Biosynthesis of Costunolide, Dihydrocostunolide, and Leucodin. Demonstration of Cytochrome P450-Catalyzed Formation of the Lactone Ring Present in Sesquiterpene Lactones of Chicory

doi:10.1104/pp.010957

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Biosynthesis of Costunolide, Dihydrocostunolide, and Leucodin. Demonstration of Cytochrome P450-Catalyzed Formation of the Lactone Ring Present in Sesquiterpene Lactones of Chicory

Jan-Willem de Kraker, Maurice C.R. Franssen,¹ ^* Maaike Joerink, Aede de Groot, and Harro J. Bouwmeester¹

Laboratory of Organic Chemistry, Wageningen University, Dreijenplein 8, 6703 HB Wageningen, The Netherlands (J.-W.d.K., M.C.R.F., M.J., A.d.G.); and Plant Research International, P.O. Box 16, 6700 AA Wageningen, The Netherlands (J.-W.d.K., M.J., H.J.B.)

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

Chicory (Cichorium intybus) is known to contain guaianolides, eudesmanolides, and germacranolides. These sesquiterpene lactonesare postulated to originate from a common germacranolide, namely(+)-costunolide. Whereas a pathway for the formation of germacra-1(10),4,11(13)-trien-12-oicacid from farnesyl diphosphate had previously been established,we now report the isolation of an enzyme activity from chicoryroots that converts the germacrene acid into (+)-costunolide.This (+)-costunolide synthase catalyzes the last step in the formationof the lactone ring present in sesquiterpene lactones and is dependenton NADPH and molecular oxygen. Incubation of the germacrene acidin the presence of ¹⁸O₂ resulted in the incorporation of one atom of ¹⁸O into (+)-costunolide. The label was situated at the ring oxygenatom. Hence, formation of the lactone ring most likely occursvia C₆-hydroxylation of the germacrene acid and subsequent attackof this hydroxyl group at the C₁₂-atom of the carboxyl group.Blue light-reversible CO inhibition and experiments with cytochromeP450 inhibitors demonstrated that the (+)-costunolide synthaseis a cytochrome P450 enzyme. In addition, enzymatic conversionof (+)-costunolide into 11(S),13-dihydrocostunolide and leucodin,a guaianolide, was detected. The first-mentioned reaction involvesan enoate reductase, whereas the formation of leucodin from (+)-costunolideprobably involves more than one enzyme, including a cytochromeP450enzyme.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Chicory (Cichorium intybus), also known as French endive, Witloof, and succory is probably a native of Europe and Asia. Atpresent, this composite plant is mainly cultivated for its roots(C. intybus var sativum) that contain high amounts of inulin (aFru polymer) or for its sprouts (C. intybus var foliosum Hegi)that are a well-known salad crop (Vogel et al., 1994; Kruistum,1997; Westerdijk, 2000). The white sprouts, which are grown inthe dark, have a slightly bitter taste that is associated withthe presence of sesquiterpene lactones. These compounds occurthroughout the plant, though at highest levels in the roots (0.42%dry weight), and act as deterrents toward insects (Rees and Harborne,1985; Price et al., 1990).

Sesquiterpene lactones are a major class of plant secondary metabolites that are mainly found in the Asteraceae but also occurinfrequently in other high plant families and lower plants (Seigler,1998). The majority of the more than 4,000 known different structureshas a guaiane, eudesmane, or germacrane framework. Also the sesquiterpenelactones of chicory belong either to the guaianolides, eudesmanolides,or germacranolides (Fig. 1; Seto et al., 1988; van Beek et al.,1990). (+)-Costunolide (Fig. 2, 15) is structurally thesimplest of all germacranolides and is generally accepted as theparent compound of the three mentioned types of sesquiterpenelactones (Geissman, 1973; Fischer et al., 1979; Seaman, 1982;Fischer, 1990).

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Figure 1. The sesquiterpene lactones of chicory: the guaianolides lactucin (1), 8-deoxylactucin (2), lactucopicrin (3), 11(S),13-dihydrolactucin (4), 11(S),13-dihydro-8-deoxylactucin (5), and 11(S),13-dihydrolactucopicrin (6); the eudesmanolides cichoriolide A (7) and sonchuside C (8); and the germacranolides sonchuside A (9) and cichorioside (10). The major sesquiterpene lactones in chicory are compounds 1 through 3.

