Purified gamma -Glutamyl Transpeptidases from Tomato Exhibit High Affinity for Glutathione and Glutathione S-Conjugates

doi:10.1104/pp.122.4.1417

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Purified $gamma$ -Glutamyl Transpeptidases from Tomato Exhibit High Affinity for Glutathione and Glutathione S-Conjugates¹

Melinda Neal Martin² ^* and Janet P. Slovin

Climate Stress Laboratory, Beltsville Agricultural Research Center, Agricultural Research Service, United States Department of Agriculture, 10300 Baltimore Avenue, Beltsville, Maryland 20705

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

$gamma$ -Glutamyl transpeptidases ( $gamma$ GTases) are the only enzymes known to hydrolyze the unique N-terminal amide bonds of reducedglutathione ( $gamma$ -L-glutamyl-cysteinyl-glycine), oxidized glutathione,and glutathione S-conjugates. Two $gamma$ GTases (I and II) with K_m valuesfor glutathione of 110 and 90 µM were purified 2,977-fold and2,152-fold, respectively, from ripe tomato (Lycopersicon esculentum)pericarp. Both enzymes also hydrolyze dipeptides and other tripeptideswith N-terminal, $gamma$ -linked Glu and the artificial substrates $gamma$ -L-glutamyl-p-nitroanilideand $gamma$ -L-glutamyl(7-amido-4-methylcoumarin). They transfer theglutamyl moiety to water or acceptor amino acids, including L-Met,L-Phe, L-Trp, L-Ala, or the ethylene precursor 1-aminocyclopropane-1-carboxylicacid. $gamma$ GTase I and II were released from a wall and membrane fractionof a tomato fruit extract with 1.0 M NaCl, suggesting that theyare peripheral membrane proteins. They were further purified byacetone precipitation, Dye Matrex Green A affinity chromatography,and hydrophobic interaction chromatography. The two $gamma$ GTases wereresolved by concanavalin A (Con A) affinity chromatography, indicatingthat they are differentially glycosylated. The native and SDS-denaturedforms of both enzymes showed molecular masses of 43kD.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

$gamma$ -Glutamyl transpeptidases ( $gamma$ GTases) ([5-L-glutamyl]-peptide:amino acid 5-glutamyl transferase; EC 2.3.2.2) catalyze thehydrolysis of the uniquely linked N-terminal Glu from the reducedglutathione (GSH) ( $gamma$ -L-glutamyl-L-cysteinyl-glycine), oxidizedglutathione (GSSG), and glutathione S-conjugates, as well as froma number of dipeptides and other tripeptides having an N-terminal $gamma$ -linked Glu. The Glu moiety is transferred to either water (hydrolysis)or to an acceptor amino acid, dipeptide, or tripeptide, includingGSH (transpeptidation), resulting in a new amide bond with anN-terminal, $gamma$ -linkedGlu.

In mammals, $gamma$ GTases are well characterized and have several physiologically and pharmaco-toxicologically important functions.First, they initiate degradation of GSH to release Cys, whichis the primary stored and transported form of sulfur. GSH hydrolysisoccurs primarily on the outer surface of cell membranes in organsthat secrete a large amount of GSH; the component amino acidsare salvaged and transported back into the cells (Meister, 1988,1989). Knock-out mice lacking a functional $gamma$ GTase died of Cysstarvation unless their diets were supplemented with Cys (Liebermanet al., 1996). The $gamma$ -glutamyl peptides resulting from the transpeptidationreaction may enter the " $gamma$ -glutamyl cycle," where they are alsohydrolyzed and the amino acids are salvaged (Meister, 1988, 1989).Cys-Gly dipeptidases complete the hydrolysis of GSH (Habib etal., 1998). Second, $gamma$ GTases are part of the pathway for detoxificationand elimination of many xenobiotics and pharmaceuticals (Meister,1988; Ishikawa, 1992). These compounds are first conjugated toGSH by glutathione S-transferases, which reduces their reactivity,increases their polarity, and tags them for transport or excretionby the ATP-binding cassette class of transporters (Ishikawa, 1992). $gamma$ GTases initiate degradation of the excreted conjugates by hydrolyzingthe $gamma$ -Glu moiety (Meister, 1988). Finally, $gamma$ GTases are part ofa pathway for sequestering, transporting, and modulating the activityof hormones, neurotransmitters, and other biologically activecompounds, including hepoxilins, leukotrienes, and prostaglandins(Meister, 1988; Pace-Asciak et al., 1990; Ishikawa, 1992; Carteret al., 1997). As with xenobiotics, the pathway involves glutathioneS-conjugation, transport, and, finally, further metabolism ofthe conjugate. For conjugates of some hormones, removal of theN-terminal Glu by a highly specific $gamma$ GTase results in 100-foldactivation, while for other hormone conjugates it results in inactivation(Ishikawa, 1992; Carter et al., 1997).

