Sesquiterpene Synthases from Grand Fir (Abies grandis)
COMPARISON OF CONSTITUTIVE AND WOUND-INDUCED ACTIVITIES, AND cDNA ISOLATION, CHARACTERIZATION, AND BACTERIAL EXPRESSION OF delta -SELINENE SYNTHASE AND gamma -HUMULENE SYNTHASE*

Christopher L. SteeleDagger §, John CrockDagger , Jörg Bohlmann, and Rodney Croteaupar

From the Institute of Biological Chemistry, Program in Plant Physiology, and Department of Biochemistry and Biophysics, Washington State University, Pullman, Washington 99164-6340

    ABSTRACT
Top
Abstract
Introduction
Procedures
Results
Discussion
References

Grand fir (Abies grandis) has been developed as a model system for the study of oleoresin production in response to stem wounding and insect attack. The turpentine fraction of the oleoresin was shown to contain at least 38 sesquiterpenes that represent 12.5% of the turpentine, with the monoterpenes comprising the remainder. Assays of cell-free extracts from grand fir stem with farnesyl diphosphate as substrate indicated that the constitutive sesquiterpene synthases produced the same sesquiterpenes found in the oleoresin and that, in response to wounding, only two new products were synthesized, delta -cadinene and (E)-alpha -bisabolene. A similarity based cloning strategy yielded two new cDNA species from a stem cDNA library that, when expressed in Escherichia coli and the gene products subsequently assayed, yielded a remarkable number of sesquiterpene products. The encoded enzymes have been named delta -selinene synthase and gamma -humulene synthase based on the principal products formed; however, each enzyme synthesizes three major products and produces 34 and 52 total sesquiterpenes, respectively, thereby accounting for many of the sesquiterpenes of the oleoresin. The deduced amino acid sequence of the delta -selinene synthase cDNA open reading frame encodes a protein of 581 residues (at 67.6 kDa), whereas that of the gamma -humulene synthase cDNA encodes a protein of 593 residues (at 67.9 kDa). The two amino acid sequences are 83% similar and 65% identical to each other and range in similarity from 65 to 67% and in identity from 43 to 46% when compared with the known sequences of monoterpene and diterpene synthases from grand fir. Although the two sesquiterpene synthases from this gymnosperm do not very closely resemble terpene synthases from angiosperm species (52-56% similarity and 26-30% identity), there are clustered regions of significant apparent homology between the enzymes of these two plant classes. The multi-step, multi-product reactions catalyzed by the sesquiterpene synthases from grand fir are among the most complex of any terpenoid cyclase thus far described.

    INTRODUCTION
Top
Abstract
Introduction
Procedures
Results
Discussion
References

Conifer oleoresin is a mixture of turpentine (monoterpene (C10) and sesquiterpene (C15) olefins) and rosin (diterpene (C20) resin acids) that functions in insect defense and in wound sealing (1, 2). Grand fir (Abies grandis) has been developed as a model system for the study of both constitutive and wound-induced oleoresin formation (oleoresinosis). The composition of the monoterpene olefin and the diterpene resin acid fractions of grand fir oleoresin has been defined (3), and the induced biosynthesis of these natural products upon stem wounding has been described in detail (2, 4-6). The time course of induction of the monoterpene synthases involved in turpentine formation has been analyzed by immunoblotting techniques, and the process of induced oleoresinosis was thus shown to involve de novo synthesis of these enzymes (5). The cDNA sequence of a diterpene cyclase from grand fir (abietadiene synthase involved in resin acid biosynthesis (7)) has been reported (8), and several cDNA clones encoding monoterpene synthases from this conifer species have recently become available (9).

The sesquiterpenes of conifer turpentine have received relatively little experimental attention because they constitute less than 10% of the oleoresin. However, sesquiterpenoid phytoalexins are well known in angiosperm species (10), suggesting that the sesquiterpenes of conifer oleoresin may play a similar role in antibiosis and thus be of greater significance than their lower concentration in resin might otherwise indicate. Sesquiterpenes are produced in the cytosol/endoplasmic reticulum compartment, whereas monoterpene and diterpene biosynthesis are compartmentalized in plastids (11), which raises the additional issue of coordinate regulation of oleoresin terpene biosynthesis at several cellular sites. Only a single sesquiterpene synthase, (E)-beta -farnesene synthase, from a gymnosperm source, maritime pine (Pinus pinaster), has been reported (12), whereas several sesquiterpene synthases from angiosperms have been described (13-15), and a number of genes encoding sesquiterpene synthases involved in phytoalexin biosynthesis in angiosperms have been isolated (16-18).

To examine the possible role of sesquiterpenes in conifer defense against stem boring insects and their associated fungal pathogens, it is first necessary to examine in greater detail the origin of these oleoresin constituents. In this paper, we describe the sesquiterpene composition of grand fir oleoresin, and the cell-free biosynthesis of these terpenoids from the common isoprenoid intermediate farnesyl diphosphate in extracts from wounded (induced) and nonwounded control (constitutive) sapling stems. In addition, we report on the use of a general cloning strategy (9, 19) in the isolation and functional expression of two cDNA species encoding sesquiterpene synthases from this gymnosperm. These multiple product enzymes, termed delta -selinene synthase and gamma -humulene synthase based on their corresponding major products, synthesize 34 and 52 sesquiterpene olefins, respectively, and thus constitute the most mechanistically complex terpenoid cyclases to be described thus far from any source.