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Figure 2. Proposed biosynthetic route for (+)-costunolide, a postulated key intermediate in sesquiterpene lactone biosynthesis. I, Cyclization of farnesyl diphosphate (FPP) to (+)-germacrene A (11) by (+)-germacrene A synthase (a sesquiterpene synthase). II, Hydroxylation of the isopropenyl side chain by (+)-germacrene A hydroxylase, a cytochrome P450 enzyme. III, Oxidation of germacra-1(10),4,11(13)-trien-12-ol (12) via germacra-1(10),4,11(13)-trien-12-al (13) to germacra-1(10),4,11(13)-trien-12-oic acid (14) catalyzed by NAD(P)⁺-dependent dehydrogenase(s). IV, Postulated hydroxylation at the C₆-position of germacratrien-12-oic acid (14) and subsequent lactonization will yield (+)-costunolide (15).

Our studies with chicory roots have made it apparent that its sesquiterpene lactones are derived from (+)-germacrene A (11;de Kraker et al., 1998). This sesquiterpene olefin is oxidizedthrough germacra-1(10),4,11(13)-trien-12-ol (12) and germacra-1(10),4,11(13)-trien-12-al (13) into germacra-1(10), 4,11(13)-trien-12-oicacid (14; Fig. 2; de Kraker et al., 2001a). Formation of(+)-costunolide (15) from the germacrene acid is expectedto be the next step, but this has not yet been demonstrated. Ithas been postulated to occur via hydroxylation at the C₆-positionby a cytochrome P450 enzyme, after which lactonization yields(+)-costunolide (Geissman, 1973; Fischer et al., 1979; Seaman,1982; Fischer, 1990). Germacrene acid (14) was only veryrecently isolated from fresh costus roots in quantities that makeit possible to investigate this last crucial step in the formationof the lactone ring present in sesquiterpene lactones (de Krakeret al., 2001b).

(+)-Costunolide (15) is also considered to be a branching point in the biosynthesis of sesquiterpene lactones fromwhere pathways for the formation of guaianolides, eudesmanolides,and germacranolides divide. It has been postulated by variousauthors that cyclization of (+)-costunolide to either guaianolidesor eudesmanolides is mediated by C₄-C₅ epoxidation (i.e. via parthenolide[22]) or C₁-C₁₀ epoxidation, respectively (Brown et al.,1975; Fischer, 1990; Teisseire, 1994; Piet et al., 1995). As analternative, the possibility of a C₃-hydroxylation of the germacranolidefor formation of a guaianolide has been suggested (Piet et al.,1996). This article will mainly focus on the formation of (+)-costunolide(15) from germacrene acid (14), but some attentionis also paid to the subsequent conversions of (+)-costunolide.

	RESULTS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Conversion of Germacrene Acid into Sesquiterpene Lactones

Gas chromatography-mass spectroscopy (GC-MS) analyses of the pentane-ether extract from the incubation of a 20,000g chicoryroot supernatant with germacra-1(10),4,11(13)-trien-12-oic acid(14) and NADPH revealed three products that were detectedneither in incubations without NADPH nor in incubations with boiledsupernatant (Fig. 3, A and B). The major peak co-eluted with astandard of (+)-costunolide (15) that at an injection porttemperature of 320°C is detected as its Cope rearrangement productdehydrosaussurea lactone (16; Fig. 3C). At this high injectionport temperature, germacrene acid, the substrate, is also Coperearranged, and this results inthe formation of elemene acid (21)and diastereomeric elemene acid, which elute at different retentiontimes (de Kraker et al., 2001b).

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Figure 3. A, GC-MS analyses of the products formed in the incubation of a 20,000g supernatant from chicory roots with NADPH and germacra-1(10),4,11(13)-trien-12-oic acid (14) displays peaks of dehydrosaussurea lactone (dHSausL [16]), saussurea lactone (SausL [18]), and leucodin (Leuc [19]). B, These products are not observed in the absence of NADPH. Germacrene-1(10),4,11(13)-trien-12-oic acid (14) is observed as elema-1,3,11(13)-trien-12-oic acid (EAc) plus its diastereomer (EAc*); the internal standard (i.s.) is 1 nmol of cis-nerolidol. The huge fronting peaks (

) are fatty acids (palmitic and linoleic acid). C, The standard of 0.5 mM costunolide (15) in ethanol yields a tailing peak of dehydrosaussurea lactone (dHSausL [16]).

The two other products were identified as 11(S),13-dihydrocostunolide (17), which is Cope rearranged into saussurealactone (18), and leucodin (19; Fig. 4). Both 11(S),13-dihydrocostunolideand leucodin are enzymatically formed from (+)-costunolide (15),because they also appeared in incubations of (+)-costunolide withthe 20,000g supernatant and NADPH (vide infra). It cannot be excludedthat even more products are formed during the incubation of germacreneacid, because higher oxygenated sesquiterpene lactones are likelynot volatile enough for detection by GC. Furthermore, the presenceof fatty acids in chicory extracts (Sannai et al., 1982) complicatesthe GC-analysis, because they yield big peaks under which smallerproduct peaks may "disappear." Similar incubations with the 20,000gsupernatant of the substrate analogs $alpha$ - and $gamma$ -costic acid (Fig.5; 20) and elema-1,3,11(13)-trien-12-oic acid (Fig. 5;21) did not result in any product formation.