Plant $gamma$ GTases are poorly characterized, and it is not known whether they serve the same functions as in animals. GSH is reportedto be the major form in which reduced sulfur (Cys) is stored andtransported in plants, but there are conflicting data as to thesequence of reactions leading to Cys release from GSH. $gamma$ -Glu-Cyswas identified as an intermediate in the degradation of [³⁵S]GSH by tobacco (Steinkamp and Rennenberg, 1985). The authorsproposed that a carboxypeptidase initiates hydrolysis of GSH atthe C terminus, followed by hydrolysis of $gamma$ -Glu-Cys by a $gamma$ GTaseor the " $gamma$ -glutamyl cycle" enzymes ( $gamma$ -glutamylcyclotransferaseand oxo-prolinase). Cys-Gly is found in soybeans, suggesting thatGSH hydrolysis is catalyzed by the sequential action of a $gamma$ GTaseand a Cys-Gly dipeptidase (Bergmann and Rennenberg, 1993). Thesequence of reactions leading to hydrolysis of GSH in plants maybe species specific. Only Cys-Gly has been identified as an intermediatein the degradation of GSH and GSSG by animals (Meister, 1988).

Plants also form glutathione S-conjugates of many herbicides and pesticides (Marrs, 1996). Some of these conjugates are transportedto the vacuole by ATP-binding cassette transporters (Martinoiaet al., 1993; Gaillard et al., 1994; Li et al., 1995; Rea et al.,1998). In the vacuole, conjugates undergo modification, whichmay begin with the cleavage of Glu and Gly (Lamoureux and Rusness,1981, 1983, 1993; Lamoureux et al., 1991). At least one endogenousplant compound, the anthocyanin cyanidin 3-glucoside, appearsto be targeted to the vacuole by the same mechanism (Marrs etal., 1995; Marrs 1996; Alfenito et al., 1998). The glutathioneS-transferases (Marrs, 1996) and glutathione S-conjugate transporters(Rea et al., 1998) have been at least partially characterized.The enzymes responsible for subsequent modifications of theseconjugates have not beencharacterized.

$gamma$ GTases may have an additional role in plants for which there is no analogy in animals. Numerous dipeptides with an N-terminal $gamma$ -linked Glu have been isolated from plant tissues, most oftenfrom storage tissues such as seeds or bulbs. Examples includeGlu $gamma$ -linked to Met, methionine sulfoxide, Leu, Tyr, Asp, andPhe in legumes (Thompson et al., 1962a); Phe, Asp, and Tyr insoybeans (Ishikawa et al., 1967); Asp, Glu, and Tyr in asparagus(Kasai et al., 1982); 2-methylenecyclopropyl-alanine in ackeefruit (Kean and Hare, 1980); D-Ala and homoserine in pea seedlings(Kawasaki et al., 1982); and $beta$ -cyanoalanine in vetch seeds (Ressleret al., 1969). In Allium species, at least 18 $gamma$ -glutamyl peptidesof sulfur compounds such as alk(en)yl-cysteine sulfoxides havebeen identified (Lancaster et al., 1989; Lancaster and Shaw, 1989,1991). $gamma$ GTases are the only enzymes known to catalyze the formationof the N-terminal $gamma$ -linked amide bond with Glu. One exceptionis $gamma$ -glutamyl cysteine synthetase, which catalyzes the first stepin GSH synthesis and uses only Cys as the acceptor amino acid.Likewise, $gamma$ GTase and $gamma$ -glutamyl cyclotransferase (operating inthe $gamma$ -glutamyl cycle) are the only enzymes known to hydrolyzethe unique N-terminal amide bond in thesedipeptides.

$gamma$ GTases are widely distributed in monocots and dicots, and both constitutive and developmentally regulated activities havebeen reported (Thompson et al., 1962b; Goore and Thompson, 1967;Kean and Hare, 1980; Kasai et al., 1982; Kawasaki et al., 1982;Steinkamp and Rennenberg, 1984; Lancaster and Shaw, 1994; Martinet al., 1995; M. Martin, unpublished results). Activity is particularlyhigh in seeds and storage tissues (Lancaster and Shaw, 1994; Martinet al., 1995; Martin and Slovin, 1996; M. Martin, unpublishedresults). In contrast, other activities that might have a rolein GSH and glutathione S-conjugate hydrolysis (GSH carboxypeptidase,Cys-Gly dipeptidase, and the " $gamma$ -glutamyl cycle" enzymes $gamma$ -glutamylcyclotransferaseand oxo-prolinase) have been reported in only one or two planttissues (Rennenberg et al., 1981; Steinkamp et al., 1984, 1985).In plants, a $gamma$ -glutamyl cycle has not been established. A vacuolarcarboxypeptidase capable of initiating hydrolysis of glutathioneS-conjugates from the carboxy terminus was recently isolated frombarley (Wolf et al., 1996).

We have previously reported the identification of a $gamma$ GTase in tomato (Lycopersicon esculentum) fruit and seeds. This enzymeuses the precursor to the plant hormone ethylene, 1-aminocyclopropane-1-carboxylicacid [ACC], as an acceptor amino acid (Martin et al., 1995). Wemeasured a high level of this activity in tomato seeds throughoutdevelopment and dehydration, and an increase in the activity inthe pericarp and other maternal tissues during the course of fruitdevelopment and ripening (Martin et al., 1995). We report theisolation from the pericarp of ripe tomato fruit of several $gamma$ GTasesthat differ in $gamma$ -glutamyl donor specificity. We also describethe purification and characterization of two of these enzymes,both of which exhibit high affinity for GSH, GSSG, and glutathioneS-conjugates.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Plant Material

Red ripe fruit from tomato (Lycopersicon esculentum Mill cv Ailsa Craig) were used. Plants were grown in a greenhouse andreceived supplemental lighting duringwinter.