    EXPERIMENTAL PROCEDURES
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Abstract
Introduction
Procedures
Results
Discussion
References

Plant Materials, Substrates, and Reagents-- Two-year-old grand fir (A. grandis Lindl.) saplings were purchased from the Forestry Research Nursery, University of Idaho, Moscow, ID. Saplings were grown in standard potting mix (Sals Inc., Puyallup, WA) with a 16-h photoperiod (200-300 microeinsteins/m2·s) and a 26 °C day/15 °C night temperature cycle and were fertilized (15:30:15 (N:P:K)) weekly and watered daily. The syntheses of [1-3H]farnesyl diphosphate (125 Ci/mol) (13), [1-3H]geranylgeranyl diphosphate (120 Ci/mol) (7), and [1-3H]geranyl diphosphate (250 Ci/mol) (20) have been reported previously. The sources of authentic sesquiterpene standards were as follows: alpha -longipinene, cyclosativene, sativene, and alpha -ylangene were from Abies balsamea oleoresin; delta -selinene was from Abies alba oleoresin; alpha -, beta -, and gamma -himachalene, alpha - and delta -amorphene, alpha -muurolene, guaia-6,9-diene, alpha -cadinene, delta -selinene, germacrene A, beta -ylangene, beta -longipinene, (E)-alpha - and beta -bisabolene were gifts from Larry Cool (University of California, Berkeley); germacrene B and black pepper oleoresin containing alpha -cubebene and alpha -copaene were gifts from Robert Adams (Baylor University); gamma -humulene was from allspice seeds and as a gift from Ron Binder (USDA, Albany, CA); sibirene and longicyclene were from Pinus sibirica oleoresin; longifolene was purchased from Sigma; (E)-beta -farnesene was from parsley leaf oil; germacrene D was from the essential oil of caraway and Nepeta mussini; beta -caryophyllene was a gift from Rudolf Hopp (Haarmann and Reimer GmbH); gamma -bisabolene was isolated from carrot roots; alpha -humulene was purchased from Fluka Chemical Co.; beta -cubebene was from the essential oil of Valencia orange peels; alpha -selinene and seli-3,7(11)-diene were from celery seed; delta -cadinene was a gift from Margaret Essenberg (Oklahoma State University); alpha -guaiene was from patchouli essential oil; germacrene C was isolated from tomato leaf oil; bicyclogermacrene was from the essential oil of marjoram; and beta -gurjunene was from ginger root. All other biochemicals and reagents were purchased from Sigma or Aldrich, unless otherwise noted.

Oleoresin Isolation and Analysis-- Grand fir sapling stems were sectioned into 2-3-mm discs and extracted overnight with pentane (3.0 ml/g tissue) at room temperature. The pentane extract was decolorized with activated charcoal, washed with water, and passed over a column of MgSO4 and silica gel (Mallinckrodt, type 60A) to remove any traces of water and to bind oxygenated metabolites, thereby providing the turpentine fraction. The oxygenated metabolites were then released from the column by rinsing with diethyl ether. Capillary GLC1 (flame ionization detector) was utilized for identification and quantification of the turpentine monoterpene and sesquiterpene olefin components (Hewlett-Packard model 5890 with cool (40 °C) on-column injection, detector at 300 °C, and H2 carrier at 14 p.s.i.; column: 0.25 mm inner diameter × 30 m fused silica with 0.25-µm film of FFAP (Alltech) programmed from 35 to 50 °C at 50 °C/min (5 min hold) then to 230 °C at 10 °C/min). Capillary GLC-MS was employed to confirm identifications by comparison of retention times and 70 eV mass spectra to those of authentic standards (Hewlett-Packard model 6890 gas chromatograph coupled to a Hewlett-Packard model 5872 mass spectrometer with cool (40 °C) on-column injection, and He carrier at 0.7 ml/min; column: 0.25 mm inner diameter × 30 m fused silica with 0.25-µm film of 5MS (Hewlett-Packard) or polyethylene glycol ester (AT1000, Alltech) and programmed from 40 to 50 °C at 50 °C/min (5 min hold) then to 230 °C at 10 °C/min).

Enzyme Isolation and Assay-- Grand fir saplings in active growth were used as the enzyme source for determination of constitutive terpenoid synthases and of terpenoid synthases induced by stem wounding by a standard protocol (6). Stems from control saplings and saplings 8 days after wounding (usually 10 saplings) were harvested by removing the top and lateral growth and cutting at about 5 cm from the base. The stems were chopped into 5-7-cm segments, frozen in liquid N2, and following removal of any needles were ground to a powder in a liquid N2-chilled number 1 Wiley mill. The frozen powder was added to chilled extraction buffer (5 ml/g fresh tissue weight) consisting of 10 mM dibasic potassium phosphate and 1.8 mM monobasic potassium phosphate (pH 7.3), 140 mM NaCl, 20 mM beta -mercaptoethanol, 10 mM MgCl2, 5 mM MnCl2, 10% (v/v) glycerol, and 1% (w/v) each of polyvinylpyrrolidone (Mr 40,000) and polyvinylpolypyrrolidone. The extract was stirred for 30 min at 0-4 °C and then clarified by centrifugation at 5000 × g and filtration through Miracloth (Calbiochem). Partial purification of the extract was achieved by chromatography on O-diethylaminoethyl-cellulose (Whatman DE52) as described previously (21).

The assay for recombinant sesquiterpene synthase (cyclase) activity was performed in 1 ml of buffer (extraction buffer without MnCl2 or the polymeric adsorbents) containing 3.5 µM [1-3H]farnesyl diphosphate, and the total protein extracted from a 5-ml bacterial culture to produce 105-106 dpm of product in 2 h at 31 °C. The incubation mixture was overlaid with 1 ml of pentane to trap volatile products. After incubation, the reaction mixture was extracted with pentane (3 × 1 ml), and the combined extract was passed through a MgSO4-silica gel column to provide the terpene hydrocarbon fractions as before. The columns were subsequently eluted with 3 × 1 ml of ether to collect any oxygenated products, and an aliquot of each fraction was taken for liquid scintillation counting to determine conversion rate. The monoterpene synthase and diterpene synthase activity assays were similarly performed as described in detail elsewhere (7, 9, 22).

For preparative incubations, the assay was scaled to 5 ml containing the total protein extracted from 100 ml of bacterial culture and 30 µM [1-3H]farnesyl diphosphate, and the incubation time was extended to 8 h. Aliquots of the olefin fraction and the fraction containing oxygenated metabolites (diethyl ether eluate) were evaluated by liquid scintillation counting and were analyzed by radio-GLC (23, 24) using a Gow-Mac 550P chromatograph that was equipped with a 3.18 mm × 3.66 m stainless steel column packed with 5% OV17 (50% phenyl, 50% methylsiloxane) on 100/120 mesh Gas Chrom Q (Alltech) and programmed from 150 to 220 °C at 2 °C/min with He as carrier. The elution of co-injected standards was monitored with the Gow-Mac thermal conductivity detector (250 °C and 150 mA), and the radioactivity signal was continuously monitored with a Nuclear Chicago model 8731 gas proportional counter; output data were processed using Perkin-Elmer Turbochrom Software.

