in maximal ribulose-P₂-dependent carboxylase activity (V_c^max) in leaf protein extracts from tissue-cultured plants in response to CO₂-Mg²⁺ activation during incubation at 25°C.

Supplemental Figure S4. Growth of tobacco^Rst in air.

	ACKNOWLEDGMENTS

 
We thank Archie Portis for his helpful comments on the manuscript and John Andrews for his contribution to the research.

Received September 13, 2007; accepted November 1, 2007; published November 9, 2007.

	FOOTNOTES

 
¹ This work was supported by a Discovery grant (no. DP0450564) awarded to S.M.W. by the Australian Research Council. Research in P.M.'s laboratory was supported by the National Science Foundation (grant no. MCB 93–05037).

The author responsible for distribution of materials integral to the findings presented in this article in accordance with the policy described in the Instructions for Authors (www.plantphysiol.org) is: Spencer Michael Whitney (spencer.whitney{at}anu.edu.au).

^[W] The online version of this article contains Web-only data.

^[OA] Open Access articles can be viewed online without a subscription.

www.plantphysiol.org/cgi/doi/10.1104/pp.107.109058

^* Corresponding author; e-mail spencer.whitney{at}anu.edu.au.

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				S. M. Whitney, H. J. Kane, R. L. Houtz, and R. E. Sharwood Rubisco Oligomers Composed of Linked Small and Large Subunits Assemble in Tobacco Plastids and Have Higher Affinities for CO2 and O2 Plant Physiology, April 1, 2009; 149(4): 1887 - 1895. [Abstract] [Full Text] [PDF]

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