Sulfate Transport and Assimilation in Plants

doi:10.1104/pp.120.3.637

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Sulfate Transport and Assimilation in Plants¹

Thomas Leustek^* and Kazuki Saito

Biotechnology Center for Agriculture and the Environment, Rutgers University, New Brunswick, New Jersey 08901-8520 (T.L.); and Faculty of Pharmaceutical Sciences, Chiba University, Yayoi-cho 1-33, Inage-ku, Chiba 263-8522, Japan (K.S.)

INTRODUCTION

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Introduction
References

Sulfur is one of the six macronutrients required by plants and is found in the amino acids Cys and Met and in a variety ofmetabolites. When one considers that sulfur in plants is only3% to 5% as abundant as nitrogen, it is perhaps understandablethat sulfur assimilation has been less well studied. As a partof the Cys molecule, the sulfur group, called a thiol, is stronglynucleophilic (electron-donating), making it ideally suited forbiological redox processes. When oxidized, two Cys molecules canform a covalent linkage called a disulfide bond, which is readilybroken by reduction to form two thiol groups. Disulfide $left-right-arrow$ dithiolinterchange is so versatile that nearly all aerobic forms of life,including plants, have evolved to use this reaction as the dominantform of redox control. Redox control regulates enzymes and protectsagainst oxidative damage.

	SULFUR IS THE FUNCTIONAL COMPONENT OF GSH AND OTHER REDOX FACTORS

Free Cys is not used for redox control. It is much too readily oxidized to cystine, the disulfide form, which is visible inthe laboratory as a white precipitate that is formed within hoursafter preparing a solution of Cys. A variety of more stable thiolcompounds are involved in redox regulation. The most abundantis glutathione, an enzymatically synthesized tripeptide in whichCys is linked via peptide bonds to the $gamma$ -carboxyl group of Gluand the $alpha$ -amino group of Gly. In plants glutathione is thoughtto be between 3 and 10 mM, and it is present in the major cellularcompartments. The reduced form of glutathione is often referredto as GSH, whereas the disulfide form is GSSG. The balance betweenforms is overwhelmingly maintained in favor of GSH by the enzymeglutathione reductase, using NADPH as an electron source. Theresult is that the plant cytoplasm, chloroplast stroma, and mitochondrialmatrix are highly buffered in the reducing state. Many intracellularenzymes require reducing conditions for activity, just as theyrequire a specific pH or other properties of their chemical environment.The reason is that Cys residues in proteins can also form disulfidebonds, resulting in a disruption of structure and a loss of activity.There are special cases in which specific disulfide bonds arerequired for formation of tertiary and quaternary structure ina protein, but this is less common, especially for soluble intracellularproteins.

	REDOX FACTORS REGULATE PLANT METABOLIC PATHWAYS

Other factors that use the chemistry of disulfide $left-right-arrow$ dithiol interchange to mediate redox reactions include the proteins thioredoxin,glutaredoxin, and protein disulfide isomerase. These proteinsare nearly ubiquitous and play fundamental roles in many differenttypes of regulation (Fig. 1). One of the first and best examplesof the function of thioredoxin comes from Buchanan (1991). Thedark reactions of CO₂ fixation must be strictly coordinated withthe light reactions of photosynthesis. The coordination mechanismrelies on the reductive activation of specific enzymes by thioredoxin,which is reduced by photosynthetically reduced Fd. New disulfide $left-right-arrow$ dithiol redox regulated processes are being discovered eachyear, which attests to the prevalent roles that sulfur chemistryplays in biology.

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Figure 1. Regulation of metabolism by disulfide $left-right-arrow$ dithiol interchange. The diagram shows how thioredoxin functions as a regulation factor through reduction of a regulatory disulfide on a target enzyme. In the case of C assimilation, the source of electrons for thioredoxin reduction is Fd, reduced via the light reactions of photosynthesis. Thioredoxins also exist in the cytoplasm of plants where NADPH + H⁺ serves as an electron source. Recent evidence shows that thioredoxin has the potential to act as an oxidant mediating the formation of a disulfide bond on a target enzyme (Stewart et al., 1998

). This activity could be important for activation of antioxidant enzymes during oxidative stress.