Liquid scintillation counting was performed in 10 ml of toluene:ethanol (7:3, v:v) containing 0.4% (w:v) Omnifluor (NEN Life Science Products) at a 3H counting efficiency of 43%. Protein concentrations were determined by the method of Bradford (25) using the Bio-Rad reagent and bovine serum albumin as standard.

cDNA Isolation, 5'-RACE, and Expression of Sesquiterpene Synthases-- Construction of the wound-induced fir stem cDNA library has been described (8), and the details of hybridization probe generation and library screening are reported elsewhere (9). In summary, hybridization probes for terpenoid synthases were generated by PCR using degenerate oligonucleotide primers designed from conserved amino acid sequences (designated in boldface in Fig. 7) of several monoterpene, sesquiterpene, and diterpene synthases from angiosperm species (19). DNA from a lambda  phage cDNA library, constructed from mRNA isolated from wounded grand fir sapling stems (8), was purified and used as template for PCR reactions (26). Four unique, 110-bp fragments were amplified, cloned, and shown to be cyclase-like in sequence, and they were designated probes 1, 2, 4, and 5. Upon screening of the cDNA library, probes 4 and 5 hybridized, respectively, to two unique cDNA species designated ag4.30 and ag5.9; the location of each probe is doubly underlined in the sequences illustrated in Fig. 7.

Since neither of the cDNA isolates encoded a starting methionine, 5'-RACE was carried out using the Marathon cDNA amplification kit (CLONTECH) by following the manufacturer's protocol with slight modification (see below). Total RNA was extracted from 60 saplings (2-year-old; 6 or 8 days after wounding) by scale-up of a published procedure (27). Poly(A)+ mRNA was isolated using Oligotex beads and the spin column procedure described by Qiagen. To prevent RNA secondary structural features from obstructing full-length cDNA synthesis, three different cDNA synthesis reactions were performed by first denaturing the RNA at 42 or at 50 °C or by treatment with methylmercury hydroxide (28). Twice as much mRNA (2 µg) as recommended in the protocol was used, and PCR amplification was performed as indicated, except that a low fidelity Taq polymerase was substituted. The respective cDNA-specific reverse PCR primers were 5'-CTGCGAACCTTGAGAGTGGTCTGCAG-3' for ag4.30 and 5'-GTCTATCGATTCCCAGCCATTCC-3' for ag5.9. The resulting PCR products were cloned into the pT7Blue-vector (Novagen) following standard procedures, and they were partially sequenced to reveal in each case a putative starting methionine codon, thus indicating that successful 5'-RACE syntheses had occurred. Full-length representatives were generated by designing 5'- and 3'-specific PCR primers for each cDNA for subsequent high fidelity amplification. The 5'-specific primers were designed with a BamHI restriction endonuclease site immediately upstream of the starting methionine codon for each cDNA (5'-GGAGGATCCATGGCTGAGATTTCTG-3' for ag4.30 and 5'-TGGTACCATGGCTGGCGTTTCTGCTGTATC-3' for ag5.9). The 3'-specific primers were designed to encompass the stop codon; the ag4.30 primer included an XhoI site, whereas the ag5.9 primer included an EcoRI site (5'-AAAGTCTCGAGATATTAATTATTGCC-3' for ag4.30 and 5'-TATGAATTCTCAAATAGGCACGGGGAC-3' for ag5.9) to facilitate ligation into the pGEX-4T-1 expression vector (Pharmacia Biotech Inc.). PCR reactions were performed at 94 °C for 1 min, 50 °C for 1 min, and 72 °C for 6 min for 30 cycles followed by a 5-min final extension period at 72 °C, using Pfu polymerase and the buffer described by the manufacturer (Stratagene). The resulting DNA fragments were sequentially cloned by standard methods, first into pBluescript (SK-) (Stratagene) and then into pGEX (Pharmacia) vectors designated as pGAG4 and pGAG5. For further subcloning of cDNAs into the pSBETa vector for high level expression (29), inserts of pGAG4 and pGAG5 were amplified by PCR (Stratagene Pfu polymerase as above) using primer combinations 4-NdeI (5'-CTGGTTCCGCGTGGACATATGGCTGAGT-3') and 4-BamHI (5'-CTACAACCAAGAGGATCCCTATTCCTCCATTGG-3') with pGAG4, and 5-NdeI (5'-CTGGTTCCGCGTGGACATATGGCTCAG-3') and 5-BamHI (5'-GTCAGTGACGATGGATCCTCAAATAGGCACGG-3') with pGAG5. The PCR products were digested with the above indicated restriction enzymes, purified by ultrafiltration, and then ligated into NdeI/BamHI-digested pSBETa to yield plasmid pSBAG4 and pSBAG5, respectively.

The original isolates, ag4.30 and ag5.9, and their full-length cDNA representatives, inserts of ag4 in pGAG4 and pSBAG4, and of ag5 in pGAG5 and pSBAG5, were entirely sequenced on both strands via primer walking using the dye-terminator-cycle sequencing method (Applied Biosystems) on a ABI 373 DNA Sequencer Stretch instrument at the Washington State University Laboratory for Biotechnology and Bioanalysis. Sequence analysis was done using programs from the Wisconsin Package Version 9.0 of the Genetics Computer Group (30).

