Increased Calcium Levels and Prolonged Shelf Life in Tomatoes Expressing Arabidopsis H+/Ca2+ Transporters

doi:10.1104/pp.105.066266

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Increased Calcium Levels and Prolonged Shelf Life in Tomatoes Expressing Arabidopsis H⁺/Ca²⁺ Transporters¹

Sunghun Park^*, Ning Hui Cheng, Jon K. Pittman², Kil Sun Yoo, Jungeun Park, Roberta H. Smith and Kendal D. Hirschi

Vegetable and Fruit Improvement Center, Texas A&M University, College Station, Texas 77845 (S.P., K.S.Y., J.P., R.H.S., K.D.H.); and Plant Physiology Group, United States Department of Agriculture/Agricultural Research Service, Children's Nutrition Research Center, Baylor College of Medicine, Houston, Texas 77030 (N.H.C., J.K.P., K.D.H.)

ABSTRACT

TOP
ABSTRACT
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

Here we demonstrate that fruit from tomato (Lycopersicon esculentum)plants expressing Arabidopsis (Arabidopsis thaliana) H⁺/cationexchangers (CAX) have more calcium (Ca²⁺) and prolonged shelflife when compared to controls. Previously, using the prototypicalCAX1, it has been demonstrated that, in yeast (Saccharomycescerevisiae) cells, CAX transporters are activated when the N-terminalautoinhibitory region is deleted, to give an N-terminally truncatedCAX (sCAX), or altered through specific manipulations. To continueto understand the diversity of CAX function, we used yeast assaysto characterize the putative transport properties of CAX4 andN-terminal variants of CAX4. CAX4 variants can suppress theCa²⁺ hypersensitive yeast phenotypes and also appear to be morespecific Ca²⁺ transporters than sCAX1. We then compared thephenotypes of sCAX1- and CAX4-expressing tomato lines. The sCAX1-expressingtomato lines demonstrate increased vacuolar H⁺/Ca²⁺ transport,when measured in root tissue, elevated fruit Ca²⁺ level, andprolonged shelf life but have severe alterations in plant developmentand morphology, including increased incidence of blossom-endrot. The CAX4-expressing plants demonstrate more modest increasesin Ca²⁺ levels and shelf life but no deleterious effects onplant growth. These findings suggest that CAX expression mayfortify plants with Ca²⁺ and may serve as an alternative tothe application of CaCl₂ used to extend the shelf life of numerousagriculturally important commodities. However, judicious regulationof CAX transport is required to assure optimal plant growth.

Calcium (Ca²⁺) plays a fundamental role in plant membrane stability,cell wall stabilization, and cell integrity (Hirschi, 2004

).Reduced Ca²⁺ in edible plant tissues negatively impacts totalyield. Plant tissues low in Ca²⁺ are more susceptible than tissueswith normal Ca²⁺ levels to some parasitic diseases during storage(Marschner, 1995

). This is of particular concern in the caseof fleshy fruits with their typically low Ca²⁺ levels. Applicationof Ca²⁺ to soils seems to be of questionable value (Lester andGrusak, 1999

; Lopez-Lefebre et al., 2001

); however, supplementalCa²⁺ applied immediately before or just after harvest has beenshown to maintain cell turgor, plasma membrane integrity, andfruit firmness and extend storage life (Gerasopoulos et al.,1996

; Miklus and Beelman, 1996

). In these treatments, applicationof Ca²⁺ increases total Ca²⁺ levels in the fruits by 20% to40%; however, these procedures are labor intensive and oftenresult in tissue damage and fungal infections.

The problems associated with low plant Ca²⁺ levels can be attributedto soil problems. For example, Ca²⁺ deficiencies are favoredby very low soil pH and on soils high in magnesium and potassium.Probably the most recognizable Ca²⁺deficiency is blossom-endrot (BER) of tomato (Lycopersicon esculentum) fruits, whichis induced by water stress (Bennett, 1993; Ho and White, 2005).At the time of fruit set, cells at the blossom end of fruitsare injured. This is caused by insufficient Ca²⁺ translocationresulting in a dry-rot area on the expanding fruit.

One molecular-genetic approach to alter the Ca²⁺ levels in plantsis to engineer high expression of Ca²⁺ transporters and Ca²⁺-bindingproteins (Wyatt et al., 2002; Hirschi, 2004). Increased expressionof a modified vacuolar Ca²⁺ antiporter, cation exchanger 1 (CAX1),in plants causes dramatic increases in Ca²⁺ when compared tovector control plants (Hirschi, 1999; Park et al., 2004, 2005).In a similar fashion, expression in tobacco (Nicotiana tabacum)of a wheat (Triticum aestivum) cation transporter LCT1 increasesshoot Ca²⁺ levels (Antosiewicz and Hennig, 2004). Recent findingssuggest that the corresponding changes in plant growth and developmentdepend on the levels of transporter activity and the particularplant being modified.

The CAX1 cDNA that has been expressed in various plants wasoriginally cloned through a yeast (Saccharomyces cerevisiae)suppression screen (Hirschi et al., 1996). We have identifieda full-length CAX1 cDNA (previously termed long-CAX1) that isidentical to the original clone except that it encodes a proteinwith an additional 36 amino acids at the N terminus (Pittmanand Hirschi, 2001). This CAX1 cannot transport Ca²⁺ in a yeastbiochemical assay, and we have shown that the N terminus functionsas a regulatory region (Pittman et al., 2002). The originalCAX1 is a partial-length cDNA that is deregulated for H⁺/Ca²⁺antiport and is now termed N-terminally truncated CAX 1 (sCAX1).It is this activated form of CAX1 that when expressed in tobacco,carrots (Daucus carota), and potatoes (Solanum tuberosum) resultsin increased Ca²⁺ accumulation (Hirschi, 1999; Park et al.,2004, 2005). Recent work in yeast suggests that full-lengthCAX transporters may have some weak H⁺/Ca²⁺ transport capabilities(Cheng et al., 2005). In addition, various domains within theCAX transporters have been identified that confer substratespecificity. For example, the Ca²⁺ domain of CAX1 appears tobe necessary for Ca²⁺ transport (Shigaki et al., 2001). An unexaminedmeans of marginally increasing activity of H⁺/Ca²⁺ antiportersmay be to express the entire CAX open reading frame or mutantCAX variants in plants.

Arabidopsis (Arabidopsis thaliana) appears to have up to 12putative CAX transporters (Mäser et al., 2001). Like sCAX1,sCAX2 and sCAX4 can function in yeast as H⁺/Ca²⁺ exchangers(Hirschi et al., 1996; Cheng et al., 2002; Pittman et al., 2004b).Our preliminary biochemical analysis of sCAX1 and sCAX2 suggeststransport of various metals (Mäser et al., 2001; Shigakiet al., 2003; Pittman et al., 2004b). However, the specifictransport properties of numerous CAX transporters, includingCAX4, have not been previously examined. Hence, efforts to specificallyalter the Ca²⁺ levels in plants may be more efficient utilizingregulated expression of CAX transporters other than sCAX1.