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Figure 4. Products formed from germacra-1(10),4,11(13)-trien-12-oic acid (14) in the presence of NADPH and oxygen by a 20,000g supernatant from chicory roots. Leucodin (19) is detected as such, whereas costunolide (15) and 11,13-dihydrocostunolide (17) are detected as their Cope rearrangement products dehydrosaussurea lactone (16) and saussurea lactone (18), respectively.

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Figure 5. Various substrates that were also incubated with the 20,000g supernatant and NADPH. A mixture of $alpha$ -costic acid (20a) and $gamma$ -costic acid (20b) or elema-1,3,11(13)-trien-12-oic acid (21) may serve as substrate analogs of germacrene acid (14). Parthenolide (22) and dehydrocostus lactone (23) serve as model compounds for conversions that might occur during chicory sesquiterpene lactone biosynthesis after formation of (+)-costunolide.

Characterization of the (+)-Costunolide Synthase

For characterization of the (+)-costunolide synthase the response of the GC-MS to different concentrations of (+)-costunolide(15) should preferably be linear. Yet, at the injectionport temperature of 320°C we used, the GC-trace of costunolide(Fig. 3C) does not show a sharp peak of dehydrosaussurea lactone(16) but a tailing peak that contains minor peaks of costunolide-relatedproducts like $alpha$ - and $beta$ -cyclocostunolide. (+)-Costunolide is apparentlymore resistant to Cope rearrangement than, for instance, germacreneacid (14). In literature, it has also been noted that alactone ring has a strong influence on the thermal stability ofgermacrenes and that Cope rearrangement of (+)-costunolide isreversible (Jain et al., 1970; Minnaard, 1997). Grieco and Nishazawa(1977) even used this thermal equilibration to prepare (+)-costunolidefrom dehydrosaussurea lactone (16) on a preparative GC.Despite the lower susceptibility of (+)-costunolide to Cope rearrangement,a lowered injection port temperature (200°C) still resulted inCope rearrangement of (+)-costunolide during its migration throughthe GC-column and yielded a broad hump (similar to the one shownfor germacrene aldehyde in de Kraker et al., 2001b). Althoughof poor quality, the dehydrosaussurea lactone GC-peak visualizedin Figure 3C proved to be linear with the injected (+)-costunolideconcentration in a range of 5 to 50 µM. Costunolide concentrationsbelow 5 µM, i.e. 0.25 nmol in the 1-mL incubation mixture, werenotmeasurable.

A more serious problem for characterization of the (+)-costunolide synthase is that, almost certainly, all subsequent conversionproducts of (+)-costunolide have not been detected, let alonequantified. Hence, the given enzyme activities are a summationof the peaks of dehydrosaussurea lactone (16), saussurealactone (18), and leucodin (19) and are consequentlymore an indication than an absolute value of (+)-costunolide synthaseactivity. Quantitative measurement of the elemene acid peak (substratepeak) area was not an option, because it is not linear with theconcentration and, more generally, acid peaks in GC-measurementsare of poorquality.

Table I shows that (+)-costunolide synthase is dependent on oxygen and NADPH, whereas NADH was much less effective as a reductant.This suggests the involvement of a cytochrome P450 enzyme, whichwas confirmed by the effect of various established cytochromeP450 inhibitors (West, 1980; Mihaliak et al., 1993). In the presenceof cytochrome c (100 µM), no enzymatic products of germacreneacid (14) were measured; 100 µM miconazole reduced theamount of measurable products with 71%, 100 µM aminobenzotriazolewith 44%, 1 mM metyrapone with 78%, and 100 µM clotrimazole with97%.

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Table I. Requirements for (⁺)-costunolide synthase activity

The strongest proof for the involvement of a cytochrome P450 enzyme is blue light-reversible inhibition of enzyme activityby CO (West, 1980; Mihaliak et al., 1993). The results depictedin Figure 6 show an inhibitory effect of CO on the produced sumof (+)-costunolide (15), 11(S),13-dihydrocostunolide (17),and leucodin (19), which could to some extent be reversedby blue light.