	GLUTATHIONE IS IMPORTANT IN STRESS MITIGATION

Because of its nucleophilic properties, glutathione serves as the first line of defense against the products of oxygen metabolism,reactive oxygen species, and other electrophilic compounds suchas toxins (herbicides), xenobiotics, and heavy metals (May etal., 1998). When plants encounter reactive oxygen species, glutathioneis a direct source of electrons for stress mitigation by the enzymeglutathione peroxidase or an indirect means to maintain a reducedpool of ascorbate, another antioxidant. Glutathione reacts directlywith toxins in a reaction mediated by glutathione S-transferase.In this way the toxins are inactivated and tagged for transportinto the vacuole and for degradation (Kreuz et al., 1996). Insome plants heavy-metal detoxification is mediated by glutathionederivatives called phytochelatins, which have the general structure( $gamma$ -glutamylcysteine)_nGly (n = 2-11), and by Cys-rich proteinscalled metallothioneins. In both molecules thiol groups serveas the metal ion ligand.

	PLANT SULFUR ASSIMILATION IMPACTS AGRICULTURE AND THE ENVIRONMENT

The preceding discussion illustrates sulfur's essential, general biological role. However, plants also incorporate sulfurinto a wide range of secondary compounds that have an impact,in varied and subtle ways, on our use of plants and on the waythat plants influence the environment. For example, the pungentodor and taste of onions, garlic, and cabbage are caused by sulfur-containingsecondary compounds. The same compounds can impart an objectionableflavor to canola oil, diminishing its commercial value; but theyalso have been attributed to disease prevention in humans (Faheyet al., 1997). Some sulfur-containing phytoalexins such as camalexinmay be important in combating plant pathogens (Zhao et al., 1998).Although sulfur was long thought not to limit plant productivity,the recent restrictions on emissions of sulfurous air pollutants,the ingredients of acid rain, have resulted in sulfur deficiencyin some agricultural areas of the world. Another example is thatsulfur assimilation by plants has been implicated as a potentialfactor in moderating climate. Marine algae are prodigious producersof dimethylsulfoniopropionate, a sulfur-containing analog of betaine(Cooper and Hanson, 1998). Dimethylsulfoniopropionate degradationreleases dimethylsulfide, which volatilizes from the ocean andseeds the formation of clouds in the atmosphere. The global scaleof this process is such that algal growth may actually influenceclimate.

	OVERVIEW OF THE SO₄² ASSIMILATION PROCESS IN PLANTS

Sulfur is available to plants primarily in the form of anionic sulfate (SO₄²) present in soil. It is actively transported into roots and thendistributed, mostly unmetabolized, throughout the plant. SO₄² is a major anionic component of vacuolar sap; therefore, it doesnot necessarily enter the assimilation stream. Gaseous sulfurdioxide (SO₂) is readily absorbed and assimilated by leaves, butit is significant as a nutrient source only in industrial areaswith air pollution. Sulfur is assimilated in one of two oxidationstates. SO₄² can be added to a hydroxyl group of an organic molecule. Thereaction is referred to as sulfation and it is catalyzed by sulfotransferases.By contrast, Cys contains reduced sulfur, which is produced fromSO₄² in a multistep pathway in which eight electrons are added toform sulfide (S²; Reaction 1). The reduction of SO₄² to S² consumes 732 kJ mol¹. By comparison, reduction of nitrate to NH₃ requires 347 kJ mol¹. The pathways of SO₄² assimilation in plants are depicted in Figure 2. The figure showsonly those enzymes that are known with certainty by characterizationof the defined activity of a purified enzyme and through genecloning.

<UP>SO2−4 + ATP + 8 e− + 8 H+ → S2− + 4H2O + AMP + PPi</UP>

<UP>(Reaction 1)</UP>

Cys, the end product of the reductive pathway, is the starting material for production of Met, glutathione, and other metabolitescontaining reduced sulfur.