Our primary focus here was to evaluate the potential for increasingthe Ca²⁺ levels of tomatoes through expression of ArabidopsisH⁺/Ca²⁺ transporters and its potential impact on plant growthand development. Herein, utilizing yeast assays, we have characterizedthe transport properties of variants of CAX4. We also compareand contrast the effect of sCAX1 and CAX4 expression in tomatoas a method to determine if utilizing full-length CAX expressionmay be a means to reduce deleterious phenotypes. This studysuggests that modulation of Ca²⁺ transporters could make animportant contribution toward increasing the value of variousagriculturally important crops.

RESULTS

TOP
ABSTRACT
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

Transport Activity and Cation Selectivity Comparisons of CAX4 Variants

When expressed in yeast, the N-terminal region of CAX transportersacts as an autoinhibitory domain for H⁺/Ca²⁺ transport activity(Pittman et al., 2002, 2004b). To further examine the propertiesof CAX4 transporters with (CAX) and without (sCAX) the putativeN-terminal autoinhibitory domain, we expressed these plasmidsin a yeast strain deficient in vacuolar Ca²⁺ transporters andlacking functional calcineurin (Cunningham and Fink, 1996; Hirschiet al., 1996). This strain (K667) lacks the endogenous vacuolarCa²⁺-ATPase PMC1 and vacuolar H⁺/Ca²⁺ antiporter VCX1 and thusis defective in vacuolar Ca²⁺ transport, making it unable togrow on high Ca²⁺ media (Cunningham and Fink, 1996). We examinedthe growth of yeast cells expressing empty vector control, sCAX1,and full-length CAX1 and CAX4 in media containing 50 mM CaCl₂.Under these semipermissive conditions, the vector control andCAX4-expressing strains grew poorly; however, the full-lengthCAX1 and truncated sCAX1-expressing cells suppressed the Ca²⁺sensitivity, although the suppression by CAX1 was weaker thansCAX1 (data not shown). We then tested those constructs andCAX4 variants (Cheng et al., 2002) on higher Ca²⁺-containingmedia (100 mM CaCl₂). One chimeric CAX4 construct has a 37-aminoacid N-terminal truncation and contains the 9-amino acid CAX1Ca²⁺ domain (Shigaki et al., 2001; sCAX4-9), while the otherform contains a triple copy of the epitope tag hemagglutinin(HA) fused to the N terminus of full-length CAX4 (HA-CAX4).As shown in Figure 1A, CAX4 variant-expressing cells can stronglysuppress the Ca²⁺ sensitivity in a similar manner to sCAX1.

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Figure 1. Substrate characteristics of CAX4 variants expressed in yeast. A, Suppression of Ca²⁺ sensitivity of the pmc1 cnb vcx1 yeast mutant (K667) by CAX1, sCAX1, CAX4, sCAX4, sCAX4-9, and HA-CAX4. Saturated liquid cultures of K667 containing various plasmids were diluted to the cell densities, as indicated, and then spotted onto selection medium (–His) and yeast-extract peptone dextrose (YPD) medium containing 100 mM CaCl₂. B, Inhibition of Ca²⁺ uptake by sCAX1, HA-CAX4, and sCAX4-9 into yeast vacuolar membrane vesicles in the presence of other metals. ${Delta}$ pH-dependent uptake of 10 µM ⁴⁵Ca²⁺, estimated as the difference between uptake with and without 5 µM FCCP, was measured in the absence (control) or presence of 10 x (100 µM) or 100 x (1 mM) of nonradioactive CaCl₂, MnCl₂, CdCl₂, ZnCl₂, NiCl₂, NaCl, or KCl after 10 min. Ca²⁺ uptake values are shown following subtraction of the FCCP background values and expressed as percentages of the control in the absence of any excess nonradiolabeled metals. The data represent means of two to four replications from two to three independent membrane preparations, and the bars indicate SE. An asterisk indicates significant difference from the control (P $≥$ 0.001).

The Ca²⁺ transport activities of CAX4 and sCAX4 are too weakand cannot give measurable ⁴⁵Ca²⁺ transport in yeast (Chenget al., 2002

; data not shown), so to further infer the transportproperties of CAX4, competition transport experiments were performedusing the deregulated CAX4 variants HA-CAX4 and sCAX4-9. Thisallowed us to compare cation selectivity between sCAX1 and theseCAX4 variants. ${Delta}$ pH-dependent 10 µM ⁴⁵Ca²⁺ uptake was measuredat a single 10-min time point into yeast vacuolar-enriched membranevesicles isolated from K667 strains expressing sCAX1, sCAX4-9,and HA-CAX4. Ca²⁺ uptake (10 µM) determined in the absenceof excess nonradioactive metal (control) was compared with uptakedetermined in the presence of two concentrations (10x and 100x)of nonradioactive metals CaCl₂, MnCl₂, CdCl₂, ZnCl₂, NiCl₂,NaCl, and KCl (Fig. 1B). Inhibition of Ca²⁺ uptake by nonradioacitveCa²⁺ was used as an internal control, and as expected Ca²⁺ uptakeby each CAX transporter was strongly inhibited by excess Ca²⁺.Nonradioactive Ca²⁺, particularly the 10x concentration, didnot completely inhibit Ca²⁺ uptake, further highlighting thelow Ca²⁺ affinity of the CAX transporters. Ca²⁺ uptake by sCAX1and sCAX4-9 was inhibited by Cd²⁺, Na⁺, and K⁺, but this inhibitionwas only significant at the higher concentrations. Interestingly,HA-CAX4 Ca²⁺ transport was not inhibited by any of the metalstested (Fig. 1B). These results indicate that CAX4 may be morespecific for Ca²⁺ than sCAX1 or the sCAX4 variants that containthe Ca²⁺ domain of CAX1.

CAX Expression in Tomato

The phenotypes of transgenic plants expressing sCAX1, in conjunctionwith the biochemical properties of sCAX1 in yeast, suggest thatexpression of this transporter can alter Ca²⁺ homeostasis intomatoes (Hirschi et al., 1996; Hirschi, 1999). Given the Ca²⁺deficiency-like symptoms caused by sCAX1 expression in tobaccousing the cauliflower mosaic virus (CaMV) 35S promoter (Hirschi,1999), we opted to express sCAX1 under the control of the cdc2apromoter (Doerner et al. 1996; Fig. 2A). In Arabidopsis, cdc2atranscript levels are correlated with the competence to divide;however, the expression of this Arabidopsis promoter has notbeen detailed in tomato. In our preliminary analysis, we foundthat cdc2a::sCAX1 plants expressed less than half the amountof sCAX1 RNA as compared to 35S::sCAX1 plants (data not shown).Initially we transformed cdc2a::sCAX1 into tomato cv Red Cherry,a BER-tolerant variety. We use the abbreviation TCX1 (for tomatosCAX1) to identify plants expressing the cdc2a::sCAX1 construct.A tomato vector control (TVC1)-expressing line is representativeof the empty vector controls used in this study. We generatedeight TCX1-expressing lines and eight TVC1-expressing lines.Initially, we examined the transgenic tomato lines by Southernanalysis. TCX1 lines contain various copy numbers of the sCAX1expression construct (Fig. 2C). The line termed TCX1-2 containeda single insertion. The RNA gel blot documented that sCAX1 transcriptsaccumulated in all TCX1 lines. We consistently saw two transcriptsusing the cdc2a promoter and only one with the 35S::sCAX1 tomatoes(Fig. 2D; data not shown). We attribute the two transcriptsto multiple transcriptional initiation sites on the vector.The lower band of the two corresponded to the band seen in 35S::sCAX1plants (data not shown). The inability to detect a tomato CAX1homolog in the TVC lines by either Southern or northern blotsmay be due to the stringency of hybridization used in this study.