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Figure 6. Demonstration of blue-light reversible CO inhibition of the costunolide synthase. Product formation in the presence of 90% (v/v) N₂ + 10% (v/v) O₂ (labeled as $-$ CO) is set at 100% and this activity corresponds to a peak size of dehydrosaussurea lactone (16) (costunolide), saussurea lactone (18) (dihydrocostunolide), and leucodin (19) of 0.58, 0.27, and 0.15 × internal standard (1 nmol of cis-nerolidol) respectively. The inhibition in the presence of 90% (v/v) CO + 10% (v/v) O₂ (labeled as +CO) was reversed to some extent by irradiation with blue light (450 nm). All incubations were done in the absence of FAD and FMN.

Characterization of the Subsequent Conversions of (+)-Costunolide

Incubation of (+)-costunolide with a 20,000g chicory root supernatant in the presence of NADPH yielded 11(S),13-dihydrocostunolide(17) and leucodin (19). No other products were detectedby GC-MS analysis of the incubation, but comparison of the decreasein peak height of dehydrosaussurea lactone (16) with theintensity of the product peaks strongly suggested the formationof other products that are not detected by GC. The enzyme activitythat catalyzes the reduction of the 11(S),13-exocyclic doublebond of (+)-costunolide was not capable of doing the same withthe model compound dehydrocostus lactone (Fig. 5; 23),i.e. it did not yield 11(S),13-dihydro-dehydrocostus lactone.Nevertheless, incubation of dehydrocostus lactone in the presenceof NADPH and a chicory root extract gave a new unknown productthat had a shorter retention time, the same molecular mass, andexhibited a very similar mass spectrum as dehydrocostus lactone.It is probably the result of a double bond isomerization somewherein the molecule. Incubation of parthenolide (Fig. 5; 22) $---$ apostulated intermediate of guaianolide biosynthesis $---$ did not yieldleucodin (19), but conversion of parthenolide into othernon-GC-MS-measurable sesquiterpene lactones cannot be excluded.Parthenolide itself disintegrates upon GC-analysis in a numberof compounds; for this reason, no quantitative determination couldbe done of the amount of parthenolide present afterincubation.

To test which type(s) of enzymes might catalyze the formation of 11(S),13-dihydrocostunolide (17) and leucodin (19),the pyridine nucleotide cofactors were varied (Table II). Formationof both compounds was dependent on NADPH, but a part of the (+)-costunolidereductase activity was retained in the absence of any cofactor.

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Table II. Pyridine nucleotide cofactor dependency of 11(S),13-dihydrocostunolide and leucodin biosynthesis from (⁺)-costunolide

Table III shows that the formation of leucodin (19) from (+)-costunolide (15) is dependent on oxygen, whereasthe formation of 11(S),13-dihydrocostunolide (17) is not.Formation of leucodin was strongly inhibited by CO, which suggeststhe involvement of a cytochrome P450 enzyme. The reaction wasalso inhibited by all of the tested cytochrome P450 inhibitorsexcept amino-benzotriazole. Interestingly, the measured amountof 11(S),13-dihydrocostunolide was raised in the presence of carbonmonoxide or the absence of oxygen. This indicates that in theseincubations, at least a part of the successive (hypothetical)conversion of 11(S),13-dihydrocostunolide to higher oxygenatedsesquiterpene lactones is inhibited and that some of the involvedreactions are possibly cytochrome P450 catalyzed. It is somewhatcontradictory that the detected amount of 11(S),13-dihydrocostunolidewas hardly effected or even lowered when cytochrome P450-inhibitorshad been added to the incubations. Perhaps each individual inhibitoreffects only some of the successive cytochrome P450-catalyzedreactions, whereas CO and cytochrome c inhibit all cytochromeP450-catalyzed reactions. It cannot be excluded that the inhibitorsthemselves influence the formation of 11(S),13-dihydrocostunolideas well, because they were also able to inhibit the (+)-germacreneA synthase (de Kraker et al., 2001a).

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Table III. Inhibition of 11(S),13-dihydrocostunolide and leucodin biosynthesis from (⁺)-costunolide

Incorporation of Oxygen-18

Incubation of germacrene acid (14) in the presence of ¹⁸O₂ led to the incorporation of one atom of ¹⁸O into (+)-costunolide (15). As a result, the ion peakin the mass spectrum of dehydrosaussurea lactone (16) wasshifted from 232 to 234 atomic mass units (amu; Fig. 7). Similarchanges were observed in the mass spectrum of saussurea lactone(18), the Cope rearrangement product of 11(S),13-dihydrocostunolide(17; data not shown). The ion peak of this compound wasshifted from 234 to 236 amu, whereas the [M-Me]⁺ peak was shifted from 219 to 221 amu. Genuine costunolide (15)and dehydrosaussurea lactone (16) have an almost similarmass spectrum (Jain et al., 1971), and the small peak of 204 amuin their mass spectra arises from the loss of carbon monoxidefrom the lactone moiety of the molecular ion (Sathe et al., 1969,1971). Because in the ¹⁸O₂-labeling experiment, the ion peak of 204 amu from dehydrosaussurealactone is shifted to 206 amu (Fig. 7) $---$ i.e. carbon monoxide expulsiondoes not result in the loss of the ¹⁸O-label $---$ it is most likely the ring oxygen atom of costunolidethat has been labeled.