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Figure 2. Plant sulfur assimilation pathways showing only those enzymes that have been conclusively demonstrated. The top line shows SO₄² activation and reduction. The sulfation pathway is shown in the second line on the left and assimilation of reduced sulfur into Cys on the second line on the right. All enzymes are shown in bold above the reaction arrow, whereas intermediates are shown below the chemical structure or in isolation when the chemical structure is not shown. The R- group in sulfated metabolite refers to the metabolite that is sulfated. Fd indicates the reduced and oxidized forms of Fd.

In higher plants sulfation is a relatively minor fate for sulfur when compared with the reductive pathway. However, in marinealgae, which produce large amounts of sulfated extracellular polysaccharidessuch as agar, sulfation accounts for a much greater proportionof the total assimilated sulfur.

	SO₄² UPTAKE IS MEDIATED BY A FAMILY OF TRANSPORTERS WITH SPECIALIZED FUNCTIONS

The transport of SO₄² occurs across several membrane systems as it enters and is distributed throughout the plant and withincells. Transport across the plasma membrane occurs with protonsat a ratio of 1 SO₄²:3 H⁺ (symport) and is driven by a proton gradient maintained by aproton ATPase. Transport across the tonoplast membrane is mediatedby an unknown mechanism that is driven by the electrical gradientbetween the vacuole sap and cytoplasm. The phosphate/triose phosphatetranslocator of the inner chloroplast membrane or a proton/SO₄² symporter may mediate SO₄² transport into chloroplasts.

The plasma membrane transporters of plants have been characterized (Smith et al., 1997; Takahashi et al., 1997). The sequencesof cDNAs cloned from Stylosanthes hamata, Arabidopsis, soybean,barley, maize, resurrection grass, and Indian mustard showed thatthe plasma membrane transporters of plants are most closely relatedto fungal and animal proton/SO₄² cotransporters. Hydropathy analysis revealed that the plant transportersmay span the membrane 12 times, a structural feature that is typicalof many types of solute symporters.

In most of the species that have been analyzed, SO₄² transporters are encoded by a gene family. The situation in S. hamatais probably typical for most plants. In this species the individualtransporters may have specialized functions, since they differwidely in affinity for SO₄², and they show distinct spatial and regulated patterns of expression(Smith et al., 1997). High-affinity forms with K_m for SO₄² of approximately 9 µM are expressed exclusively in roots, whereasthe lower-affinity form with K_m for SO₄² of approximately 100 µM is expressed principally in leaves butalso in roots. The steady-state level of mRNA for the high-affinityform increases rapidly after sulfur starvation, whereas the lower-affinityform is unresponsive or responds more slowly to changes in externalSO₄² supply. These results imply that the increase in SO₄² transport activity observed in roots of sulfur-starved plantsis due to an increase in the expression of specific transporters.One of the earliest observations of SO₄² transport into roots was that the uptake rate varies in relationto the [SO₄²] of the bathing solution. The results with S. hamata suggestthat this multiphasic behavior may be due to the activities ofseparate transporters with different affinities for SO₄².

What is the function of multiple SO₄² transporters? The expression pattern of the high-affinity type suggests that it mediatesuptake of SO₄² into the plant and is a way to adjust to variation in the externalsulfur supply. By contrast, low-affinity transporters could functionin SO₄² uptake, both from soil and from the apoplast solution that bathesinternal cells. Evidence for specialization of function has beenobtained from analysis of an Arabidopsis SO₄² transporter that is most closely related in sequence to the low-affinitytype from S. hamata (Takahashi et al., 1997). It is expressedexclusively in the vascular parenchyma of roots and leaves andnot in endodermal, cortical, or epidermal cells. The spatial expressionpattern of this low-affinity-type transporter indicates that itmust be responsible for uptake from the internal apoplastic poolof SO₄², not from the soil.