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Figure 2. Molecular analyses of sCAX1- and CAX4-expressing tomatoes. A and B, T-DNA regions of pcdc2A::sCAX1 (A) and pCaMV35S::CAX4 (B). RB, Right border; LB, left border; Nos-pro, nopaline synthase promoter; NPTII, neomycin phosphotransferase; Nos-ter, nopaline synthase terminator; CDC2a-pro, cell division cycle promoter; 35S-pro, CaMV 35S promoter; CAX4, cation exchanger 4; N-ter, nopaline synthase terminator. C and E, Southern-blot analysis of transgenic tomato plants. Five to 10 µg of tomato genomic DNA were digested with EcoRI or SalI (for pcdc2A::sCAX1) and with XbaI (for pCaMV35S::CAX4), and hybridized with the sCAX1 cDNA probe (C) and CAX4 cDNA probe (E), respectively. D and F, Northern-blot analysis of transgenic tomato plants. Ten micrograms of total RNA from expanded leaves and green fruit (gf) were hybridized with the sCAX1 cDNA probe (D) and CAX4 cDNA probe (F), respectively. Ethidium bromide-stained rRNA (bottom) is shown as a loading control.

The 35S::CAX4 construct, in which CAX4 was driven by the CaMV35S promoter (Fig. 2B), was transformed into tomato (cv Rubion).Ten independent CAX4-expressing lines were generated. We randomlyselected four transgenic lines, and the stable integration andtransmission of the 35S::CAX4 chimera in the genome of T₁ TCX4tomatoes was confirmed by Southern-blot analysis (Fig. 2E).The lines we have termed TCX4-8, TCX4-9, and TCX4-10 appearedto contain more than one integration event, while line TCX4-16had a single-copy insertion. RNA gel blot documented that CAX4transcripts accumulated in all of the transgenic lines (Fig. 2F;data not shown).

Three T₁ transgenic lines (TCX4-8, TCX4-9, and TCX4-16) showinga low copy number of the CAX4 gene were selected and subjectedto further analysis of Ca²⁺ accumulation and shelf life in CAX4-expressingfruits.

sCAX1 Expression Altered Tomato Growth

The expression of sCAX1 caused all the tomato plants to be morecompact and sturdier throughout their lives (Fig. 3, A and B).sCAX1 expression caused necrotic lesions to form on primarytransformants (Fig. 3D, left). This phenotype was apparent onall the sCAX1-expressing transformants, while none of the vectorcontrol lines displayed this phenotype. With the addition ofCa²⁺ to the growth media, the primary sCAX1-expressing transformantsno longer had extensive apical burning (Fig. 3D, right). ThesCAX1-expressing plants grown in soil also manifested mild Ca²⁺deficiency-like symptoms; again, this phenotype could be significantlysuppressed by adding Ca²⁺ to the watering solution. Examinationof the root structure showed a 40% increase in the root massin all of the sCAX1-expressing plants (root weight at day 40was 34 ± 3 g for TCX1 lines, right, and 25 ± 3g for TVC1 lines, left; Fig. 3E). Examination of plant heightfor the sCAX1-expressing plants (plant height from soil surfaceto the upper leaf; 105 ± 15 cm for TCX1 lines) foundthat they were approximately 50-cm shorter than vector controlplants (165 ± 23 cm for TVC1 lines) after 5 months ofgrowth in soil (Fig. 3B). The mature sCAX1-expressing plantsappeared to have thicker leaves (0.4 ± 0.05 mm for TCX1lines, right, and 0.2 ± 0.05 mm for TVC1 lines, left;Fig. 3F). The morphology of the sepals of sCAX1-expressing lines(right) was also altered compared to vector control lines (left;Fig. 4A). The fruit set was delayed by approximately 4 to 5weeks in six of the sCAX1-expressing lines; the other two linesdid not produce fruit. The overall shape of the transgenic fruitwas indistinguishable from that of vector controls (Fig. 4, B, C, and E).However, the seed size was significantly reducedin the sCAX1-expressing lines compared to vector control lines(Fig. 4, B–D). One out of six sCAX1-expressing primarytransformants was capable of making viable seed, in contrastto most of the vector control lines. Another striking phenotypeof the sCAX1-expressing lines was a significantly increasedoccurrence of BER. The incidence of BER was higher in all ofthe sCAX1-expressing lines (75% ± 14% for TCX1 linesand 8% ± 5% for TVC1 lines; Fig. 4, I and J). cdc2a::sCAX1was also transformed into tomato cv FM9, another BER-tolerantvariety, to determine whether the sCAX1-induced phenotypes werenot a consequence of the Red Cherry variety used in the study.Severe BER symptoms were also observed for the FM9 variety expressingsCAX1 in addition to the other changes in plant morphology thatwere found in sCAX1-expressing Red Cherry tomato lines (datanot shown).

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Figure 3. Phenotypes of sCAX1- and CAX4-expressing tomato plants. A, Growth of TVC1-1 vector control (left) and the sCAX1-expressing TCX1-2 plant (right) after 3 weeks in soil. B, Growth of vector control (left) and sCAX1-expressing TCX1-2 plant (right) after 5 months in soil. C, Growth of vector control (left) and CAX4-expressing TCX4-16 plant (right) after 4 months in soil. D, sCAX1-expressing TCX1-2 tomato grown in soil for 2 months without application of exogenous Ca²⁺ (left) and with the addition of Ca²⁺ (right). E, Root structure of vector control (left) and sCAX1-expressing TCX1-2 plant (right). F, Leaf phenotype of vector control (left) and sCAX1-expressing TCX1-4 plant (right).

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Figure 4. Phenotypes of sCAX1- and CAX4-expressing tomato fruits. A, Sepals of vector control (left) and sCAX1-expressing plants (right). B and C, Tomato longitudinal section of sCAX1-expressing tomato fruit (B) and vector control (C). D, Seeds of vector control (left) and sCAX1-expressing plants (right). E, Fruit from vector control (left) and sCAX1-expressing TCX1-2 and TCX1-4 plants (right) 20 d after breaker stage. F, Fruits from vector control (left) and sCAX1-expressing TCX1-2 and TCX1-4 plants (right) 40 d after breaker stage. G, Fruits from vector control (left) and CAX4-expressing TCX4-9 and TCX4-16 plants (right) 30 d after breaker stage. H, Tomato longitudinal section of vector control (left) and CAX4-expressing tomato fruit (right). I and J, BER of tomato fruits from vector control (I) and sCAX1-expressing tomato plant (J). The incidences of BER were mainly seen in the sCAX1-expressing plants. K and L, BER of tomato fruits from vector control (K) and CAX4-expressing tomato plant (L). No incidences of BER were mainly seen in the CAX4-expressing plants.