Both putative sesquiterpene cyclase cDNAs were expressed in bacterial strains Escherichia coli XL1-Blue/pGAG4, E. coli XL1-Blue/pGAG5, E. coli BL21(DE3)/pSBAG4, and E. coli BL21(DE3)/pSBAG5. Bacteria were grown to A600 = 0.5 at 37 °C in 5 ml or 100 ml of LB medium supplemented with 100 µg of ampicillin/ml or 30 µg of kanamycin/ml as determined by the vector. Cultures were then induced by addition of 1 mM isopropyl-1-thio-beta -D-galactopyranoside and grown for another 12 h at 20 °C. Cells were harvested by centrifugation (2000 × g, 10 min) and resuspended in either 1 or 5 ml of sesquiterpene synthase assay buffer. Cells were disrupted by sonication (Braun-Sonic 2000 with microprobe at maximum power for 15 s at 0-4 °C), and the homogenates were cleared by centrifugation (18,000 × g, 10 min). Preparative assays were employed to generate product for GLC-MS analysis as before, with quantification of composition via the total ion current chromatogram.

    RESULTS
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Abstract
Introduction
Procedures
Results
Discussion
References

Oleoresin Sesquiterpenes-- Grand fir has been utilized as a model system for the study of induced oleoresin production in conifers in response to wounding and insect attack (19). The monoterpene and diterpenoid components of the oleoresin have been defined, and several of the responsible monoterpene and diterpene synthases have been purified and characterized and the corresponding cDNAs isolated to provide tools for examining the regulation of this defense response (6-9, 21). The third component of the oleoresin, the sesquiterpenes, has not been examined in any detail as it comprises the smallest fraction of the defensive secretion. Capillary GLC-MS analysis of grand fir stem turpentine revealed a minimum of 38 sesquiterpenes constituting approximately 12.5% of this material, with the remaining 87.5% composed of previously identified monoterpenes (3). The six major sesquiterpenes present are alpha -cubebene, alpha -copaene, beta -caryophyllene, alpha -muurolene, delta -cadinene and (E,E)-germacrene B, representing 62% of the total sesquiterpene fraction (Fig. 1). delta -Selinene, guaia-6,9-diene, delta -amorphene, sibirene, gamma -humulene, longifolene, alpha -, beta -, and gamma -himachalene, alpha -longipinene, beta -bisabolene, alpha -ylangene, sativene, and cyclosativene were also identified (~33% of the sesquiterpene fraction), with the remaining minor fraction (~5%) composed of some 20 as yet unidentified sesquiterpene olefins.


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Fig. 1.   Structures of the six major sesquiterpene olefins of grand fir turpentine. The percentage contribution to the total sesquiterpene fraction is indicated in parentheses. The stereochemistry illustrated is relative.

Sesquiterpene Synthases-- To examine the sesquiterpene synthases of grand fir, a soluble enzyme extract from non-wounded (control) sapling stems was prepared by methods previously employed in the study of monoterpene and diterpene synthases from this tissue (7, 31). These preparations catalyzed the divalent metal ion-dependent conversion of [1-3H]farnesyl diphosphate, the universal precursor of sesquiterpenoids (32, 33), to a labeled olefin fraction (12 × 2 ml assays yielded ~1.6 nmol of product) that upon radio-GLC analysis (Fig. 2a) was shown to contain the same spectrum of sesquiterpenes found in the oleoresin. Enzyme extracts were similarly prepared from sapling stems 9 days after wounding and were assayed as before (2 × 2 ml assays yielded 1.8 nmol of product). Radio-GLC analysis of the olefin fraction revealed the presence of an apparently single component with retention time very similar to that of delta -cadinene (Fig. 2b). Partial purification of the extract from induced saplings to eliminate traces of endogenous oleoresin, followed by preparative-scale assay, provided sufficient material for capillary GLC-MS analysis. This higher resolution method revealed that the product derived from farnesyl diphosphate by the induced enzyme(s) consisted of two components that were identified as delta -cadinene and (E)-alpha -bisabolene. Differential loss of the delta -cadinene synthase activity during storage (data not shown) suggested that delta -cadinene and (E)-alpha -bisabolene were the products of two different enzymes. Boiled controls, and control reactions without farnesyl diphosphate, confirmed that both the constitutive and inducible sesquiterpene synthase activities observed were enzymatic and substrate-dependent. The Km value for [1-3H]farnesyl diphosphate with the partially purified inducible sesquiterpene synthases was determined to be about 0.4 µM. It is of interest, and of probable physiological significance,2 that the constitutive sesquiterpene synthase activities differ from the wound-induced enzyme activities in product composition. A similar phenomenon has been previously observed with the constitutive and wound-inducible monoterpene and diterpene synthases of this tissue (6, 21).


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Fig. 2.   Radio gas-liquid chromatographic analysis of the products generated from [1-3H]farnesyl diphosphate by soluble enzyme preparations from non-wounded (control, constitutive) grand fir sapling stems (A) and from wounded (induced) grand fir sapling stems (B). The upper tracing in A and B is the radioactivity detector response, and the lower smooth tracing is the thermal conductivity detector (mass) response to co-injected grand fir oleoresin as internal standard (alpha -cubebene (a), alpha -copaene (b), beta -caryophyllene (c), alpha -muurolene (d), delta -cadinene (e), (E,E)-germacrene B (f)). The time scale for analyses A and B differs slightly, as the ramp temperature and column pressure were lowered in an attempt to achieve higher resolution in the latter case. Inset C illustrates the high resolution capillary gas chromatographic separation (flame ionization detection) of the products (delta -cadinene and (E)-alpha -bisabolene) generated from farnesyl diphosphate by the wound-inducible sesquiterpene synthases following partial purification of the preparation to remove traces of endogenous oleoresin.

cDNA Isolation and Expression-- A similarity-based PCR cloning strategy for terpenoid synthases (9) yielded two different truncated cDNA species, ag4.30 and ag5.9, upon screening a grand fir stem cDNA library. The full-length forms, ag4 and ag5, were acquired by a 5'-RACE technique, and both of these, and the original cDNA isolates, were sequenced completely on both strands. Sequence similarity to other terpenoid synthases of plant origin (see below) and the apparent lack of an encoded plastidial transit peptide characteristic of both monoterpene and diterpene synthases (8, 9, 34) suggested that the two new sequences represented sesquiterpene synthases. The sequences of ag5.9 and ag5 were identical to each other; however, comparison of the ag4.30 cDNA to ag4 indicated six nucleotide differences resulting in three amino acid changes from ag4.30 to ag4 at positions 47 (Glu to Gln), 437 (Val to Leu), and 447 (Gly to Asp) (see Fig. 7). These differences may represent alleles in the tetraploid genome or members of a small gene family but are more likely to simply reflect polymorphic variation within the 120 individual trees used in cDNA library construction.