	SO₄² IS AN INERT COMPOUND THAT MUST BE ACTIVATED BEFORE IT CAN BE METABOLIZED

The low reactivity of SO₄² is a barrier to assimilation that is overcome by formation of a phosphate-SO₄²-anhydride bond in the compound APS. The reaction is catalyzedby ATP sulfurylase (Reaction 2) and is the sole entry point formetabolism of SO₄².

<UP>SO2−4 + MgATP &lrarr2; MgPPi + APS(Reaction 2)</UP>

The equilibrium of the adenylation reaction favors the production of SO₄² and ATP, the reverse reaction. The K_eq is 10⁷ M in vitro, and the forward reaction can be measured only ifenzymes that hydrolyze PPi and modify APS are included. Exactlyhow ATP sulfurylase operates in the forward direction in vivohas yet to be determined, since the conditions do not appear tobe in equilibrium. The PPi concentration is approximately 0.3mM in plant cells. Despite the theoretical difficulty, ArabidopsisATP sulfurylase is able to produce APS in vivo under apparentlynonequilibrium conditions, since it is fully able to substitutefor Escherichia coli ATP sulfurylase even though the PPi concentrationin the E. coli cytoplasm is approximately 0.5 mM (Murillo andLeustek, 1995). The Arabidopsis enzyme does not have an intrinsicability to overcome PPi inhibition, which indicates that extrinsicmechanisms in E. coli facilitate the forward operation of plantATP sulfurylase, mechanisms that may also function in plant cells.

There are two ATP sulfurylase isoforms in most plants: a major form localized in plastids and a minor form localized in thecytoplasm. Both enzymes have similar kinetic and structural properties.The isoenzymes are encoded by a gene family, and in Arabidopsisthere are multiple genes for the plastid enzyme. Arabidopsis containsa cytosolic form of ATP sulfurylase, but the corresponding genehas not yet been identified (Rotte, 1998). The plastid enzymeexists in both leaves and roots and is responsible for initiatingthe reductive assimilation of SO₄^2-, since isolated chloroplasts can form Cys from SO₄² (Schürmann and Brunold, 1980). The cytoplasmic form probablyfunctions by generating APS for sulfation reactions.

Whether plant ATP sulfurylase plays a role in regulating sulfur assimilation has been studied by a number of investigators(Logan et al., 1996; Lappartient et al., 1999). In general, theactivity and steady-state mRNA levels increase when plants arestarved for sulfur and decrease when plants are fed reduced formsof sulfur (Cys or glutathione). However, the changes in activityand mRNA, although reproducible, are relatively small; they increaseor decrease by approximately 2-fold or less, and the regulationoccurs mainly in roots. Two publications report the use of transgenicplants to explore whether ATP sulfurylase regulates SO₄² assimilation. Hatzfeld et al. (1998) concluded that it is notrate limiting, based on an analysis of a transgenic tobacco cellculture that overexpresses an Arabidopsis ATP sulfurylase butthat does not show increased sulfur assimilation. By contrast,transgenic Indian mustard lines that overexpress a different ATPsulfurylase isoenzyme from Arabidopsis accumulate glutathioneand show increased resistance to SeO₄² (Pilon-Smits et al., 1999). SeO₄² is a toxic analog of SO₄² that Indian mustard can reduce via the sulfur pathway to a nontoxic,volatile form. The opposite results could be due to differencesin experimental systems.

	THE SULFATION ROUTE FOR ASSIMILATION: SO₄² IS DIRECTLY INCORPORATED INTO PLANT METABOLITES

Plant sulfotransferases have been characterized that catalyze the sulfation of flavonol, desulfoglucosinolate, choline, andgallic acid glucoside (Varin et al., 1997). Sulfotransfer is theterminal step in the biosynthesis of these compounds. The functionof sulfated flavonol and choline is unknown. Glucosinolates arethe compounds responsible for the distinctive taste of mustards.Gallic acid glucoside, also known as turgorin or periodic leafmovement factor, is responsible for triggering nictinastic leafmovement in Mimosa pudica. Sulfation may regulate the processby activating the movement factor. The number of sulfated compoundsin plants is not known. In contrast, sulfation plays a key rolein the production of growth-regulating peptides in animals. However,recently, a sulfated regulator of cell proliferation, phytosulfokine- $alpha$ ,was identified from plants (Matsubayashi et al., 1997).