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Figure 7. Mass spectra of dehydrosaussurea lactone (16) originating from (+)-costunolide (15) that has been produced from germacrene acid (14) under standard assay conditions (A), in the presence of ¹⁸O₂ (B), or that originates from a standard of (+)-costunolide (C).

The mass spectra of leucodin (19) showed the incorporation of two atoms of ¹⁸O because the mass of the ion peak was shifted with 4 units from246 to 250 amu (Fig. 8). Unfortunately, in the enzyme assay, theGC-peak of leucodin is superpositioned on the tailing peak oflinoleic acid (Fig. 3A), which obscures the mass spectrum of leucodinparticular in the lower mass (m/z) range. In general, bubblingof the enzyme assay with ¹⁸O₂ did not have any effect on the detected amounts of enzymaticproducts, i.e. it does not effect the enzyme activities.

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Figure 8. Mass spectra of leucodin (19) produced from germacrene acid (14) in an enzyme assay under standard conditions (A) or in the presence of ¹⁸O₂ (B). C, Mass spectrum of the leucodin standard.

	DISCUSSION

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

(+)-Costunolide

The present results show that chicory roots contain an enzyme that converts germacra-1(10),4,11(13)-trien-12-oic acid (14)into (+)-costunolide (15), yielding the lactone ring presentin sesquiterpene lactones. This step is the final proof for thepostulated pathway depicted in Figure 2 from farnesyl diphosphateto (+)-costunolide via (+)-germacrene A (11), germacra-1(10),4,11(13)-trien-12-ol (12), and germacra-1(10),4,11(13)-trien-12-oic acid (14; Geissman, 1973; Fischer etal., 1979; Fischer, 1990; de Kraker et al., 2001a).

The (+)-costunolide synthase is a cytochrome P450 enzyme that is dependent on NADPH and O₂ and is accordingly inhibited byvarious established cytochrome P450 inhibitors. Blue light-reversibleCO inhibition of the (+)-costunolide synthase could be demonstratedas well, although the results are somewhat obscured by subsequentenzymatic conversions of (+)-costunolide. Incubation of germacreneacid (14) in the presence of ¹⁸O₂ showed the incorporation of one atom of ¹⁸O into (+)-costunolide, another typical feature of cytochromeP-450 enzymes (West, 1980; Mihaliak et al., 1993). This incorporationof one atom of oxygen inside the ring also validates that germacreneacid (14) is first hydroxylated at the C₆-position (Fischeret al., 1979), after which this hydroxyl group attacks, possiblyenzyme-mediated, the carboxyl group at C₁₂ (Fig. 9). After lactonization,the oxygen isotope is incorporated in the lactone, inside thering. The obtained result rules out an alternative mechanism forformation of the lactone ring in which hydride abstraction atC6 (by an oxidase) is followed by an internal quenching of theresultant C₆ carbocation by the carboxyl group. In such a caseboth oxygen atoms present in costunolide (15) would havearisen from the carboxyl group of germacrene acid (14)and no ¹⁸O would have been incorporated.

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Figure 9. Mechanism for the enzyme catalyzed formation of (+)-costunolide (15) from germacrene acid (14) that results in the incorporation of one atom of ¹⁸O from ¹⁸O₂.

The (+)-costunolide synthase is not capable of converting the substrate analogs $alpha$ -costic acid (20a) and elema-1,3,11(13)-trien-12-oicacid (21), which is not unexpected because the C₆-positionis not allylic. However, $gamma$ -costic acid (20b) $---$ in which theC₆-position is allylic $---$ was not converted either, so apparentlythe geometry of the cyclodecadiene ring system is also requiredfor the reaction catalyzed by the (+)-costunolidesynthase.

Germacranolides, Guaianolides, and Eudesmanolides

The present results clearly show that (+)-costunolide (15) is the intermediate sesquiterpene lactone in the biosynthesisof the guaianolides, and germacranolides present in chicory (Fig.1), and presumably the eudesmanolides as well. It is reasonableto assume that this conclusion is also valid for other plant speciesthat contain these skeletal types of sesquiterpene lactones. Althoughthe used GC-MS technique is not the appropriate method to measurehigher oxygenated sesquiterpene lactones, some information wasobtained about the steps between (+)-costunolide and the finalproducts of sesquiterpene lactone biosynthesis in chicory. Incubationsof (+)-costunolide and a 20,000g supernatant in the presence ofNADPH and oxygen yielded 11(S),13-dihydrocostunolide (17)and leucodin (19; Fig. 10).