Radiometric Measurement of Transpeptidase Activity

The assays were performed in 0.5-mL microcentrifuge tubes and contained in a volume of 50 µL, enzyme, 100 mM Tris-Cl, pH 8.0,2 mM GSH, 5 mM ACC, and 3.75 kBq [2,3-¹⁴C]ACC per assay. [2,3-¹⁴C]ACC with a specific activity of 1.87 GBq/mmol was synthesizedby the Commissariat a L'Energie Atomique, France. The reactionswere initiated with GSH, incubated for 15 to 60 min at 30°C, andterminated by the addition of 50 µL of absolute ethanol or byboiling. Five microliters of each assay mix was spotted on a laneof a 10 × 20 cm HPTLC-GHLF³ normal phase silica TLC plate (Analtech, Newark, DE). [¹⁴C]ACC and the product, [¹⁴C]-1-( $gamma$ -glutamyl)cyclopropane-1-carboxylic acid ([¹⁴C]-GACC), were resolved using a solvent system of 1-propanol:ammoniumhydroxide (6:4, v/v). Prior to chromatography, assays containingcrude protein extracts were centrifuged for 5 min at 13,000g topellet protein and other debris. Products and substrate were detectedand quantified using a radioisotope image acquisition and analysissystem (Ambis model 1000, Scanalytics, Billericka, MA). Whereindicated, other $gamma$ -glutamyl donors were substituted for GSH, andother amino acids were substituted for ACC or added as competitiveacceptors. One unit of enzyme activity was defined as the amountcatalyzing the formation of 1 nmol of GACC perminute.

Spectrophotometric Measurement of $gamma$ -Glutamyl-p-Nitroanilide ( $gamma$ -GPNA) Hydrolysis

The assays were performed at 30°C in 96-well microtiter plates. Each well contained in a volume of 100 µL, 100 mM Tris-Cl,pH 8.0, enzyme, 5 mM $gamma$ -GPNA, and 5 mM ACC. Assays were initiatedwith $gamma$ -GPNA and activity was measured spectrophotometrically asthe formation of p-nitroaniline at 405 nm using a microplate reader(Thermomax, Molecular Devices, Menlo Park, CA). One unit of enzymeactivity was defined as the amount catalyzing the formation of1 nmol p-nitroanilide perminute.

Purification of the $gamma$ GTase

Six kilograms of pericarp and epidermis was obtained from tomato fruit harvested at the red-ripe stage. All subsequent stepswere performed at 5°C. The tissue was ground for 30 s in a blenderin aliquots of 200 g with 1 g of Polyclar AT powder (GAF, NewYork) and 400 mL of buffer A, which contained 100 mM Tris-Cl,pH 8.0, 1 mM benzamindine, 1 mM 6-amino-n-hexanoic acid, 1 mMphenylmethylsulfonyl fluoride (PMSF), 250 µM N- $alpha$ -p-tosyl-L-argininemethyl ester, 250 µM N-tosyl-L-phenylalanine chloromethyl ketone,3 µM pepstatin, and 1 µM leupeptin. The crude extract was centrifugedfor 20 min at 7,000g, and the pellet was recovered and reextractedwith 2 L of buffer A. The pellet was again recovered and extractedtwice with 3 L of buffer A plus 1.0 M NaCl and 5 mM EDTA. Thesupernatants from the two extractions with NaCl were filteredthrough Miracloth (Calbiochem, La Jolla, CA) to remove any remainingdebris. Acetone (chilled to $-$ 20°C) was added to 75% (v/v).

After 6 h, precipitated proteins were pelleted by centrifugation for 15 min at 7,000g. The pellet was dissolved in buffercontaining 100 mM Tris-Cl, pH 8.0, 5 mM EDTA, 1 M NaCl, 1 mM benzamidine,1 mM 6-amino-n-hexanoic acid, 3 µM pepstatin, and 1 µM leupeptin,and centrifuged for 1 h at 150,000g. The 150,000g supernatantwas diluted 1:4 with 100 mM Tris-Cl, pH 8.0, to a final NaCl concentrationof 0.25 M, and applied at a flow rate of 0.5 mL min¹ to a Dye-Matrex Green A column (1.0 × 30 cm, Amicon, Beverly,MA) that had been equilibrated in 100 mM Tris-Cl, pH 8.0 plus0.25 M NaCl (buffer B). This and subsequent columns were interfacedwith a FPLC system (Pharmacia, Piscataway, NJ). The column waswashed with buffer B, followed by a gradient of 0.25 to 0.4 MNaCl in 100 mM Tris-Cl, pH 8.0, which removed most of the boundprotein. The $gamma$ GTase activity was then eluted with a 0.4 to 2.0M gradient of NaCl. Active fractions were pooled, ammonium sulfatewas added to a concentration of 1.7 M, and the protein was loadedat a flow rate of 0.5 mL min¹ onto a Phenyl Superose HR 5/5 column (Pharmacia) equilibratedwith 100 mM Tris-Cl, pH 8.0, containing 1.7 M ammonium sulfate.The enzyme was eluted with a 1.7 to 1.0 M gradient of ammoniumsulfate in 100 mM Tris-Cl, pH 8.0. Fractions with activity werepooled, concentrated, and desalted using concentrators (Centricon10, Amicon). They were then loaded at a flow rate of 0.25 mL min¹ onto a 0.5- × 19-cm Con A column (Pharmacia) equilibrated inbuffer C (100 mM Tris-Cl, pH 8.0, plus 0.5 M NaCl). After washingwith buffer C, the column was washed with a gradient of 0 to 15mM Glc in buffer C followed by a gradient of 0 to 50 mM methyl- $alpha$ -D-glucopyranosidein buffer C. After elution from this column, active fractionswere used immediately or stored at $-$ 80°C. The $gamma$ GTases eluted fromthe Con A column were used for all furthercharacterization.