Several common features of sulfotransferases have emerged from analysis of the enzymes and the encoding cDNAs. The sulfotransferasesare strictly dependent upon the phosphorylated APS derivative,PAPS, as a SO₄² donor, and they all have remarkably high affinity for PAPS. Theyall contain two highly conserved, sulfotransferase signature sequencesthat may be involved in PAPS binding. Last, they are all localizedin the cytoplasm or, in the case of the gallic acid glucosidesulfotransferase, to the inner surface of the plasma membrane.

Enzymes that synthesize PAPS have been described in plants. But how PAPS is supplied to the sulfotransferases is still tobe determined. PAPS is formed through ATP-dependent phosphorylationof the 3 $'$ -hydroxyl group of APS, catalyzed by APS kinase (Reaction3).

<UP>APS + ATP → PAPS + ADP(Reaction 3)</UP>

Cytoplasmic ATP sulfurylase exists in most plants, but a cytoplasmic form of APS kinase has not yet been specifically identified.However, such an enzyme could exist, or at least cannot be ruledout, because in Arabidopsis there are three different genes thatencode APS kinase, and the localization of only one of them hasbeen studied (Lee and Leustek, 1998; Schiffman and Schwenn, 1998).An alternative to in situ, cytoplasmic synthesis of APS and/orPAPS is a system in which the sulfonucleotides are exported fromchloroplasts.

	SO₄² IS REDUCED BEFORE INCORPORATION INTO Cys AND THE REDUCTION PATHWAY BEGINS WITH APS

Eight electrons are required to reduce SO₄² to S². The process occurs through the sequential action of two different enzymes.The exact mechanism in plants has been vigorously debated, resultingin a confusing proliferation of hypotheses (Hell, 1997). Ratherthan reiterating the debate, we discuss here only those enzymesthat are known with certainty. Our intention is to simplify aconfusing topic.

Several lines of evidence conclusively demonstrate that SO₄² reduction begins with APS in plants and eukaryotic algae. Schmidt(1972) identified an enzyme he called APS sulfotransferase, whichhas now been completely purified from a marine red macroalga (Kannoet al., 1996). cDNAs that encode APS sulfotransferase have beencloned from a marine green alga and from several higher plants,most notably Arabidopsis (Bick and Leustek, 1998). That the enzymeencoded by the cloned cDNAs was named APS reductase rather thanAPS sulfotransferase has inadvertently confounded the subject(Gutierrez-Marcos et al., 1996; Setya et al., 1996). Althoughthere were reasonable arguments for the new name, none of thesewere conclusive enough to warrant abridgment of the original name.Here we submit to historical precedent and refer to the enzymeas APS sulfotransferase.

The two names derive from two possible catalytic mechanisms, neither of which has yet been confirmed. As proposed by Schmidt(1972), the sulfotransferase transfers SO₄² from APS to a thiol compound, generating a thiosulfonate. IfGSH were used, the product would be S-sulfoglutathione (Reaction4).

<UP>APS + GSH → GS−SO−3 + H+ + AM(Reaction 4)</UP>

By contrast, a reductase would be expected to transfer electrons from two GSH to APS, generating free sulfite (SO₃²) and GSSG (Reaction 5).

<UP>APS + 2 GSH → SO2−3 + 2 H+ + GSSG + AMP</UP>

<UP>(Reaction 5)</UP>

It is clear from the amino acid sequence of APS sulfotransferase that, if it functions as a sulfotransferase, it belongsto a different class than the enzymes described earlier in relationto sulfation. They do not share any common sequence motifs. Rather,based on its amino acid sequence and its function, APS sulfotransferaseappears to belong to a family of thiol-dependent reductases andthioltransferases.