All subsequent experiments with sCAX1-expressing Red Cherrytomato lines were done on primary transformants that had similarphenotypes. The cdc2a::sCAX1-expressing primary transformants(TCX1-2 and TCX1-4), which have a single copy of CAX1, wereused for all other analysis.

Phenotypes of CAX4-Expressing Tomatoes

While the sCAX1-expressing lines were sensitive to Ca²⁺ deficiencyand showed Ca²⁺ deficiency-like symptoms that were suppressedby addition of Ca²⁺, the CAX4-expressing lines were not sensitiveto Ca²⁺ deficiency and did not require any additional Ca²⁺ supplementationfor normal growth. In addition, both CAX4-expressing lines andwild-type control grew similarly on one-half strength Murashigeand Skoog medium, Ca²⁺-depleted one-half strength Murashigeand Skoog medium, and the one-half strength Murashige and Skoogmedium supplemented with various ion metals, such as NaCl andMgCl₂ (data not shown). In TCX4 plants, CAX4 expression didnot perturb the morphology, growth (Fig. 3C), or fruit set (Fig. 4, K and L).Moreover, the fruit set was not delayed, all CAX4transformants were capable of making viable seed (Fig. 4H),and the total fruit yield of CAX4 plants was indistinguishablefrom the wild-type control (data not shown). As the expressionof sCAX1 caused a significant increase in BER occurrence insupposed BER-tolerant tomato varieties (Red Cherry and FM9),we chose to express CAX4 in a BER-susceptible tomato variety(cv Rubion) in order to examine the effect of CAX4 expressionon BER induction. The incidence of BER was equivalent in theCAX4-expressing lines (BER ratio; 15% ± 5% for TCX4 lines)and vector control lines (BER ratio; 18% ± 6% for TVC4lines).

H⁺/Ca²⁺ Antiport in sCAX1-Expressing Tomatoes

Expression of sCAX1 in yeast restores H⁺/Ca²⁺ antiport activityto yeast strains deficient in this transporter (Hirschi et al.,1996). In plants, expression of sCAX1 in tobacco also causesincreased H⁺/Ca²⁺ antiport (Hirschi, 1999). H⁺/Ca²⁺ antiportactivity was measured in tonoplast-enriched vesicles from sCAX1transgenic and vector control tomato roots to confirm that expressionof sCAX1 resulted in increased ${Delta}$ pH-dependent Ca²⁺ transport.The sCAX1 transcript was found to be constitutively expressedthroughout the tomato plant in all lines (data not shown); therefore,root tissue was used to determine antiport activity. A protongradient (acid inside vesicles) was formed by activation ofthe Mg²⁺ATP-dependent H⁺-ATPase. H⁺/Ca²⁺ antiport activity measuredin the presence of the P-type ATPase inhibitor, vanadate, wassignificantly higher in vesicles from the TCX1-2 line comparedto the TVC1 (Fig. 5B). A TVC line accumulated Ca²⁺ to approximatesteady-state concentrations of 0.22 ± 0.01 nmol Ca²⁺mg protein^–1 (Ca²⁺ uptake in the presence of vanadatewithout carbonyl cyanide p-(trifluoromethoxy)phenylhydrazone[FCCP] was 0.93 ± 0.01 nmol Ca²⁺ mg protein^–1 andin the presence of vanadate with FCCP was 0.71 ± 0.01nmol Ca²⁺ mg protein^–1), while TCX1-2 accumulated Ca²⁺to concentrations of 0.39 ± 0.09 nmol Ca²⁺ mg protein^–1(Ca²⁺ uptake in the presence of vanadate without FCCP was 1.2± 0.08 nmol Ca²⁺ mg protein^–1 and in the presenceof vanadate with FCCP was 0.81 ± 0.02 nmol Ca²⁺ mg protein^–1).Ca²⁺ transport activity measured in the absence of vanadateand in the presence of the protonophore FCCP was identical invesicles from both plants (Fig. 5A).

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Figure 5. Ca²⁺ uptake activity into tonoplast-enriched vesicles from tomato root. A and B, Time courses of Mg²⁺ATP-energized 10 µM ⁴⁵Ca²⁺ uptake were performed in the presence of 0.1 mM NaN₃, 10 mM KCl, 3 mM ATP, and 3 mM MgSO₄. Ca²⁺-ATPase activity (A) was determined in the absence of orthovanadate and the presence of 5 µM FCCP. ${Delta}$ pH-dependent H⁺/Ca²⁺ antiport activity (B) was determined in the presence of 0.2 mM orthovanadate as the difference between Ca²⁺ uptake in the absence and presence of 5 µM FCCP. The Ca²⁺ ionophore A23187 (5 µM) was added at the time indicated. Black circles, sCAX1-expressing TCX1-2 plant; white circles, vector controls. Results are the average (± SE) of six replicate experiments using two independent membrane preparations.

Ca²⁺ Accumulation in CAX-Expressing Tomato Plants

Altered H⁺/Ca²⁺ antiport activity in tonoplast-enriched membranevesicles from sCAX1-expressing tomato plants indicated perturbedCa²⁺ transport properties. To ascertain whether sCAX1 expressionaltered ion levels, Ca²⁺ levels and other minerals were measuredin the transgenic plants. The leaves of all sCAX1-expressingplants showed at least a 20% increase in Ca²⁺ levels (data notshown), while initial measurements of fruit Ca²⁺ levels showedthat three (TCX1-2, -3, and -4) of the sCAX1-expressing lineshad significant alteration in Ca²⁺ (Fig. 6A). Over time theTCX1-2 and TCX1-4 fruits contained more than twice the Ca²⁺levels as vector control plants that were supplemented withCa²⁺ (Fig. 6B). TCX1-2 and TCX1-4 fruits also contained increasedlevels of Cu²⁺, Fe²⁺, Mg²⁺, Mn²⁺, and Zn²⁺ (Fig. 6, C and D).Similar changes were seen in the other sCAX1-expressing line(TCX1-3), which contains multiple copies of sCAX1 (data notshown).

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Figure 6. Concentrations of Ca²⁺ and other minerals in fruits of sCAX1- and CAX4-expressing plants. A to E, Fruit Ca²⁺ and mineral analysis was performed at 20 d after breaker stage. Total Ca²⁺ (A, B, and E) and mineral contents (C and D) of fruits (pooled at least five-fruit batches) were determined by inductively coupled plasma emission spectrophotometer. Data represent the values obtained from pools containing at least five fruit over a 6-month period (B), and the means (±SD) of four independent analyses (A and C–E). E, Concentrations of Ca²⁺ in fruits of CAX4-expressing plants.

All of the CAX4-expressing T₁ tomatoes (TCX4-8, -9, and -16)contained significantly more Ca²⁺ (40%–50% increase) thanvector controls (Fig. 6E). No significant increase of otherminerals (Cu²⁺, Fe²⁺, Mg²⁺, Mn²⁺, and Zn²⁺) was observed withany of the lines analyzed (data not shown). In addition, nosignificant differences were observed for Na⁺ and K⁺ levelsin both sCAX1- and CAX4-expressing lines compared to wild-typelines (data not shown).