All stages in the purification were monitored by both the hydrolysis of $gamma$ -GPNA and transpeptidation to form GACC. Proteinconcentrations were determined using a Bio-Rad (Richmond, CA)protein assay kit or a protein-gold reagent (Integrated SeparationSystems, Natick, MA). Bovine serum albumin (BSA) was used as astandard for both assays. Protein purity was determined by one-dimensionalSDS-PAGE (8%-25% gradient of acrylamide) using the Pharmacia PhastSystem. The 10-kD protein ladder from Gibco-BRL (Gaithersburg,MD) was used as standard. Proteins were detected by silver stainingusing a modified Phast System protocol. Identical gels or halvesof gels were blotted to a polyvinylidene difluoride (PVDF) membrane(Bio-Rad) using the Phast System, probed with a Con A-horseradishperoxidase conjugate (Sigma, St. Louis), and visualized usingan ImmunoPure Metal Enhanced DAB Substrate Kit (Pierce, Rockford,IL). Molecular masses were estimated by gel filtration on twoPharmacia Superdex 75 HR 10/10 columns connected in series. Thecolumns were calibrated with proteins of known molecularmass.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Purification of $gamma$ GTases

Red-ripe pericarp was used for the purification of $gamma$ GTases because we previously showed that $gamma$ GTase activity increased inall maternal tissues as the tomato fruit developed and ripened(Martin et al., 1995). Because mammals have some $gamma$ GTases withvery broad specificity and others with very narrow specificityfor their $gamma$ -Glu donor, we monitored the progress of the purificationby two methods using two different $gamma$ -Glu donors. The spectrophotometricassay measures p-nitroaniline formed by the hydrolysis of theartificial substrate $gamma$ -GPNA (Pennickx and Jasper, 1985). The radiometrictranspeptidase assay measures transfer of the $gamma$ -glutamyl moietyfrom the donor (GSH) to [¹⁴C]ACC to form [¹⁴C]GACC. Representative results are summarized in Table I forpurification of two $gamma$ GTases from 6 kg of pericarp. $gamma$ GTase I waspurified 2,977-fold to a specific activity of 24,028, and $gamma$ GTaseII was purified 2,152-fold to a specific activity of 17,366, asmeasured by the hydrolysis of $gamma$ -GPNA.

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Table I. Purification of two $gamma$ GTases with different affinities for Con A from ripe tomato pericarp

After centrifugation of the crude tomato extract at low speed, 100% of the activity measured by both methods was recoveredin the pellet. Activities measured by both methods were quantitativelyreleased from the pellet by washing with buffer containing either1.0 M NaCl or 1.0 KCl. Lower concentrations of salt failed torelease as much as 50% of both activities from the pellet. The $gamma$ GTases released by NaCl were concentrated by precipitation with75% (v/v) acetone. Ultracentrifugation was used to remove remainingmembranes and particulate material from the resuspended acetonepellet. Nearly 70% of the activity measured by the transpeptidaseassay, but less than 20% of the $gamma$ -GPNA-hydrolyzing activity, pelletedat this stage. As a result, the ratio of $gamma$ -GPNA-hydrolyzing totranspeptidase activities in the soluble fraction increased from0.75 to 2.6. Only the soluble $gamma$ GTase activity was applied to aDye-Matrex Green A column and further purified; elution from thiscolumn with 0.8 to 1.2 M NaCl resulted in a 1,875-fold overallpurification, as measured by hydrolysis of $gamma$ -GPNA. The $gamma$ GTaseexhibited no requirement for ATP/ADP, pyridine nucleotides, orcoenzyme A as cofactors, substrates, or activators (Martin etal., 1995). Thus, we have no explanation for the high-affinitybinding of the $gamma$ GTase to Dye-Matrex Green A and other dye-ligandcolumns, including Amicon Dye-Matrex Red A and Blue A and CibacronBlue 3GA-agarose (Sigma; M. Martin, unpublishedresults).

The final step in the purification protocol, chromatography on a Con A affinity matrix, resolved the $gamma$ GTase activity intothree fractions. One fraction, containing about 30% of the $gamma$ -GPNA-hydrolyzingactivity, failed to bind to Con A. This $gamma$ GTase was not furthercharacterized. Two fractions, designated $gamma$ GTase I and II, boundto the column and were eluted as sharp peaks with Glc and methyl- $alpha$ -D-glucopyranoside,respectively. Overall, recovery of activity ( $gamma$ GTase I plus II)as measured by hydrolysis of $gamma$ -GPNA was 18% and by the transpeptidaseassay was 4%.

Properties of the Purified $gamma$ GTases

$gamma$ GTase I and II and the $gamma$ GTase that did not bind Con A appeared as single 43-kD bands when visualized by silver staining afterSDS-PAGE (Fig. 1, lanes 1-3). Further manipulation of the purified $gamma$ GTases often resulted in the appearance of a 27-kD band (Fig.1, lanes 4 and 5), that may be the result of proteolysis. Both $gamma$ GTase I and II and the 27-kD peptide reacted with the Con A-horseradishperoxidase conjugate, confirming that they are glycosylated. $gamma$ GTaseI and II exhibited identical native molecular masses of 43 kDby gel filtration chromatography on Superdex 75 columns, indicatingthat each is monomeric.