	GSH PROVIDES ELECTRONS FOR THE FIRST REDUCTION STEP

Mounting evidence indicates that GSH is the most likely in vivo reactant. APS sulfotransferase shows a K_m [GSH] that is consistentwith the in vivo concentration of GSH; it appears to be unableto efficiently use other common biological thiol compounds suchas thioredoxin (Prior et al., 1999), and a domain of the enzymeis a GSH-dependent reductase that functions in a manner similarto that of glutaredoxin (Bick et al., 1998). Although it is functionallyrelated to glutaredoxin, the amino acid sequence of the domainshows greater homology to thioredoxin. The distinction betweenthioredoxin and glutaredoxin is more a matter of the preferredelectron source than of the sequence. For example, only glutaredoxinis able to use GSH. In this respect, it may be of some significancethat glutaredoxin catalyzes reduction of disulfide substratesthrough a thioltransferase mechanism, i.e. the thiol is transferredwith the formation of a glutathione-mixed disulfide intermediate.The analogous reaction for APS sulfotransferase would be the onedepicted in Reaction 4. SO₃² can be produced under the reducing conditions in the chloroplastbecause S-sulfoglutathione is readily reduced nonenzymaticallyin the presence of excess GSH (Reaction 6) (Schürmann and Brunold,1980). Based on these considerations we think it is very likelythat APS sulfotransferase functions as a GSH:APS sulfotransferase.This hypothesis is depicted in Figure 2.

<UP>GS− SO32− + GSH ↔ SO32− + GSSG + H+(Reaction 6)</UP>

	SO₃²⁺ REDUCTASE COMPLETES THE REDUCTION OF SULFUR WITH ELECTRONS FROM REDUCED Fd

In considering the next reduction step it is significant that S-sulfoglutathione and SO₃² could be available in plastids. Plant SO₃² reductase catalyzes the reduction of SO₃² using electrons donated from reduced Fd (Reaction 7). The enzymehas been convincingly demonstrated by purification and cloningof the corresponding gene and cDNA (Bork et al., 1998). SO₃² reductase shows a high affinity for SO₃² (K_m = approximately 10 µM), which would serve well for efficientmetabolism of SO₃².

<UP>SO2−3 + 6 Fdred → S2− + 6 Fdox(Reaction 7)</UP>

An Fd-dependent enzyme that reduces thiosulonate to thiosulfide has been measured in cell lysates, but it has not been purifiedor unambiguously demonstrated. The hypothesis that sulfur is reducedas a thiol-bound form, called the "carrier-bound pathway," hasbeen a tenet of the plant SO₄²-assimilation field. As indicated by the preceding discussion,the carrier-bound pathway need not be invoked because there isconvincing evidence for an efficient SO₃² reductase. However, the existence of thiosulfonate reductaseshould not be dismissed as improbable, especially since therehas not been a concerted effort to demonstrate it conclusively.Cloning of a thiosulfonate reductase cDNA would be definitive.It is our opinion that an excellent opportunity exists for devisinga cloning strategy based on functional complementation of an E.coli SO₃² reductase mutant if the strain is engineered to express plantFd and NADPH:Fd oxidoreductase.

	APS SULFOTRANSFERASE MAY BE A REGULATION POINT IN THE SULFUR-REDUCTION PATHWAY

APS sulfotransferase is encoded by a gene family in Arabidopsis (Bick and Leustek, 1998), all of whose members appear to encodeplastid-localized enzymes. APS sulfotransferase is localized onlyin plastids and not in other cellular compartments (Rotte, 1998).No specialization of function has yet been ascribed to the APSsulfotransferase isoenzymes. SO₃² reductase is also plastid localized. In Arabidopsis there maybe a single gene encoding this enzyme (Bork et al., 1998).