Increased Fruit Firmness and Prolonged Shelf Life in CAX-Expressing Plants

In some agriculturally important crops, addition of exogenousCa²⁺ increases fruit firmness and shelf life (Lester and Grusak,1999; Lopez-Lefebre et al., 2001). We were interested in determiningwhether the increased Ca²⁺ in the transgenic fruit would causeincreased firmness in the TCX1 lines. As shown in Figure 7,the decline in fruit firmness that is associated with fruitripening was greatly delayed in sCAX1-expressing plants. Duringthe first 30 d after the breaker stage, the TCX1 fruits weretwice as firm as the controls. After 40 d, tomato fruits harvestedfrom sCAX1-expressing plants maintained their structural integrity,while the vector control lines were significantly shrunken (Fig. 4F).Similar changes were seen in the sCAX1-expressing line(TCX1-3) containing multiple copies of the transgene (data notshown).

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Figure 7. Firmness analysis in fruits of sCAX1-expressing plants. Fruits were harvested at 10 (10d), 20 (20d), 30 (30d), and 40 (40d) days after the first color change (the breaker stage). Four fruits were used for each measurement. Firmness was determined using a texture analyzer. Values shown are the means (±SD) of four fruits. White bars, control; black bars, fruits of sCAX1-expressing plants.

To determine whether the increased Ca²⁺ in the transgenic fruitincreased firmness and prolonged shelf life in the TCX4 lines,we measured the mean separations at specific time points (i.e.5, 10, 15, 20, 25, 30, 35, and 40 d). A significant change wasobserved in break date and treatment (Table I). At 30 d afterthe breaker stage, the TCX4 fruits harvested from CAX4-expressingplants maintained their structural integrity, while the vectorcontrol fruits were significantly shrunken (Fig. 4G). Overall,the decline in fruit firmness that is associated with fruitripening was slightly delayed in CAX4-expressing plants (datanot shown), and the shelf life of CAX4-expressing T₂ tomatoesextended the time until shrinkage about 5 d compared to thevector controls (Table I).

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Table I. Shelf life analysis of CAX4-expressing tomato fruits

The letters (a, b, c, and d) denote statistically significant differences between TCX4 fruits and control fruits. One balanced design (12 plots) and one unbalanced design (eight plots) containing each of 20 fruits a plot were used for shelf life analysis by a randomized-complete block design with three replications. Data were analyzed by ANCOVA, and mean separations was based on the Tukey-Kramer procedure at ${alpha}$ = 0.05.

Sugar Concentration and Ethylene Production

Because the phenotypes were the most prevalent in the sCAX1-expressingplants, we measured sugar and ethylene levels in these transgenicfruit during ripening. The sugar concentration and ethyleneproduction in the sCAX1-expressing lines were comparable tothose of the vector control lines (Fig. 8, A and B). Again,similar results were obtained in two sCAX1-expressing lineshaving a single copy (TCX1-4) and multiple copies (TCX1-3) ofthe transgene (data not shown). Like the sCAX1-expressing fruit,the CAX4-expressing fruit has no alteration in sugar concentrationcompared to wild-type (data not shown).

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Figure 8. Sugar and ethylene production in fruits of sCAX1-expressing plants. A, Concentration of total sugars in fruits of sCAX1-expressing plants. Control (30.60 mg g^–1 fresh weight and sCAX1-expressing fruits (30.54 mg g^–1 fresh weight) were harvested at 20 d after breaker stage, and the concentration of soluble sugars in fruits (pooled four-fruit batches) were analyzed by HPLC. Values (Suc, Glc, and Fru) shown are the means of three injections on the HPLC. White bars, control; black bars, fruits of sCAX1-expressing plants. B, Ethylene production was assayed during a 10-d ripening period after initiation of the first color change. Data shown are the means of values obtained from three fruits. White circles, control; black circles, fruits of sCAX1-expressing plants.

	DISCUSSION

TOP ABSTRACT RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

We selected tomato as the vegetable in which to express H⁺/Ca²⁺transporters as a means to increase Ca²⁺ content. Three tomatocultivars, Red Cherry and FM9, fresh market tomatoes reportedto have some tolerance to BER (K. Crosby, Texas AgriculturalExperiment Station, personal communication), and Rubion, a processingtomato completely susceptible to BER (R. Johns, Seminis, personalcommunication), were selected in this study. Ca²⁺ deficiencyis the most common nutritional problem affecting tomatoes, whichcomprise the second-largest vegetable crop in the United States,after potatoes. A lack of Ca²⁺, water, or both can cause BERin tomatoes (Ho and White, 2005

). In addition, tomatoes arehighly susceptible to postharvest decay, and must be handledwith special care to avoid wounds, bruises, and other injuriesthat would serve as ports of entry for various pathogens. Toensure firmness on arrival after shipping, tomatoes are pickedat the mature green stage, which precludes extended vine ripening.Here we have demonstrated the ability to increase Ca²⁺ levelsin tomatoes, which may be a means to deliver more Ca²⁺ to consumers,adjust growth constraints, and vary the harvesting practicesof an agriculturally important commodity.

Previous studies have demonstrated that expression of Ca²⁺-signalingcomponents, such as a Ca²⁺ transporter or a Ca²⁺-binding protein,can be used to increase Ca²⁺ levels in various plants (Wyattet al., 2002; Hirschi, 2004). In this study, we have expressedsCAX1 driven by the cell cycle promoter cdc2a (Doerner et al.,1996; Fig. 2A). To our knowledge, the Arabidopsis cdc2a promoterhas not been previously used in tomato and here we show thefirst preliminary examination of its use in this plant. Thecdc2a-driven sCAX1 expression was found to be constitutivelyexpressed in all tomato tissues analyzed (data not shown), suggestingthat sCAX1 H⁺/Ca²⁺ antiport activity would be equally enhancedin all tissues compared to control plants. We therefore choseto measure antiport activity from root tissue rather than tomatofruit as it is technically much more difficult to isolate intactmembrane vesicles from fruit, particularly when ripe, ratherthan from other tissues. Roots from TCX1 plants showed a 44%increase in tonoplast-enriched H⁺/Ca²⁺ transport (Fig. 5B) andno change in Ca²⁺-ATPase activity (Fig. 5A). These results showwe have not measurably perturbed another Ca²⁺ transport mechanismon the root vacuolar membrane.

The cdc2a::sCAX1-expressing tomatoes without additional Ca²⁺supplementation in the soil demonstrate symptoms of Ca²⁺ deficiencies,particularly apical burning (Fig. 3D, left). The alterationsin plant size, leaf morphology, fruit set, and ripening (Figs. 3and 4) further emphasize the importance of regulated Ca²⁺transport in plant growth and development. Several of thesephenotypes, particularly the apical burning, are similar tothose of sCAX1-expressing tobacco plants (Hirschi, 1999). Thus,despite the increased Ca²⁺ in both tobacco and tomato plants,they are suffering from Ca²⁺ deficiency symptoms (see below).Ca²⁺ supplementation in the soil (Fig. 3D, right) was requiredto obtain maximal growth of sCAX1-expressing tomato plants (Fig. 3,D and F). The roots of the cdc2a::sCAX1-expressing tomatoesappeared more vigorous than those of the control plants. Thesefindings implicate the levels of Ca²⁺ in strongly influencingroot growth (Picchioni et al., 2001). This is interesting whenone considers that 35S::sCAX1 expression in tobacco decreasesroot mass (Hirschi, 1999). Our findings suggest that the useof the cdc2a promoter mitigated some of the most severe symptomsassociated with high-level expression of sCAX1. Some cation/H⁺antiporters are known to have a role in regulating cytoplasmicor vacuolar pH (Yamaguchi et al., 2001). We have not analyzedthe effect of CAX expression on pH levels in the tomato, andit will be interesting to see whether any morphological changesto the plants are due to altered pH homeostasis.