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Figure 10. (+)-Costunolide (15) is enzymatically converted into 11(S),13-dihydrocostunolide (17) and leucodin (19) in the presence of NADPH and O₂. Incubation of germacrene acid (14) in the presence of ¹⁸O₂ gives incorporation at positions marked with an asterisk. It is unclear whether leucodin (19) is formed via 17. Both (+)-costunolide and 11(S),13-dihydro-costunolide are likely precursors for other sesquiterpene lactones present in chicory. Notably, leucodin (19) is only one hydroxylation away from 11(S),13-dihydro-8-deoxylactucin (5), a minor sesquiterpene lactone of chicory.

The formation of 11(S),13-dihydrocostunolide is not dependent upon oxygen but is strongly enhanced in the presence of NADPH,whereas some enzyme activity (15%) is retained in the absenceof NADPH. The reduction of the C₁₁-C₁₃ exocyclic double bond iscomparable with the type of reactions catalyzed by enoate reductases.This is a group of iron-sulfur flavoproteins that are involvedin fatty acid biosynthesis and can be found in many micro-organismssuch as Clostridia sp. and baker's yeast, but they have also beenobserved in plant cell cultures such as that of tobacco. Theycatalyze the reduction of double bonds that are "activated" byan electron-withdrawing substituent, like the olefinic bond of $alpha$ , $beta$ -unsaturated carboxylic acids and esters, under anaerobic conditionsin the presence of reducing agents (generally NADH; Holland, 1992;Faber, 2000). An enoate reductase type of reaction has also beendescribed for a cell-free system of peppermint (Mentha piperita)leaves. It contains a so-called terpenone- $Delta$ ^4.8-reductase that converts the isopropylidene side chain of (+)-pulegone,which is positioned next to a keto group, into an isopropyl sidechain (Battaile et al., 1968; Croteau and Venkatachalam, 1986).This NADPH-catalyzed reaction involved in monoterpene metabolismis thought to occur stereoselectively, and distinct terpenone- $Delta$ ^4.8-reductases yield either ( $-$ )-menthone or (+)-isomenthone (Croteauet al., 1991).

Similar to the stereoselective reactions catalyzed by enoate reductases of microorganisms and the terpenone- $Delta$ ^4.8-reductase, reduction of the C₁₁-C₁₃ exocyclic double bond of(+)-costunolide yields only one isomer, i.e. the 11(S),13-stereoisomerof dihydrocostunolide. This compound has the same stereochemistrythat is present in the 11,13-dihydro sesquiterpene lactones (4-6and 8) of chicory (Seto et al., 1988; van Beek et al.,1990). This notwithstanding, some plant species do contain C₁₁-epimers,like achillin, which is the 11(R)-epimer of leucodin (Martínezet al., 1988; Ho et al., 1998), indicating that a stereoselectiveenzyme that synthesizes these C₁₁-epimers should also exist. Theenzyme exhibits at least some substrate specificity because theC₁₁-C₁₃ exocyclic double bond of dehydrocostus lactone (6)was not reduced. The detected formation of leucodin (19)proves that guaianolides originate from (+)-costunolide (15).Interestingly, leucodin is only one hydroxylation away from 11(S),13-dihydro-8-deoxylactucin(5; Fig. 10), a minor sesquiterpene lactone of chicory (vanBeek et al., 1990). The conversion of (+)-costunolide into leucodinmost likely involves more than one enzyme, but whether leucodinoriginates from 11(S),13-dihydrocostunolide (17) was notinvestigated. Parthenolide (5) was shown not to be involvedin leucodin biosynthesis, but it still cannot be excluded that11(S),13-dihydroparthenolide is. Various authors have suggestedthat either such a 4,5-epoxide or a C₃-hydroxyl group is necessaryto direct the cyclization of (+)-costunolide toward a guaianeframework (Brown et al., 1975; Fischer, 1990; Teisseire, 1994;Piet et al., 1995, 1996).

Formation of leucodin from (+)-costunolide is oxygen dependent and it could be inhibited by the addition of cytochrome P450inhibitors or CO, whereas formation of 11(S),13-dihydrocostunolidecould not. Furthermore, experiments with ¹⁸O₂ demonstrated that the oxygen atom of the keto group in leucodinalso originates from molecular oxygen. Taken together, these observationsat least suggest the involvement of a cytochrome P450-enzyme inleucodin biosynthesis (West, 1980; Mihaliak et al., 1993).