Both ag4 and ag5 were expressed in E. coli using pGEX and pSBET (29) vectors; the latter encodes a tRNA for rare arginine codon usage in E. coli that is common in higher plants. Levels of expressed enzyme activity were 50 to 100 times higher in extracts from E. coli BL21(DE3)/pSBAG4 and E. coli BL21(DE3)/pSBAG5 as compared with extracts from E. coli XL1-Blue/pGAG4 and E. coli XL1-Blue/pGAG5. Therefore, for subsequent product identification, recombinant enzymes were produced with pSBET expression constructs in E. coli BL21(DE3). Large scale incubation with [1-3H]farnesyl diphosphate, followed by isolation of the derived olefins and GLC-MS analysis (Fig. 3), revealed the enzyme encoded by ag4 to produce mainly delta -selinene, for which this synthase is named, along with germacrene B and guai-6,9-diene as major products. In addition, 17 other sesquiterpene olefins were identified by GLC-MS, and another 14 products which displayed the characteristic sesquiterpene olefin mass spectral pattern (m/z 204 (P+), 189 (P+-CH3), and 161 (P+-C3H7)) were detected for a total of at least 34 different sesquiterpene products (Table I).


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Fig. 3.   Total ion chromatograms of the sesquiterpene products derived from farnesyl diphosphate by delta -selinene synthase (ag4) (A) and gamma -humulene synthase (ag5) (H). In the column below each total ion chromatogram are the mass spectra and retention times for the numbered peaks and the spectra and retention times for the corresponding authentic standards.

                              
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Table I
Sesquiterpene products of delta -selinene synthase (ag4) and gamma -humulene synthase (ag5)
Products are listed in order of their abundance and were identified by matching GLC retention time and mass spectrum to authentic standards. Compounds labeled as (tent.) were tentatively identified based on the mass spectrum alone.

A cyclization scheme to account for the generation of this remarkable number of products has been formulated (Fig. 4) and begins with the ionization and subsequent isomerization of (E,E)-farnesyl diphosphate to the corresponding tertiary allylic isomer, nerolidyl diphosphate, a process known to occur in the biosynthesis of other sesquiterpenes (33). The route to the principal product, delta -selinene, is based upon the formation of other eudesmane sesquiterpenes (32, 33, 35) and is initiated by ionization of the transoid-conformer of nerolidyl diphosphate, with C-10 to C-1 (farnesyl backbone numbering) ring closure, to afford the germacrane skeleton from which deprotonation yields germacrenes A and B or (following hydride shift) germacrenes C and D. These germacrenes may be released by the synthase (they account for 28.3% of the olefins generated) or they may be reprotonated to allow for additional ring closures (at least 58% of the carbon flux involves reprotonation). Reprotonation at C-6 restricts carbon flow to the eudesmane-structural types, whereas protonation at C-3 directs flux to the azulane (guaiane)-structural types. After protonation, the fate of the intermediates generated is determined by the position of the terminal double bond formed during germacrene biosynthesis. Although only the products of C-3 protonation of germacrene A and C were found, it is likely that both germacrene B and D also undergo protonation at C-3 to yield products that are not yet identified (Table I). Each of the germacrenes yields a product derived by protonation at C-6 (Fig. 4). Closure of the transoid-nerolidyl cation to the C11 macrocyclic cation provides for formation of both alpha -humulene and beta -caryophyllene (Fig. 4). Similar closure of the cisoid-nerolidyl cation also allows formation of beta -caryophyllene, the only identified olefin from this synthase that can be produced via either cisoid- or transoid-nerolidyl diphosphate.


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Fig. 4.   Proposed mechanism for sesquiterpene formation by delta -selinene synthase (ag4). Numbering of the farnesyl system is indicated, and OPP denotes the diphosphate moiety. Structures enclosed in boxes indicate products that have been identified by GLC-MS.

Carbon flow through the cisoid-nerolidyl diphosphate pathway accounts for approximately 13% of the products identified (Table I). Besides closure to the C11 macrocycle, C-6 to C-1 closure of this intermediate may also occur to form beta -bisabolene, in a reaction analogous to the formation of the monoterpene limonene by limonene synthase (34); no other isomers of bisabolene were detected. The C-10 to C-1 closure leads to a (Z,E)-intermediate that may deprotonate to form (Z,E)-germacrene B. Although this compound has not been reported from a natural source, it is analogous to the naturally occurring helminthogermacrene or (Z,E)-germacrene A (36). (Z,E)-Germacrene B was tentatively identified as an enzyme product based on an exact mass spectral match to (E,E)-germacrene B and a similar GLC retention time (data not shown). Although the mass spectrum of gamma -elemene is very similar to that of germacrene B, and the former is the Cope rearrangement product of germacrene B, the GLC retention time of gamma -elemene is much earlier than that of germacrene B. Likewise, although bicyclogermacrene (the tricyclic, dimethylcyclopropyl analog of germacrene B) has a mass spectrum similar to (E,E)-germacrene B, the GLC retention time did not match that of the putative (Z,E)-germacrene B. Given the mass spectrometric and GLC retention data, and the fact that the enzyme can deprotonate the (E,E)-intermediate to form (E,E)-germacrene, it seems likely that (Z,E)-germacrene is, in fact, a product of the delta -selinene synthase.