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Figure 1. SDS-PAGE of the purified $gamma$ GTases visualized by silver staining. Lane 1, Purified $gamma$ GTase I after Con A; lane 2, purified $gamma$ GTase II after Con A; lane 3, the $gamma$ GTase activity not binding to Con A; lane 4, purified $gamma$ GTase I after Superdex 75; and lane 5, purified $gamma$ GTase II after Superdex 75. Molecular masses in kD of protein standards are designated at the left.

$gamma$ GTase I and II exhibited almost identical pH profiles (Fig. 2). Both enzymes had very broad pH optima between 7.0 and 9.0as measured by either the hydrolysis of $gamma$ -GPNA or the transferof Glu from GSH to ACC. However, the effect of pH on the activitymeasured by the two methods was notable. The rate of transpeptidationby both $gamma$ GTase I and II was near zero between pH 5.5 and 6.5.In contrast, the rate of hydrolysis of $gamma$ -GPNA by both $gamma$ GTase Iand II was only 2- to 3-fold lower between pH 5.5 and 6.5 thanat the optima. At pH 10, the rates of transpeptidation of Gluto form GACC and the rate of hydrolysis of $gamma$ -GPNA were nearlyequal.

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Figure 2. $gamma$ GTase I (A) and $gamma$ GTase II (B) have similar pH profiles for hydrolysis of $gamma$ -GPNA ( $black-triangle$ ) and for transpeptidation using GSH as the donor (

). Assays were performed as described in "Materials and Methods" in several buffers over their operating pH range. These included MES, MOPS, POPSO, Tris, AMPSO, and CAPSO. Data using only MES, Tris, AMPSO, and CAPSO are shown because activities were 2-fold lower in MOPS or POPSO than in Tris at the same pH values.

Substrate Specificity

$gamma$ GTase I and II exhibited very broad and similar specificities for the $gamma$ -glutamyl donor substrate in the transpeptidationreaction. For both activities, the rates of transpeptidation werevery similar for GSH, GSSG, and several S-substituted analogsof GSH. Activities, expressed as a percentage of the rate withGSH, are shown using 0.4 and 2 mM donor peptide (Table II). $gamma$ GTaseII, but not $gamma$ GTase I, was inhibited by S-substituted analogs ofGSH at 2 mM. Several dipeptides with N-terminal $gamma$ -linked Glu,including $gamma$ -Glu-Cys, also served as donors for both $gamma$ GTase I andII (Table III). The rates of reaction for all dipeptides testedexcept $gamma$ -Glu-Cys and $gamma$ -Glu-Trp were lower than for GSH, and theK_m values were higher (data not shown). Several of the dipeptideswere less effective donors for $gamma$ GTase II than for $gamma$ GTase I. Forboth $gamma$ GTase I and II, the reaction rates were consistently lowerwith the artificial substrates routinely employed in spectrophotometric,fluorimetric, or histochemical assays of animal $gamma$ GTases than withGSH (Table III). 4-Methoxy- $beta$ -napthylamide exhibited a low rateof reaction with $gamma$ GTase I and II when $gamma$ -linked to Glu, and noreaction when $alpha$ -linked. Dipeptides and tripeptides lacking theN-terminal $gamma$ -linked Glu failed to function as donors (data notshown).

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Table II. S-Substituted analogs of GSH serve as donors for both $gamma$ GTase I and II
Radiometric transpeptidase assays were performed as described in "Materials and Methods" using GSH or other donor peptide concentrations of 0.4 or 2 mM. The acceptor was 5 mM [¹⁴C]ACC. The specific activity of $gamma$ GTase I was 13,200 nmol min¹ mg¹ with both 0.4 and 2 mM GSH. The specific activity of $gamma$ GTase II was 8080 nmol min¹ mg¹ with both 0.4 and 2 mM GSH. Values are the mean ± SD of three to six measurements and are representative of results obtained in three independent experiments.

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Table III. Several dipeptides with N-terminal $gamma$ -L-glutamic acid serve as donors for $gamma$ GTase I and II
Radiometric transpeptidase assays were performed as described in "Materials and Methods" using 0.4 or 2 mM GSH or other donor. [¹⁴C]ACC was the acceptor. Concentrations of 2 mM but not 0.4 mM were saturating for all dipeptides but not for the artificial substrates. All amino acids are L-isomers except where otherwise indicated. Values are the mean ± SD of three to six data points and are representative of results obtained in three independent experiments. The specific activity of $gamma$ GTase I was 13,100 nmol min¹ mg¹ with both 0.4 and 2 mM GSH. The specific activity of $gamma$ GTase II was 7,990 nmol min¹ mg¹ with both 0.4 and 2 mM GSH.