We assume that 11(S),13-dihydrocostunolide (17) is the precursor of all 11(S),13-dihydro-sesquiterpene lactones (4-6and 8-10) present in chicory, including 11(S),13-dihydro-8-deoxylactucin(5; Fig. 10). However, in the major sesquiterpene lactonesof chicory, the guaianolides 1 and 3 (van Beek etal., 1990), the C₁₁-C₁₃ bond is unsaturated and these compoundsare most likely formed from (+)-costunolide without the intermediacyof 11(S),13-dihydrocostunolide. Perhaps some of these sesquiterpenelactones were already formed during the experiments, but unfortunatelythese compounds cannot be detected in GC-MS measurement becauseof their polarity and reduced volatility. The detection and analysisof such higher oxygenated compounds in enzymatic reaction mixtureswill need derivatization and/or the use of other chromatographictechniques likeHPLC.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION RESULTS DISCUSSION MATERIALS AND METHODS LITERATURE CITED

Materials

Fresh roots of cultivated chicory (Cichorium intybus L. cv Focus) were harvested during late summer and obtained from a grower(J. de Mik) in Veenendaal, The Netherlands. The chicory rootswere cut into small pieces, frozen in liquid nitrogen, and storedat $-$ 80°C. Germacra-1(10),4,11(13)-trien-12-oic acid (14),(+)-costunolide (15), and dehydrocostus lactone (23)were isolated from costus roots (de Kraker et al., 2001b). Thesynthesis of a mixture of $alpha$ - and $gamma$ -costic acid (20) andthe synthesis of elema-1,3,11(13)-trien-12-oic acid (21)have previously been described (de Kraker et al., 2001b, 2001a;respectively). The germacrene acid, costic acid, and elemene acidwere dissolved in tert-butyl methyl ether at 15 mM concentrations.(+)-Costunolide, dehydrocostus lactone, and parthenolide (22;Sigma, St. Louis) were dissolved in ethanol at 10 mM concentrations.A sample of leucodin (19) was kindly provided both by Prof.M. Ando (Niigata University, Niigata City, Japan; Ando et al.,1994) and Dr. Shi Yong Ryu (Korea Research Institute of ChemicalTechnology, Yusung, Taejon, Korea), who also provided its C₁₁-epimerachillin (Ho et al., 1998). 11,13-Dihydro-dehydrocostus lactone(mokko lactone) was a gift of Prof. Y. Asakawa (Tokushima BunriUniversity, Tokushima, Japan). cis-Nerolidol was purchased fromFluka (Buchs, Switzerland); ether (diethyl ether) and pentanewere redistilled beforeuse.

A GC-standard of 11(S),13-dihydro-costunolide (17) was prepared from 2 mg of (+)-costunolide (15) that was dissolvedin 1.5 mL of ethyl acetate and stirred with 1.5 mg of NaBH₄ at0°C, a procedure described for the reduction of the C₁₁-C₁₃ exocyclicdouble bond of various sesquiterpene lactones (Asakawa et al.,1980; Asakawa, 1982; Seto et al., 1988). After 45 min, the reactionwas stopped by the addition of 1% (w/w) HAc and an extra 2 mLof ethyl acetate. The organic phase was filtered through a glass-woolplugged (dimethyl chlorosilane-treated glass wool, Chrompack,Raritan, NJ) Pasteur pipette that contained 0.45 g of silica anda little anhydrous MgSO₄. GC-MS analysis of the filtrate showedthat one-half of the (+)-costunolide was converted into 11(S),13-dihydro-costunolide,whereas no trace of its C₁₁-epimer wasdetected.

Upon request, small samples of the sesquiterpenes used and the crude enzyme preparations studied will be made available ina timely manner for non-commercialresearch.

Enzyme Isolation and Assay for (+)-Costunolide Synthase Activity

A cell free extract of chicory roots was prepared from the frozen material in the same way as described for the isolationof the germacrene A hydroxylase (de Kraker et al., 2001a), butMgCl₂ was omitted from the extraction buffer. The prepared 20,000gsupernatant was desalted with an Econo-Pac10 DG column (Bio-Rad,Hercules, CA) to an assay buffer containing 25 mM Tris (pH 7.5),1 mM ascorbic acid, 5 µM FAD, 5 µM FMN, and 10% (v/v) glycerol.Dithiothreitol was omitted from the assay buffer, because theSH-groups present in dithiothreitol may undergo a Michael-typeaddition to the C₁₁-C₁₃ exocyclic double bond of (+)-costunolide(Kupchan et al., 1970). A 1-mL aliquot of the desalted supernatantwas incubated in the presence of 45 µM germacrene acid (14)and a 1 mM NADPH-regenerating system, which consists of 1 mM NADPH,5 mM Glc-6-phosphate, and 1.2 IU Glc-6-phosphate dehydrogenase(all from Sigma). Incubations were also done with boiled desaltedsupernatant and in the absence of NADPH. The experiments wererepeated with elema-1,3,11(13)-trien-12-oic acid (21) andwith a mixture of $alpha$ - and $gamma$ -costic acid (20), which mayserve as substrate analogs for the germacrene acid (14).After 1 h of incubation at 30°C, the reactions were stopped bystorage in the freezer at $-$ 20°C.