1,3-Hydride shift in the (Z,E)-germacryl cation, followed by C-6 to C-1 ring closure and subsequent deprotonation, provides alpha - and delta -cadinene and the diastereomers alpha - and delta -amorphene. The cadinyl cation may further cyclize to the tricyclic diastereomers, alpha -ylangene and alpha -copaene, through ring closure from C-2 to either the si or re face of C-7. Apparently, attack from C-3 of the cadinyl cation is forbidden, since this would yield cubebenes or sativenes which have not been detected as enzymatic products. It is noteworthy that many of the minor products of the delta -selinene synthase also occur as minor products in the volatiles of guava (Psidium guajava) leaves, which is also a source of delta -selinene (37). It may be that the co-occurrence of this spectrum of minor products reflects a common reaction mechanism for the delta -selinene synthases of grand fir and gauva.

Although the array of products generated by delta -selinene is remarkable, an even more bewildering spectrum of sesquiterpene olefins is produced by the synthase encoded by ag5. gamma -Humulene, the principal olefin for which this synthase has been named, sibirene, and longifolene were identified by GLC-MS analysis (Fig. 3) as major products. In addition, 23 other sesquiterpenes were identified, along with 26 unknown sesquiterpene olefins, for a total of 52 different products (Table I). These products range in complexity from the simple acyclic olefin (E)-beta -farnesene to the complex tetracyclic olefins longicyclene and cyclosativene.

Whereas delta -selinene synthase appears to utilize both cisoid- and transoid-nerolidyl diphosphate as cyclization intermediates, the gamma -humulene synthase may utilize exclusively cisoid-nerolidyl diphosphate (Fig. 5). Thus, with delta -selinene synthase, most of the germacrenes produced bear a trans-C2,C3-double bond, thereby revealing the transoid nature of the nerolidyl diphosphate intermediate. By contrast, none of the 26 identified products of gamma -humulene synthase bear a trans-C2,C3-double bond, suggesting that the reaction cascade (Fig. 5) proceeds entirely from cisoid-nerolidyl diphosphate, even in the formation of the acyclic olefin (E)-beta -farnesene and of sibirene and beta -gurjunene which, as eudesmanes, are usually considered to originate via the transoid intermediate (32, 33, 35).


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Fig. 5.   Proposed mechanism for sesquiterpene formation by gamma -humulene synthase (ag5). Numbering of the farnesyl system is indicated, and OPP denotes the diphosphate moiety. Structures enclosed in boxes indicate products that have been identified by GLC-MS. WMR indicates a Wagner-Meerwein rearrangement.

In the proposed reaction scheme (Fig. 5), C-6 to C-1 closure followed by deprotonation will produce the various bisabolenes in a manner analogous to the corresponding monoterpene cyclization (34). All remaining cyclizations catalyzed by this enzyme require C-11 to C-1 closure to form a C11 macrocycle (humulene cation) or C-10 to C-1 closure to produce a C10 macrocycle in (Z,E)-configuration (Fig. 5). Approximately 62% of the reaction flux is shuttled through the C11 macrocycle and 25% is directed through the C10 macrocycle. The C10 macrocycle can be deprotonated directly to form (Z,E)-germacrene B, which is also produced by delta -selinene synthase. Hydride shift and deprotonation of the cyclodecadienyl cation from the C-3-methyl (C-15) leads to germacrene D, which, following reprotonation at C-6, allows C-2, C-7 ring closure to the eudesmane skeleton of sibirene. In the production of beta -gurjunene, cyclopropane ring formation precedes protonation (at C-6) and C-2, C-7 closure, and is followed by an additional hydride shift and methyl migration before deprotonation to complete the reaction. In the formation of sibirene and beta -gurjunene, the original cis-configuration of the macrocyclic intermediate is obscured in the transformations.

If the 1,3-hydride shift in the (Z,E)-C10 macrocycle is followed by C-6 to C-1 closure, the amorphenes (but apparently not the diastereomeric cadinenes) can be formed by deprotonation, whereas subsequent C-2 (or C-3) to C-7 closure via the remaining double bond yields copaenes and ylangenes, as with delta -selinene synthase, or sativene and cyclosativene. The formation of sativene, and possibly cyclosativene, must occur via Wagner-Meerwein rearrangement involving a cation-induced 1,2-carbon shift, analogous to the 1,2-methyl shift that occurs in the formation of beta -gurjunene.

In the case of the C11 macrocyclic cation, 1,3-hyride shift and deprotonation from C-3 will afford gamma -humulene (Fig. 5), in a manner analogous to the formation of germacrene D from the C10 macrocycle. Ring closure from C-6 to C-1 of the humulyl cation provides the himachalyl cation, from which three alternatives for deprotonation yield alpha -, beta - and gamma -himachalenes in which the cisoid conformation at C-2,C-3 of the original nerolidyl intermediate is preserved. Ring closure from C-2 to C-7 of the himachalyl cation leads to alpha - and beta -longipinene, whereas closure from C-3 to C-7, with Wagner-Meerwein rearrangement, leads to longifolene and longicyclene. These additional ring closures, via the double bond of the bicyclo[5:4:0](himachalyl) cation, are analogous to the closures of the bicyclo[4:4:0](cadinyl/amorphyl) cation involved in the formation of the copaenes and sativenes. Similarly, the Wagner-Meerwein rearrangement involved in the formation of sativene (and possibly cyclosativene) is analogous to that which occurs in the formation of longifolene (and possibly longicyclene). Zavarin and co-workers (38) have previously identified gamma -humulene in the cortical oleoresin of many Abies species, including A. grandis, and have suggested that this macrocyclic olefin is a by-product of longifolene biosynthesis.

Although gamma -humulene synthase appears to be restricted to utilization of the cisoid-nerolidyl diphosphate intermediate, as opposed to delta -selinene synthase which utilizes both cisoid and transoid forms, the former is able to catalyze formation of the greater number and the more diverse products, including acyclic, monocyclic, bicyclic, tricyclic, and tetracyclic types, as well as olefins produced by Wagner-Meerwein rearrangements. It is worth noting that, despite the remarkable number of different sesquiterpene skeletal types generated by these two enzymes, deprotonation in each set of structures occurs from the same few carbons of the common substrate, providing at least some measure of uniformity between the two and suggesting the involvement of a limited number of enzyme bases in catalysis. The gamma -humulene synthase, in particular, catalyzes several very complex reaction cascades and generates far more products than any terpenoid synthase thus far described, and it along with delta -selinene synthase account for many of the constitutively produced cortical sesquiterpenes. However, the cDNA species encoding synthases responsible for the formation of several of the more abundant constitutive sesquiterpenes of grand fir oleoresin (e.g. alpha -muurolene, alpha -copaene, alpha -cubebene, and beta -caryophyllene) have not yet been acquired. Although (E)-alpha -bisabolene is a product of gamma -humulene synthase, and delta -cadinene is a product of delta -selinene synthase, these two sesquiterpenes account for only a small fraction of the many olefins generated by these two synthases. Thus, gamma -humulene synthase and delta -selinene synthase cannot be responsible for the wound-induced production of (E)-alpha -bisabolene and delta -cadinene.