Unexpectedly, one of the most deleterious changes in fruit developmentcaused by sCAX1 expression in the tomato cultivars, Red Cherryand FM9 (both cultivars have been reported to have toleranceto BER), was the dramatically increased incidence of BER (Fig. 4J).Evidence for Ca²⁺ deficiency as the primary cause of BERhas been derived from observations that the blossom end hasthe lowest content of Ca²⁺ within tomato fruits (Adams and Ho,1993; Nonami et al., 1995). BER is generally associated withthe disintegration and increased ion permeability of cells,resulting in loss of turgor and cell fluids invading the intercellularair space, thus causing the watery appearance in the early stages(Shear, 1975; Simon, 1978). However, despite the increased Ca²⁺in tomato fruits, the increased incidence of BER in sCAX1-expressingtomatoes is perplexing. We expect that the increased Ca²⁺ inthe tomato fruit is due to a significant increase in vacuolarCa²⁺ level within the rapidly expanding fruit due to the enhancedand unregulated vacuolar Ca²⁺/H⁺ antiport activity. Therefore,one possible explanation for the increased BER is that sCAX1-expressinglines have altered Ca²⁺ homeostasis between cytosolic, apoplastic,and vacuolar Ca²⁺ pools, with decreases in cytosolic and apoplasticCa²⁺ levels. It has been suggested that this may disrupt Ca²⁺-signalingprocesses, membrane integrity, and normal cell wall development,leading to cell death and thus the occurrence of BER (Ho andWhite, 2005). Future work will therefore need to determine whetherthere is indeed reduced cytosolic and/or apoplastic Ca²⁺ levelsin the sCAX1-expressing tomato fruit. An alternative explanationfor increased occurrence of BER might be that expression ofsCAX1 in vegetative tissues results in a localized Ca²⁺ deficiencyin early fruit development.

While the sCAX1-expressing Red Cherry and FM9 (BER-tolerantcultivars) have increased incidence of BER, no significant differencewas observed with the CAX4-expressing Rubion (a cultivar susceptibleto BER) when compared to vector controls (Fig. 4, K and L).This may be due in part to the more modest increase in tomatofruit Ca²⁺ levels seen with TCX4 lines compared to the TCX1lines. Moreover, CAX4 expression did not perturb the morphology,growth (Fig. 3C), or fruit set (Fig. 4L). Future work will befocused on the mechanisms of CAX expression and BER development.

The deleterious changes in plant growth caused by cdc2a::sCAX1expression in tomato plants (e.g. Fig. 3, B and E) suggest thatfurther modulation of the expression of H⁺/Ca²⁺ transportersis needed. Rather than alter the expression of the transporter,another approach is to turn down the CAX-mediated Ca²⁺ transportthroughout the plant by posttranslational down-regulation. Herewe have used full-length CAX4 containing the entire putativeN-terminal autoinhibitory domain. CAX4 is 54% identical to CAX1at the amino acid level, and previous work suggests that repositioningof the N terminus in this transporter confers Ca²⁺ transportin yeast assays (Fig. 1A; Cheng et al., 2002). When HA-CAX4is expressed in yeast, competition experiments suggest thatthis variant is a more specific Ca²⁺ transporter than sCAX1or the variant of CAX4 that contains the Ca²⁺ domain of CAX1(sCAX4-9). However, it is possible that the presence of theHA tag could disrupt the selectivity or the regulatory propertiesof CAX4. Transport experiments with sCAX4 should determine whetherthe HA tag does actually affect CAX4 activity. Unfortunatelywe were unable to obtain transport measurements for sCAX4 inthe yeast system so alternative approaches will be requiredto address this question in the future. Our working hypothesisis that in planta CAX4 is an H⁺/Ca²⁺ transporter. Interestingly,we attempted several times to generate transgenic lines expressingeither sCAX4-9 or HA-CAX4 but were unable to produce viableplants (data not shown).

While the cdc2a::sCAX1 tomato plants have increased Ca²⁺ whencompared to vector controls, they also display increased levelsof several other ions, particularly Mg²⁺, Zn²⁺, Fe²⁺, and Mn²⁺(Fig. 6). Metal competition experiments infer that sCAX1 cantransport Cd²⁺ as well as Ca²⁺ but not Mn²⁺ (Fig. 1B; Shigakiet al., 2001). Competition experiments also suggest that sCAX1cannot transport Fe²⁺ and Cu²⁺ (data not shown), while directtransport measurements have shown that wild-type sCAX1 cannotefficiently transport Ni²⁺, Co²⁺, and Mn²⁺ but has some abilityto transport Cd²⁺ and Zn²⁺ in addition to Ca²⁺ (Shigaki et al.,2005). Similar direct transport experiments will be needed tofurther determine the transport properties of CAX4 and CAX4variants. Meanwhile, in agreement with the yeast uptake assaysusing HA-CAX4, the CAX4-expressing plants have increased levelsonly of Ca²⁺. The lack of deleterious morphological phenotypesin the CAX4-expressing plants may correlate with the absencein accumulation of various transition metals. Even at micromolarconcentrations some transition metals can be particularly toxic(Marschner, 1995); therefore, some of the phenotypes in thesCAX1-expressing plants could also be due in part to toxicityinduced by Fe²⁺, Zn²⁺, or Mn²⁺ accumulation. It is also worthnoting that increased H⁺/Ca²⁺ transport activity may activateother proton-mediated transporters (Cheng et al., 2005) to causealterations in plant growth.

While all the sCAX1-expressing lines showed increased Ca²⁺ levelsin the leaves (data not shown), only a portion of the linesshowed changes in Ca²⁺ levels in the fruit. This may be becausewe did not assay fruit from older plants for all the lines.Our data suggest that fruit derived from older sCAX1-expressingplants contain more Ca²⁺ (Fig. 6B). Alternatively, the sCAX1transporter may have to be highly expressed in particular cellsin order to facilitate increased Ca²⁺.

Currently, most Americans obtain their dietary Ca²⁺ from milk-relatedproducts; fruits like tomatoes do not contribute significantlyto Ca²⁺ intake (Fleming and Heimback, 1994). In other areasof the world, communities obtain a majority of their total dietaryCa²⁺ from the consumption of fruits and vegetables (Weaver etal., 1999). Increasing the endogenous levels of Ca²⁺ in commonlyconsumed fruits should help yield improved dietary Ca²⁺ intakeswithin many population groups. However, bioavailability studiesare needed to determine to what extent these mineral changesin fruit translate into improved Ca²⁺ bioavailability and nutritionalquality.