There is a great deal of evidence indicating that APS sulfotransferase is a prime regulation point in SO₄² assimilation (Brunold and Rennenberg, 1997). The activity ofthis enzyme changes rapidly in a variety of plant species aftersulfur starvation, exposure to reduced sulfur compounds, heavy-metalstress, or other stresses. Heavy metals induce the synthesis ofphytochelatins, and high concentrations of metal ions significantlyincrease the demand for Cys. Recent studies indicate that onepotential mechanism for regulating APS sulfotransferase activitymay involve changes in the steady-state mRNA level. Sulfur starvation(Gutierrez-Marcos et al., 1996; Takahashi et al., 1997) and heavy-metaltreatment (Heiss et al., 1999; Lee and Leustek, 1999) induce theaccumulation of APS sulfotransferase mRNA, but the response islimited to roots. By contrast, SO₃² reductase does not appear to be appreciably regulated at themRNA level (Bork et al., 1998). The extent to which the regulationof mRNA abundance is responsible for changes in APS sulfotransferaseactivity has not yet been adequately explored.

	INCORPORATION OF REDUCED SULFUR INTO Cys: PROTEIN-PROTEIN INTERACTIONS MAY REGULATE THE PROCESS

The incorporation of S² into Cys is the last step in reductive SO₄² assimilation. The reaction is catalyzed by O-acetylserine(thiol)lyasefrom S² and OAS (Reaction 8). The synthesis of OAS is catalyzed by Seracetyltransferase (Reaction 9).

<UP>OAS + S2− → Cys + acetate(Reaction 8)</UP>

<UP>Ser + acetylCoA → OAS + CoA(Reaction 9)</UP>

Ser acetyltransferase and OAS(thiol)lyase exist in an enzyme complex known as Cys synthase. The stability of the complexis affected by substrates (OAS disrupts it and S² stabilizes it), and it appears to form through specific protein-proteininteractions (Bogdanova and Hell, 1997). Yet, the free form ofeach enzyme has catalytic activity, and the complex is not requiredfor channeling of OAS (Droux et al., 1998). Moreover, in chloroplaststhe ratio of OAS(thiol)lyase to Ser acetyltransferase is 300:1(Droux et al., 1998, and refs. therein); therefore, only a fractionof the total OAS(thiol)lyase can be associated in the complex.

One clue to the function of the complex is that association with OAS(thiol)lyase changes the kinetic behavior of Ser acetyltransferasefrom the Michaelis-Menten type to positive cooperativity withrespect to its substrates, Ser and acetyl-CoA (Droux et al., 1998).This suggests that OAS (thiol)lyase functions as a regulatorysubunit that regulates Ser acetyltransferase in response to OASand S². Positive cooperativity is a form of allosteric regulation inwhich the velocity of a bisubstrate enzyme is highly sensitiveto small changes in substrate concentration. One can think ofthe enzyme as having a hair-trigger control mechanism. The ideais appealing because Cys synthesis requires coordination of twoconverging pathways. If there is insufficient S² resulting from low activity of SO₄² reduction, the concentration of OAS will increase, causing dissolutionof the Cys synthase complex. By contrast, overactivity of SO₄² reduction results in overabundance of S² and a shortage of OAS, a condition that would stabilize the complex.Ser acetyltransferase activity would be regulated, its velocitybecoming less or more sensitive to its own substrates. Anotherpossible form of regulation is an increase in the steady-statemRNA level for the plastid form of Ser acetyltransferase aftersulfur starvation (Takahashi et al., 1997; Noji et al., 1998).Unlike the earlier steps in the pathway in which mRNA regulationoccurs primarily in roots, plastid Ser acetyltransferase mRNAincreases primarily in leaves. A third possible regulation mechanismis the feedback inhibition of Ser acetyltransferase by Cys. However,only the cytosolic isoform appears to be regulated in this way(Noji et al., 1998).