The incubations were extracted thrice with 1 mL of 20% (v/v) ether in pentane, after the addition of 5 µL of a 0.2 mM cis-nerolidolsolution in ethanol that serves as internal standard (responsefactor of [+]-costunolide [i.e. generated peak of dehydrosaussurealactone] relative to cis-nerolidol is 0.15). The organic phasewas filtered through a glass-wool plugged Pasteur pipette thatcontained 0.45 g of silica and a little anhydrous MgSO₄. The columnwas washed with 1.5 mL of ether, and the extract was carefullyconcentrated to approximately 50 µL under a stream of nitrogen.Samples of 2 µL were analyzed by GC-MS using an injection porttemperature of 320°C to provoke Cope rearrangement of (+)-costunolide(15). Mass spectra were recorded at 70 eV scanning from35 to 300 amu; the GC oven temperature was programmed as describedpreviously (de Kraker et al., 1998).

Characterization of (+)-Costunolide Synthase Activity

To determine whether the formation of (+)-costunolide (15) from germacrene acid (14) was catalyzed by a cytochromeP450-enzyme, the effect of various established cytochrome P450-inhibitors(cytochrome c, metyrapone, clotrimazole, micozanole, and amino-benzotriazole)on this reaction was tested, as well as the effect of CO or anargon atmosphere. The cofactor dependence was also investigated,i.e. NAD(P)⁺ or NADH was added instead of NADPH. Experiments were carriedout in a similar manner as described for the germacrene A hydroxylase(de Kraker et al., 2001a), using a 20,000g supernatant and 5 µLof 0.2 mM cis-nerolidol as internal standard. Blue-light reversalof CO inhibition was investigated with gas mixtures of 10% (v/v)O₂ + 90% (v/v) N₂ (blank) and 10% (v/v) O₂ + 90% (v/v)CO.

The origin of the oxygen incorporated in the lactone ring of (+)-costunolide was investigated with ¹⁸O₂ (99% pure; Icon Services, Mt. Marlon, NY). One milliliter ofincubation mixture in a (vented) septum-capped 4.5-mL vial wasfirst bubbled with nitrogen to remove air and subsequently bubbledwith ¹⁸O₂. The mass spectra of the compounds produced were compared withthose formed in the standard enzyme assays underair.

Investigation of Subsequent Conversions of (+)-Costunolide

To investigate the conversion (+)-costunolide (15), this compound was incubated at 30 µM concentrations in the samemanner as described for germacrene acid (14). Parthenolide(22; 20 µM) was incubated as well, because it might bean intermediate in the formation of guaianolides. Dehydrocostuslactone (23; 20 µM) was incubated to investigate the reductionof the C₁₁-C₁₃ exocyclic double bond in sesquiterpene lactonesof chicory. The effect of cytochrome P450 inhibitors and CO onthe conversion of (+)-costunolide was studied, just as the effectof various pyridine nucleotide cofactors and an argonatmosphere.

	ACKNOWLEDGMENTS

We thank Prof. M. Ando (Niigata University, Niigata City, Japan; Ando et al., 1994) and Dr. S.Y. Ryu (Korea Research Instituteof Chemical Technology, Yusung, Taejon) for the gift of leucodinand Prof. Y. Asakawa (Tokushima Bunri University, Tokushima, Japan)for the gift of dihydro-dehydrocostus lactone. We also thank J.de Mik for the gift of the chicory roots and F.W.A. Verstappenand M. Schurink for their useful suggestions and technicalassistance.

	FOOTNOTES

Received October 18, 2001; returned for revision December 6, 2001; accepted January 24, 2002.

¹ These authors contributed equally to thepaper.

^* Corresponding author; e-mail Maurice.Franssen{at}bio.oc.wag-ur.nl; fax 31-317-484914.

Article, publication date, and citation information can be found at www.plantphysiol.org/cgi/doi/10.1104/pp.010957.

LITERATURE CITED

TOP
ABSTRACT
INTRODUCTION
RESULTS
DISCUSSION
MATERIALS AND METHODS
LITERATURE CITED

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