Applications of CaCl₂ are used as a means to increase the firmnessof various fruits prior to shipment. Since little translocationof Ca²⁺ occurs from leaves to growing fruits, direct Ca²⁺ applicationon the surface is recommended. However, late-season applicationof Ca²⁺ to apples (Malus domestica), pears (Pyrus communis),and other commodities is often avoided due to the costs andthe potential of damaging the fruit or accelerating postharvestfungal infections. We have demonstrated here that expressionof CAX transporters in tomatoes can be used to increase thefirmness and shelf life of tomato fruit (Figs. 4, F and G, and7). Interestingly, sCAX1 expression does not appear to alterthe sugar concentration of the tomatoes (Fig. 8). These findingsimply that CAX-expressing tomatoes can be left on the vine toripen longer, enabling them the potential to offer improvedflavor while retaining the firmness necessary to withstand therigors of shipping. Exogenous applications of Ca²⁺ to fruithave been shown to be associated with decreased fruit respirationrate and ethylene production (Faust and Shear, 1972; Liebermanand Wang, 1982). However, an increase in fruit Ca²⁺ levels byenhanced activity of vacuolar Ca²⁺/H⁺ antiport does not appearto decrease ethylene production (Fig. 8B). The mechanisms bywhich Ca²⁺ effects ethylene biosynthesis are not fully understood,but it is conceivable that cytosolic Ca²⁺ signals may have arole in regulating ethylene production (Njoroge et al., 1998).While exogenous application of Ca²⁺ to tomato fruit will likelycause an initial increase in cytosolic Ca²⁺ and a decrease inethylene, increase in fruit Ca²⁺ by sCAX1 overexpression willincrease vacuolar Ca²⁺ levels but may prevent any substantialincrease in cytosolic Ca²⁺, thus preventing a decrease in ethyleneproduction.

Tomato fruit is a climacteric fruit in which ripening is initiatedby increased production of ethylene (Adams-Phillips et al.,2004; Giovannoni, 2004). In this study we have observed thatthe fruit from sCAX1-expressing plants ripen more slowly (Figs. 4Fand 7) despite ethylene production being unperturbed (Fig. 8B).Previous studies have also demonstrated alteration in tomatofruit ripening without an alteration in ethylene biosynthesis.The tomato mutants Green-ripe, Never-ripe (Nr), and Nr-2 donot fully ripen, yet ethylene synthesis is unchanged comparedto wild-type fruit (Lanahan et al., 1994; Barry et al., 2005).It was suggested that these altered-ripening phenotypes aredue to ethylene insensitivity. In fact, in the Nr mutant, thisinsensitivity is due to a mutation in an ethylene receptor (Wilkinsonet al., 1995). Studies suggest that Ca²⁺ is involved in signalingpathways regulating fruit ripening. For example, it has beenshown that Ca²⁺ is required for ethylene-dependent processes(Raz and Fluhr, 1992) and a tomato Ca²⁺-dependent protein kinase-relatedkinase, LeCRK1, which is regulated during ripening has beenidentified (Leclercq et al., 2005). The results from our worksuggest that altering the Ca²⁺ homeostasis of the fruit by sCAX1expression can affect the regulation of fruit ripening. Futurework will need to be directed at the actual signaling and developmentalevents that are altered in the CAX-expressing plants, such aswhether the plants are ethylene-insensitive like the Nr mutants.

In addition to the possible effect of increased Ca²⁺ on fruitripening pathways, the excess Ca²⁺ may also enhance fruit firmnessdue to improved cell wall integrity. Cell wall-associated Ca²⁺maintains cell wall integrity by generating cross-links withnonesterified pectins in the primary cell wall and middle lamella(Jarvis, 1984; Poovaiah et al., 1988). Homogalacturonan, oneof the main polymers of pectin, can form cross-links with Ca²⁺by the binding of Ca²⁺ with carboxylate ions, to form paralleland antiparallel chains, causing the wall to be more rigid.The presence of Ca²⁺-pectin bridges prevents the access of cellwall hydrolytic enzymes, thus inhibiting cell wall expansion(Jauneau et al., 1994; Konno et al., 1999). Further work isrequired to demonstrate that cell wall-associated Ca²⁺ levelsare indeed enhanced in CAX-expressing plants compared to wildtype.

Increased Ca²⁺ levels have been shown to alter the severityof several plant pathogens (Marschner, 1995). In the sCAX1-expressingtomatoes, we see no alterations to infection by Pseudomonassyringae pv tomato and Xanthomonas campestris pv vesicatoriaor Botrytis (data not shown). Further tests must be performedin various environmental conditions to firmly establish thatwe have not altered the susceptibility to pathogens. However,it is easy to envision that increasing the firmness of the tomatofruits could delay the penetration of a particular pathogen.

In this report, we have demonstrated the ability to increaseCa²⁺ levels in tomatoes through heightened activity of a Ca²⁺transporter. We have demonstrated here that expression of theH⁺/Ca²⁺ transporters can increase fruit Ca²⁺ levels as wellas firmness.

MATERIALS AND METHODS

TOP
ABSTRACT
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

Yeast Growth, Vacuolar Membrane Isolation, and Transport Measurements

The yeast (Saccharomyces cerevisiae) strain K667 (cnb1::LEU2pmc1::TRP1 vcx1 ${Delta}$ ) (Cunningham and Fink, 1996) was used to expressvarious CAX cDNA constructs in the yeast shuttle vector pHGpd(Nathan et al., 1999). Yeast transformation using the lithiumacetate/polyethylene glycol transformation method, and isolationof yeast vacuolar-enriched membrane vesicles, were performedas described previously (Pittman et al., 2004a). Measurementsof ⁴⁵CaCl₂ uptake into yeast membrane vesicles and metal competitionexperiments were performed as described previously (Shigakiet al., 2003).

Plant Material, Transformation, and Growth Conditions

Seeds of tomato (Lycopersicon esculentum) Mill. cultivars RedCherry, FM9, and Rubion were surface sterilized. Seeds weregerminated on a Murashige and Skoog (1962) inorganic salt mediumwith 30 g L^–1 Suc, pH 5.7, and solidified using 8 g L^–1TC agar (Sigma). Tomato transformation was performed via Agrobacterium-mediatedtransformation method using cotyledon and hypocotyl explantsas described (Park et al., 2003). Cultures were maintained at25°C under a 16-h photoperiod. After 6 to 8 weeks (subculturedonce at 3–4 weeks), regenerated shoots were transferredto rooting medium for 6 more weeks (for sCAX1-expressing transgeniclines, 3 mL of 2 mM CaCl₂ were added to rooting medium to suppressthe growth defects of sCAX1-expressing tomato once at 4 weeks),then established in soil. All plants were watered as needed.Once a week they were watered with Miracle-Gro for tomato (ScottsMiracle-Gro Products). The temperature of the greenhouse wasmaintained within a range of 25°C to 30°C. For maximalgrowth, sCAX1-expressing transgenic lines in the greenhousewere watered to saturation with 2 mM CaCl₂ twice a week forthe first 8 weeks.