ACC, the acceptor in the transpeptidase assay, is a neutral, optically inactive amino acid. Some L-amino acids also serveas acceptors for $gamma$ GTase I and II in the transpeptidation reaction.In transpeptidation reactions containing [¹⁴C]L-amino acids instead of [¹⁴C]ACC as the acceptor, radiolabeled products were formed fromMet, Trp, Phe, Ala, and Asp, but not from the ACC analog $alpha$ -aminoisobutyricacid (Table IV). In every case, the percentage of L-amino acidconverted to the $gamma$ -Glu-amino acid was lower than the percent ofACC converted to GACC. [¹⁴C]Dipeptides, tripeptides, and D-amino acids are not commerciallyavailable. However, two lines of evidence indicate that both $gamma$ GTaseI and II use several other L-amino acids, dipeptides, and tripeptidesas acceptors, but use the corresponding D-isomer poorly or norat all. First, L-amino acids and the L-isomers of several dipeptidesand tripeptides inhibited the [¹⁴C]ACC-dependent transpeptidation reaction (Table V and TableVI). L-Amino acids at concentrations equal to the ACC concentration(1 mM) inhibited both $gamma$ GTase I and II between 7% and 57% (TableV), suggesting that they compete with ACC as acceptors. In contrast,D-amino acids at concentrations 4-fold higher than the ACC concentrationwere poor inhibitors; the ACC-dependent $gamma$ GTase I reactions wereinhibited between 0% to 22%, and the $gamma$ GTase II reactions between0% and 33% (Table V). Both dipeptides and tripeptides at a concentrationequal to the ACC concentration inhibited $gamma$ GTase II between 20%and 95%, but only dipeptides significantly inhibited $gamma$ GTase I(Table VI). Greater than 50% inhibition of the ACC-dependent reactionsuggests that Cys-Gly and Glu-Ala may be better acceptors thanACC.

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Table IV. Other L-amino acids serve as acceptors for both $gamma$ GTase I and II
Radiometric transpeptidase assays were run for 2 h as described in "Materials and Methods" with 20 µM [¹⁴C]acceptor amino acid and 2 mM GSH. Values are the mean ± SD of three data points.

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Table V. ACC-dependent $gamma$ GTase I and II activities are inhibited more by L-amino acids than by D-amino acids
Radiometric transpeptidase assays were performed as described in "Materials and Methods," except the unlabeled amino acids (4 mM D-amino acids or 1 mM L-amino acids) were added 5 min prior to the addition of 1 mM [¹⁴C]ACC. Values are the mean ± SD of three to six data points and are representative of results obtained in two independent experiments. The specific activities of $gamma$ GTase I and II in the control assay were 5,300 and 2,700 nmol min¹ mg¹, respectively, in the control assays.

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Table VI. ACC dependent $gamma$ GTase I and II activities are inhibited by several peptides
Radiometric transpeptidase assays were performed as described in "Materials and Methods" except that 2 mM of the indicated peptide was added 5 min prior to addition of 2 mM [¹⁴C]ACC. The GSH concentration was 2 mM. Values are the mean ± SD of three to six data points and are representative of results obtained in two independent experiments. The specific activities of $gamma$ GTase I and II in the control assay were 7,200 and 4,300 nmol min¹ mg¹, respectively, in the control assays.

The [¹⁴C]dipeptide product of the transpeptidation reaction, GACC ( $gamma$ Glu-ACC), also serves as an acceptor for a second transpeptidationreaction. The product of the second transpeptidation reaction, $gamma$ Glu- $gamma$ Glu-ACC, can then serve as acceptor for a third transpeptidation,resulting in polyglutamated ACC ( $gamma$ glu- $gamma$ glu- $gamma$ glu-ACC). Polyglutamationwas observed when GSH was saturating, ACC became limiting, andthe concentration of GACC approached the concentration of ACC(Fig. 3, lane 2). When both donor and acceptor were saturating,a single product was formed (Fig. 3, lane 1). The identity ofthese products was confirmed by analyzing the products of acidhydrolysis by TLC and by GC-MS (data not shown). Multiple radiolabeledproducts were also synthesized from [¹⁴C]L-amino acids (data not shown). On the other hand, when ACCwas saturating and GSH was limiting in the assay, polyglutamationwas not observed. Instead, the reaction product, GACC, was usedas donor in subsequent reactions. GACC first increased (Fig. 3,lane 3) and then decreased during the course of an assay (Fig.3, lane 4). The reversibility of the reaction was best demonstratedby following the rapid disappearance of GACC after the additionof excess unlabeled ACC to the reaction.

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Figure 3. Radioisotope image showing the use of the reaction product GACC as a donor or acceptor in subsequent transpeptidation reactions by $gamma$ GTase I. Assays were chromatographed on a normal phase high performance silica gel thin-layer plate to resolve [¹⁴C]ACC and [¹⁴C]GACC and were imaged and quantified using an Ambis Radioisotope Imaging System. Lane 1, Both donor GSH and acceptor [¹⁴C]ACC were saturating; lane 2, GSH was 2 mM and [¹⁴C]ACC was 40 µM (ACC became limiting and GACC was used as an acceptor for the subsequent transpeptidation reaction resulting in polyglutamation of ACC); lane 3, [¹⁴C]ACC was 0.1 mM and GSH was 80 µM; and lane 4, the same reaction as in lane 3 was incubated 1 h longer following the addition of 2 mM unlableled ACC. Because GSH was limiting, [¹⁴C]GACC was used as a donor.