Sesquiterpene Synthase Characterization-- The Km values for [1-3H]farnesyl diphosphate with gamma -humulene synthase and delta -selinene synthase were estimated to be about 4.5 and 1.5 µM, respectively. The metal ion requirements of gamma -humulene synthase and delta -selinene synthase were also evaluated, as cofactor specificity is often characteristic of the different terpenoid synthase types (39). delta -Selinene synthase shows a distinct preference for Mg2+; the maximum rate with Mn2+ is less than 10% of that with Mg2+ at saturation. By contrast, gamma -humulene synthase can utilize Mg2+ or Mn2+ with comparable velocities in the cyclization reaction. For both enzymes, the Km value for Mg2+ is about 125 µM and for Mn2+ about 25 µM. Neither of the sesquiterpene synthases requires K+ or other monovalent cation for activity. The monoterpene synthases from conifers require Mn2+ or Fe2+ for activity, but Mg2+ fails to support catalysis (9, 40), and these enzymes also exhibit an absolute requirement for a monovalent cation, with K+ preferred (9, 39).

Substrate specificity of these sesquiterpene synthases was evaluated by comparing farnesyl diphosphate to geranyl diphosphate (C10) and geranylgeranyl diphosphate (C20) at saturation as precursors of the respective terpene olefins. Both enzymes failed to generate detectable olefinic products from geranylgeranyl diphosphate, whereas both synthesized monoterpenes from geranyl diphosphate at roughly half the rate of sesquiterpene biosynthesis from farnesyl diphosphate. The identities of the monoterpene products produced by the sesquiterpene synthases were determined by GLC-MS. Limonene is the principal monoterpene product of both synthases (see Fig. 6 for product structures and amounts), with most of the other products being made in roughly comparable proportions by each, with the notable exception of (Z)-ocimene which is a major product of delta -selinene synthase (22.4%) but is not detectable as a product of gamma -humulene synthase. gamma -Humulene synthase produces detectable amounts of camphene, the biosynthesis of which requires a Wagner-Meerwein rearrangement as with longifolene and sativene; delta -selinene synthase does not produce this monoterpene.


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Fig. 6.   Structures of the monoterpene olefins generated from geranyl diphosphate by delta -selinene synthase and gamma -humulene synthase. The percentage contribution to the total monoterpene fraction is indicated in parentheses for the delta -selinene synthase and gamma -humulene synthase, respectively. ND means not detected.

Sequence Analysis-- The delta -selinene synthase cDNA encodes a protein that is 581 amino acids in length with a predicted molecular weight of 67,625, and the gamma -humulene synthase cDNA encodes a protein of 593 residues with a predicted molecular weight of 67,937 (Fig. 7). The gamma -humulene synthase sequence contains a stop codon in frame with the putative initiation methionine at -21 bp of the 89-bp 5'-untranslated region, whereas the delta -selinene synthase sequence is truncated at -12 bp. The nucleotide sequence surrounding the putative starting ATG of both sesquiterpene synthase genes is conserved and resembles that which surrounds the initiating methionine of other plant genes (41). These data support the proposed location of the initiation sites and, thus, the identification of both cDNAs as sesquiterpene synthases, since the predicted molecular weights are appropriate for this class of cytosolic enzymes (16, 18) which lack a plastidial targeting peptide found in both monoterpene synthase and diterpene synthase preproteins (8, 9, 34, 42).


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Fig. 7.   Comparison of the deduced amino acid sequences of gamma -humulene synthase (ag5) (top) and delta -selinene synthase (ag4) (bottom). Conserved histidine, cysteine, and arginine residues (from comparison of all sesquiterpene synthase sequences published to date) are indicated by single arrows. Regions of sequence that were used to design PCR primers are indicated in boldface, and the amino acids encoded by the nucleotide probes that were used to isolate the corresponding full-length cDNAs are doubly underlined. The six clustered regions of high similarity found among angiosperm sesquiterpene synthases (after Chen et al. (18)) are boxed and numbered, and the domain boundaries (for domains 1-3, 4, 5, 6, and 7) corresponding to those described by Back and Chappell (54) are indicated by double arrows.

Comparison of the deduced amino acid sequences indicates that they are 83% similar and 65% identical to each other (Fig. 7), and both sesquiterpene synthases show about 66% similarity and 45% identity when compared with other terpenoid synthases from conifers, including abietadiene synthase (diterpene) from grand fir (8), myrcene synthase, pinene synthase, and limonene synthase (monoterpenes) from this species (9), and the taxadiene synthase (diterpene) from Pacific yew (43). Comparison of these gymnosperm sesquiterpene synthases to a range of terpenoid synthases from angiosperm species (17, 18) reveals similarities of about 56% and identities in the range of 30%. Interestingly, the gymnosperm sesquiterpene synthases show a greater resemblance to gymnosperm monoterpene synthases and diterpene synthases than they do to angiosperm sesquiterpene synthases, suggesting an ancient divergence of the gymnosperm tpsd family (9), which consists of monoterpene, sesquiterpene, and diterpene synthases. Comparison with microbial sesquiterpene synthases evidenced no significant similarity. For example, the delta -selinene and gamma -humulene synthases show 45-46% similarity and 18-22% identity when compared with trichodiene synthase from Fusarium sporotrichioides (44).