Bacterial Strain and Plasmids

Agrobacterium tumefaciens LBA 4404 octopine (Hoekema et al.,1983) was used for the transformations. The plasmid pcdc2A::sCAX1or pCaMV35S::CAX4 was introduced into A. tumefaciens using thefreeze-thaw method (Holsters et al., 1978). The sCAX1 open readingframe was cloned into the nos/nptII/nos-ter/cdc2a /nos-ter expressionvector, which was obtained from John Celenza (Doerner et al.,1996).

DNA Isolation and Southern-Blot Analysis

Tomato genomic DNA was extracted from leaf tissue as previouslydescribed (Paterson et al., 1983). DNA (5–10 µg)was digested with SalI or EcoRI and separated by electrophoresisand blotted onto a nylon membrane (Zeta-probe GT membrane, Bio-RadLaboratories) according to the manufacturer's instructions.The probe for the sCAX1 gene was isolated from a NotI (1.4 kb)restriction fragment of the p039 plasmid (Hirschi et al., 1996),and the probe for the CAX4 gene was isolated from a SacI-XbaI(1.3 kb) restriction fragment of the pBlue-CAX4 plasmid (Chenget al., 2002). The membranes were prehybridized overnight at65°C in 7% SDS and 0.25 M Na₂HPO₄, and then hybridized overnightat 65°C in the same solution containing the probe labeledwith ³²P-dCTP using NEBlot kit (NEB BioLabs). Membranes werewashed twice for 30 min each with 20 mM Na₂HPO₄ and 5% SDS at65°C and then washed twice again for 30 min each with 20mM Na₂HPO₄ and 1% SDS at 65°C. Membranes were exposed tox-ray film at –80°C.

RNA Isolation and Northern-Blot Analysis

Total RNA was extracted from green fruit tissues and leavesusing RNeasy plant kits (Qiagen) according to the manufacturer'sinstructions. Total RNA (7 µg) was separated on a 1.2%agarose gel containing 1.5% formaldehyde, blotted onto a Zeta-ProbeGT membrane according to the manufacturer's instructions. Hybridizationand washing were as previously described in Southern-blot analyses.

Plant Measurements

The heights of plants (from soil surface to the upper leaf)were measured after 5 months of growth in soil. The means (±SD)of three independent sCAX1-expressing lines were compared tothe means (±SD) of three control lines. At this stage,five leaves of similar age from each of these three transgeniclines and three control lines were sampled, and leaf thicknesswas measured under a microscope (model 475050, Zeiss). Picturesof the leaf shape of these plant lines were taken to recordthe phenotypes.

Root Measurements

Root mass was measured by taking three TCX1-expressing linesand three TVC1-expressing lines and after 2 months of growthin soil gently removing the soil from the roots using water.The intact plants were then transferred to hydroponic growthconditions and allowed to grow for 14 additional days as previouslydescribed (Hirschi, 1999). The roots were then harvested anddried as previously described (Hirschi, 1999).

Endomembrane Isolation and Ca²⁺ Transport Assay

Roots of 4-week-old soil-grown TVC1 and TCX1-2 plants were homogenizedat 4°C and microsomal pellets obtained (Hirschi, 1999).Endomembrane-enriched vesicles were then prepared as previouslydescribed (Pittman et al., 2002). The ⁴⁵Ca²⁺ transport assaywas performed as previously described (Pittman and Hirschi,2001) except 5 µM FCCP was used instead of gramicidin.

Ca²⁺ and Mineral Analysis

Fruit Ca²⁺ and mineral analysis was performed at 20 d afterbreaker stage, and the fruits (pooled at least five-fruit batches)were dried at 70°C for 4 d. A total of 0.25 g (dry weight)of fruits was digested for analysis (Feagley et al., 1994).Ca²⁺ and mineral contents per gram of dry weight were determinedby inductively coupled plasma emission spectrophotometer (Spectro).

Firmness Analysis

Fruits were harvested at 10, 20, 30, and 40 d after the firstcolor change (the breaker stage). Four fruits were used foreach measurement. Firmness was determined using a TA-XTZi textureanalyzer (Texture Technologies). A speed of 2 mm s^–1 wasused to compress fruit by 4 mm with a circular probe of 4.5cm in diameter.

Shelf Life Analysis

After segregation analysis on T₂ seeds from self-pollinatedT₁ plant lines (showing a segregation pattern of 3:1 on kanamycinmedium), fruit from each of 10 homozygous T₂ lines was selected.Fruit was harvested at the mature green stage and ripened at22°C to 24°C. One balanced design (12 plots) and oneunbalanced design (8 plots) containing each of 20 fruits perplot were used for shelf life analysis by a randomized completeblock design with three replications. After the breaker stage,the mean separations were performed at special break date valuesof 5, 10, 15, 20, 25, 30, 35, and 40 d. In this study, shrinkagerating scales were as follows: rate 1 (signs of shrinkage),rate 2 ( $≤$ 25%), rate 3 (25%–50%), and rate 4 (>50%).Data were analyzed by ANCOVA, and mean separations was basedon the Tukey-Kramer procedure at ${alpha}$ = 0.05. Observation on fruitnumber and percentage of incidences of BER were recorded onall fruits from all plant lines selected in this study.

Ethylene Production Analysis

Ethylene production was assayed during a 10-d ripening periodafter the start of the first color change. Three fruits wereused for each measurement. Individual fruits were placed intosealed containers at room temperature for 1 h, and then 1-mLgas samples were withdrawn. Gas samples were analyzed via gaschromatography (model 8500 gas chromatograph, Perkin-Elmer)using a 5% carbowax column (1.8 m x 2.1 mm) and a flame-ionizationdetection system.

Sugar Analysis

Standard sugar analysis was performed (Hamilton et al., 1997).Ten grams of fruits (pooled in four-fruit batches) at 20 d afterthe first color change were cut and blended with 80% ethyl alcoholand filtered.

ACKNOWLEDGMENTS

We are thankful to Leonard Pike, George Sundin, and Larry Barnesfor discussions and for providing biological reagents. We arealso grateful to Chris Hundley for help with statistical analysis.

Received May 26, 2005; returned for revision August 11, 2005; accepted August 16, 2005.

FOOTNOTES

¹ This work was supported by the U.S. Department of AgricultureCooperative State Research, Education, and Extension Service(grant no. 2001–34402–10543), Designing Foods forHealth, and the National Institutes of Health (grant no. 1R01DK 062366).

² Present address: Faculty of Life Sciences, University of Manchester,3.614 Stopford Building, Oxford Road, Manchester M13 9PT, UK.

The author responsible for distribution of materials integralto the findings presented in this article in accordance withthe policy described in the Instructions for Authors (www.plantphysiol.org)is: Sunghun Park (s-park4{at}tamu.edu).

Article, publication date, and citation information can be foundat www.plantphysiol.org/cgi/doi/10.1104/pp.105.066266.

^{^*} Corresponding author; e-mail s-park4{at}tamu.edu; fax 979–862–4522.

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MATERIALS AND METHODS
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Increased Calcium Levels and Prolonged Shelf Life in Tomatoes Expressing Arabidopsis H+/Ca2+ Transporters1

Increased Calcium Levels and Prolonged Shelf Life in Tomatoes Expressing Arabidopsis H⁺/Ca²⁺ Transporters¹