Ser acetyltransferase and OAS(thiol)lyase are the only sulfur assimilation enzymes localized in three compartments: the plastids,cytosol, and mitochondria. cDNAs have been cloned from a rangeof plant species encoding all of the different isoenzymes (Saitoet al., 1994). The multifarious localization of Cys synthase enzymespresents a problem in that only plastids contain the full complementof enzymes needed for SO₄² reduction. It may be that S² is exported from plastids to supply the substrate required bycytosolic and mitochondrial Cys synthases. Evidence for a specializationof function was obtained by analysis of the cytosolic form ofOAS(thiol)lyase from Arabidopsis. It is expressed predominantlyin roots, in the vascular parenchyma, and in cortical cells (Gotoret al., 1997). Expression in leaves is concentrated in trichomes.Gotor et al. (1997) noted that the toxic heavy-metal Cd is knownto accumulate in trichomes of exposed plants, so it could be thatthe cytosolic OAS(thiol)lyase has a specialized role, supplyingCys for a detoxification mechanism.

	NEGATIVE AND POSITIVE SIGNALS REGULATE SO₄² ASSIMILATION

From the preceding discussion it is evident that SO₄² reduction and assimilation into Cys is regulated in plants by a rangeof mechanisms that include substrate availability, modulationof enzyme activity, and gene expression. Since the exclusive functionof SO₄² reduction is to produce Cys, future studies must concentrateon the question of how the range of regulation mechanisms forindividual enzymes is coordinated. Current thinking focuses onboth negative and positive signals. It has been known for sometime that reduced sulfur compounds such as Cys and glutathione,when applied to plants, repress the activity of the sulfur-assimilationenzymes. Conversely, SO₄² starvation induces the activity of certain enzymes. With theavailability of DNA probes it was discovered that the steady-statelevels of mRNA for SO₄² transporter, ATP sulfurylase, and APS sulfotransferase declineafter the application of glutathione or Cys to plant roots (Smithet al., 1997; Lappartient et al., 1999; Lee and Leustek, 1999).In contrast, SO₄² starvation increases the steady-state level of mRNA for theseproteins. Whether these responses are due to transcriptional orposttranscriptional mechanisms is not yet known.

One form of reduced sulfur, glutathione, could act as an endogenous signal because it is known to be transported through thephloem of plants and its level in phloem sap is markedly reducedafter short-term sulfur starvation. Further support for this hypothesiscomes from the "split-root" experiments of Lappartient et al.(1999) in which a portion of the root system was sulfur starved.In another portion of the root system fed normal levels of sulfate,the steady-state mRNA level and activity for SO₄² transporter and ATP sulfurylase increased at precisely the timethat the level of transported glutathione declined. The implicationis that glutathione acts as a negative signal or repressor. Positiveregulation could be a derepression phenomenon caused by a decreasein repressor.

Recent experiments indicate, however, that a positive signal may also exist. When OAS was fed to roots of barley, the steady-statemRNA level for the high-affinity transporter increased coordinatelywith SO₄²-transport activity (Smith et al., 1997). The response was morerapid than when plants were starved for sulfur, but the magnitudeof the increase was smaller. OAS feeding also caused the levelof reduced sulfur compounds to increase, possibly explaining whythe OAS-induced increase in transporter expression was attenuatedcompared with SO₄² starvation. Regulation is probably a balance between negativeand positive signals. Other publications have noted that OAS stimulatesSO₄²-reduction enzymes (Smith et al., 1997, and refs. therein). OASis an appealing candidate as a positive regulator. It is knownto influence the Cys synthase complex. A second effect on theexpression of SO₄²-reduction enzymes could provide a means for coordination of theentire pathway.

	FOOTNOTES

¹ This work was supported by the U.S. National Science Foundation (grant nos. IBN 9601146 and MCB 9728661 to T.L.), by Grants-in-Aidfor Scientific Research from the Ministry of Education, Science,Sports and Culture, Japan, and by the Research for the FutureProgram (grant no. 96I00302) from the Japan Society for the Promotionof Science (to K.S.).
^* Corresponding author; e-mail leustek{at}aesop.rutgers.edu; fax 1-732-932-0312.

Received March 2, 1999; accepted March 23, 1999.

ABBREVIATIONS

Abbreviations: APS, 5 $'$ -adenylylsulfate. OAS, O-acetylserine. PAPS, 3 $'$ -phosphoadenosine-5 $'$ -phosphosulfate.

	LITERATURE CITED

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