$gamma$ GTase I and II, at varied GSH concentrations and a fixed ACC concentration of 5 mM, exhibited Michaelis-Menten kinetics withK_m values for GSH of 110 and 90 µM, respectively. In the hydrolaseassay, $gamma$ GTase I and II exhibited K_m values for $gamma$ -GPNA of 1.7 and2.1 mM, respectively, indicating that $gamma$ -GPNA is a poor substratefor both enzymes (Table VII). In the transpeptidase assay, $gamma$ GTaseI and II activities exhibited biphasic kinetics with respect toACC concentration. K_m values for ACC were 0.130 and 3.1 mM for $gamma$ GTase I and 0.210 and 2.0 mM for $gamma$ GTase II (Table VII). Althoughcare was taken to use only initial reaction rates, the kineticconstants for ACC should be viewed as estimates, since the reactionis reversible. GACC can serve as a donor or acceptor for subsequentreactions. Similarly, GSH can serve as either a donor or acceptor.

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Table VII. Kinetic parameters for $gamma$ GTase I and II

Other Requirements for Activity

Salts (KCl, KNO₃, KBr, NaCl, and CaCl₂) had no effect on the activity of the purified enzymes at concentrations of 0.1 and1.0 M. Several metal chlorides (10 mM MgCl₂, 1 mM, MnCl₂ or CoCl₂,or 0.1 mM ZnCl₂) also had no effect on either activity. The presenceof DTT or EDTA had no effect on either the activity or stabilityof the enzyme, suggesting that reduced sulfhydryl groups are notrequired foractivity.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Little is known about the properties, in vivo substrates, and functions of $gamma$ GTases in plants. As a first step toward elucidatingthe function(s) of these enzymes, we have identified several $gamma$ GTasesin the pericarp of ripe tomato fruit. We purified and determinedthe catalytic properties of two of theseenzymes.

The purification and characterization of $gamma$ GTases from tomato were monitored using two assay methods. The standard spectrophotometricassay, developed for measuring the activity of $gamma$ GTases from mammals,is facile but it does not detect all $gamma$ GTases. Many $gamma$ GTases frommammals have very broad specificity for their $gamma$ -Glu donor (Meister,1989). Others, such as $gamma$ -glutamyl leukotrienase, have very narrowspecificity and are unable to use $gamma$ -GPNA, GSSG, or even GSH asa glutamyl donor (Heisterkamp et al., 1991; Carter et al., 1997).A $gamma$ GTase from yeast catalyzes hydrolysis but not the transpeptidationreaction (Pennickx and Jasper, 1985). In addition, the spectrophotometricassay measures only hydrolysis. It does not address the fate ofGlu, which may be particularly important in plants in which many $gamma$ -glutamyl-linked peptides are found. We also used a radiometricassay, which measures transpeptidation reactions in which theGlu is transferred to a radiolabeled acceptor following hydrolysis.This assay can accommodate a broad spectrum of $gamma$ -Glu donors, includingGSH, $gamma$ -GPNA, and glutathione S-conjugates (Tables II and III),and an equally broad spectrum of acceptors (Tables IV-VI). The onlyrequirement is that either the donor or acceptor be appropriatelyradiolabeled. Furthermore, the spectrophotometric and radiometricmethods can be coupled to measure hydrolysis and transpeptidationin the same assay. Using these assays, we detected $gamma$ GTases that(like animal $gamma$ GTases) differ in the their specificity for $gamma$ -GPNA,GSH, and other $gamma$ -Glu donors (Tables I and II). In fact, $gamma$ GTasesdiffering in specific activity in our two assays were resolvedby ultracentrifugation at 150,000g.

In mammals, $gamma$ GTases are highly expressed in tissues with secretory or absorptive functions (Meister et al., 1981; Meister,1988, 1989). Both soluble and membrane-bound $gamma$ GTases have beenidentified. The membrane-bound enzymes are heterodimeric glycoproteins.They have a small subunit with a M_r between 21,000 and 28,000that contains the catalytic site. A large subunit, with a M_r between38,000 and 72,000, contains a short hydrophobic domain, whichanchors the enzyme in the membrane (Meister et al., 1981; Meister,1989). $gamma$ GTases were first purified from mammals as soluble proteolyticfragments lacking the short membrane-anchoring region. The twosubunits of $gamma$ GTases are synthesized as a single, nonglycosylated,precursor peptide, which is then translocated, auto-cleaved, glycosylated,and inserted into the membrane with the catalytic site most oftenon the external surface of the membrane. Eighteen $gamma$ GTase isozymesfrom humans have been identified by isoelectric focusing, andmany were shown to result from differing degrees of glycosylation(Meister, 1989).

We have presented evidence that tomato fruit also contains several $gamma$ GTases that differ in membrane association, degree ofglycosylation, and substrate specificity. Three $gamma$ GTases purifiedfrom ripe tomato exhibited native and subunit molecular massesof 43 kD. Based on their binding to and differential elution fromCon A, two of these enzymes may be differently glycosylated. Athird 43-kD $gamma$ GTase did not bind to Con A, or react with a ConA-horseradish peroxidase conjugate, indicating that it is notglycosylated. These three $gamma$ GTases were released from either 7,000or 100,000g wall and membrane pellets of tomato fruit with 1.0M NaCl, suggesting that they are peripheral membrane proteins.Even with 1.0 M NaCl, nearly 70% of the transpeptidase activitybut only 20% of the $gamma$ -GPNA-hydrolyzing activity pelleted uponultracentrifugation, resulting in a dramatic change in the ratioof hydrolase to transpeptidase activity (Table I). Work is underway to further characterize the pelleted $gamma$ GTase. It is possiblethat tomato contains both peripheral and integral membrane $gamma$ GTases.A second possibility is that high salt dissociates one catalyticallyactive subunit of a dimeric or multimeric protein. Alternatively,we may have extracted a catalytically active proteolytic fragmentof a membrane-bound $gamma$ GTase such as was initially isolated fromanimal tissues. Cognizant of this possibility, we included a cocktailof several protease inhibitors during the early stages of thepurification to reduce the likelihood of proteolysis. In fact,the purified and partially purified $gamma$ GTases were very susceptibleto proteolysis. Continued handling and even SDS denaturation oftenresulted in the appearance of a 27-kD fragment in preparationsinitially having a single 43-kD band. Additionally, some planttissues, notably leaves of Arabidopsis and Brassica juncea, containsoluble $gamma$ GTases that exhibit activity only in the spectrophotometricassay, and membrane-associated $gamma$ GTases that exhibit activity inboth assays (M. Martin, unpublished results). Work is under wayto establish the subcellular localization of these activitiesinArabidopsis.

Several earlier reports described the partial purification and characterization from other plants of soluble $gamma$ GTases thatuse $gamma$ -GPNA as a donor, but there is no consensus regarding proteinsize. A $gamma$ GTase from kidney bean was reported to have a nativemolecular mass of 180 kD (Goore and Thompson, 1967). A $gamma$ GTasefrom Blighis sapida (ackee fruit) was reported to have a nativeand subunit molecular mass of 12.5 kD (Kean and Hare, 1980). A $gamma$ GTase from onion scale was reported to have a native and subunitmolecular mass of 56.7 kD (Lancaster and Shaw, 1994). A $gamma$ GTasefrom soybean seeds was reported to have a native and subunit molecularmass of 27 kD (Martin and Slovin, 1996).

The catalytic properties of the two purified $gamma$ GTases from tomato are consistent with broad in vivo functions, including thehydrolysis of GSH, GSSG, and/or glutathione S-conjugates. In fact,the two $gamma$ GTases from tomato fruit, like some $gamma$ GTases from animalsand the $gamma$ GTase from soybean seeds, have very broad donor specificityand a high affinity for GSH (with K_m values of 90 and 110 µM forthe tomato enzymes compared with 5-10 µM for some animal enzymesand 80 µM for the soybean enzyme; Meister et al., 1981; Meister,1989; Martin and Slovin, 1996). In contrast, the enzymes isolatedfrom bean and onion have K_m values for GSH between 1 and 5 mM(Goore and Thompson, 1967; Lancaster and Shaw, 1994). Both $gamma$ GTaseI and II exhibited higher affinity for GSH, GSSG, and glutathioneS-conjugates than for most dipeptides and for several artificialsubstrates with an N-terminal, $gamma$ -linked Glu. In vitro, both $gamma$ GTaseI and II can initiate hydrolysis of GSH and glutathione S-conjugatesfrom the N terminus or can hydrolyze the dipeptide resulting frominitial hydrolysis of GSH and its conjugates at the C terminus.Both activities function only as hydrolases at low pH, and thusmight be able to hydrolyze glutathione S-conjugates in thevacuole.

Like $gamma$ GTases from animals, the acceptor specificity of $gamma$ GTase I and II is broad and includes the L-isomers of several aminoacids, dipeptides, and tripeptide. We have also shown that both $gamma$ GTase I and II catalyze a reversible reaction by using the product,GACC, as a donor for subsequent reactions. In vitro, both $gamma$ GTaseI and II can synthesize as well as hydrolyze the numerous peptideswith N-terminal, $gamma$ -linked Glu that occur in various plant tissues.In crude extracts of tomato pericarp, $gamma$ GTases catalyzed the formationof a novel conjugate of the ethylene precursor, ACC (Martin etal., 1995). $gamma$ GTase activity increased through the course of tomatofruit maturation and ripening (Martin et al., 1995) and paralleledthe increase in conjugated ACC reported by other researchers (Suet al., 1984). Similarly, levels of $gamma$ GTase activity in onion paralleledthe hydrolysis of $gamma$ -glutamyl-peptides of sulfur compounds suchas $gamma$ -glutamyl alk(en)yl-cysteine sulfoxide, making them availablefor defensive purposes at key developmental points and, incidentally,as the flavor of onion (Lancaster et al., 1989; Lancaster andShaw, 1989, 1991, 1994). The in vivo functioning of $gamma$ GTases inthese reactions has not beendemonstrated.

	FOOTNOTES

Received September 17, 1999; accepted January 3, 2000.

¹ This work was supported in part by the U.S. Department of Agriculture-National Research Initiative (grant no. 96-35304-3733to J.P.S. and M.N.M.).

² Present address: Biotechnology Center for Agriculture and the Environment, Foran Hall, Cook College, Rutgers University, NewBrunswick, NJ 08901-8520.

^* Corresponding author; e-mail mnmartin{at}aesop.rutgers.edu; fax 732-932-0312.

³ Mention of a trademark, proprietary product, or vendor does not constitute a guarantee or warranty of the product by the U.S.Department of Agriculture and does not imply its approval to theexclusion of other products or vendors that might besuitable.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

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Purified -Glutamyl Transpeptidases from Tomato Exhibit High Affinity for Glutathione and Glutathione S-Conjugates1

Purified $gamma$ -Glutamyl Transpeptidases from Tomato Exhibit High Affinity for Glutathione and Glutathione S-Conjugates¹