Studies employing amino acid-modifying reagents have implicated histidine, cysteine, and arginine residues in catalysis by terpene synthases from angiosperms and gymnosperms (7, 13, 14, 39, 40, 45-47). Comparisons of all published terpene synthase sequences reveal Cys507 (with reference to gamma -humulene synthase) as the only universally conserved cysteine residue, and His95 and His141 as the only conserved histidines. However, comparisons between only the sesquiterpene synthases reveal an additional conserved histidine residue at position 283. Comparison among the sesquiterpene synthases also shows that eight arginine residues are conserved at positions 136, 139, 243, 247, 306, 329, 364, and 485 of gamma -humulene synthase, a surprising number considering the broad taxonomic distribution of plant species compared (16-18).

The clustering of conserved regions among the terpenoid synthases of higher plant origin is notable. Chen and associates (18) have recognized six such regions of high conservation (indicated by boxing in Fig. 7). The first region from the amino terminus contains two of the conserved arginine residues, as well as one of the conserved histidines. The third region contains the highly conserved aspartate-rich motif (DDXXD) which is found in all terpenoid synthases, including those of microbial origin, as well as in prenyltransferases (48) which operate by a related mechanism on the common prenyl diphosphate substrates (49-51). Considerable evidence based on x-ray structural investigation and directed mutagenesis indicates that this motif is responsible for binding the divalent metal ion of the substrate diphosphate-metal ion complex (52, 53). The sixth region also contains a DDXXD motif (Fig. 7) of which the second aspartate residue is conserved among terpenoid synthases; the last aspartate residue is found only in the grand fir sesquiterpene synthases.

Back and Chappell (54) have conducted domain swapping experiments between two eudesmane-type sesquiterpene synthases, epi-aristolochene synthase from Nicotiana tabacum and vetispiradiene synthase from Hyoscyamus muticus, in an attempt to determine the function of each domain in these related cyclization reactions. The first three common domains (the corresponding domain boundaries, which roughly define exon boundaries, are demarcated by double arrows in Fig. 7) share a high degree of similarity (71.5%) with the corresponding regions of gamma -humulene synthase and delta -selinene synthase (i.e. amino acids 1-301/299 comprise the first three domains), whereas the remaining domains (4 (aa 301-382), 5 (aa 382-420), 6 (aa 420-484), and 7 (aa 484-593)) decrease in similarity from 66.6 to 50.9% in approaching the carboxyl terminus.

    DISCUSSION
Top
Abstract
Introduction
Procedures
Results
Discussion
References

The analysis of the sesquiterpene fraction of grand fir oleoresin reported here for the Rocky Mountain ecotype agrees well with a previous analysis of this material from the coastal ecotype (38) with but minor differences between the former (19% germacrene B without detectable beta -elemene) and the latter (8% beta -elemene without detectable germacrene B). The discrepancy is likely the result of misidentification due to methodology (identification of beta -elemene by retention time only) and has been rectified by recent re-analysis of the oleoresin of the coastal ecotype.3 Upon stem wounding, two sesquiterpene synthase activities are induced, one for the increased production of a prominent constitutive component (delta -cadinene; see Fig. 1) and one for the production of a very minor sesquiterpene of the constitutive oleoresin ((E)-alpha -bisabolene). This situation is reminiscent of that observed with the constitutive and inducible monoterpene synthases of grand fir (4, 6, 21).

Although delta -selinene synthase and gamma -humulene synthase are capable of producing monoterpenes when presented with geranyl diphosphate, several lines of evidence indicate that these enzymes are, in fact, sesquiterpene synthases. First, the corresponding cDNA species do not appear to encode preproteins bearing a plastidial transit peptide characteristic of monoterpene (and diterpene) synthases but rather mature proteins of a size typical of this class of cytosolic enzymes. Second, the divalent and monovalent ion requirements do not resemble those of the monoterpene synthases but rather those of other sesquiterpene synthases. Finally, the acyclic monoterpenes (ocimenes) produced by delta -selinene synthase and gamma -humulene synthase from geranyl diphosphate are not found in the turpentine fraction of grand fir oleoresin (3, 22, 38). The accumulated evidence therefore clearly supports the identification of these enzymes as sesquiterpene synthases. Since sesquiterpene biosynthesis occurs in the cytosol where the precursor farnesyl diphosphate is also synthesized, whereas the monoterpene synthases are compartmentalized within plastids where the precursor geranyl diphosphate also arises (11, 34, 55, 56), the ability of the sesquiterpene synthases to produce monoterpenes in vitro may simply represent the adventitious utilization of a substrate that is never encountered in vivo and against which there is no evolutionary pressure to discriminate. It now seems likely that the adventitious utilization of geranyl diphosphate by the sesquiterpene synthases accounts, in part, for the relatively high level of limonene synthase activity observed in crude stem extracts of grand fir (21).

The ability of terpene synthases to produce multiple products has been well documented (14, 39, 40, 47, 57) and may be a consequence of the unusual electrophilic reaction mechanisms employed by this enzyme type (11, 35, 58) that may also represent an evolutionary adaptation for the production of the maximum number of terpene products using the minimum genetic and enzymatic machinery (59). Nevertheless, the production of 34 different sesquiterpenes by delta -selinene synthase and 52 discrete sesquiterpenes by gamma -humulene synthase, by variations upon several different cyclization routes, is quite remarkable. The reaction cascade catalyzed by gamma -humulene synthase is particularly complex in generating (by deprotonation) stable olefinic end products corresponding to many of the proposed carbocationic intermediates of each cyclization route (Fig. 5). Significantly, the essential elements of these cyclization schemes have been delineated by Arigoni and collaborators (32, 60, 61) via a series of elegant in vivo labeling studies directed toward the biosynthesis of longifolene and sativene in the fungi Helminthosporium (victoria or sativum) or the gymnosperm Pinus ponderosa. Additionally, in vivo studies with (5R)- and (5S)-[5-3H]mevalonate provided evidence, based upon the observation of isotopically sensitive branching (62), that the formation of (-)-longifolene and (-)-sativene was catalyzed by a single enzyme. The isolation and functional expression of the gamma -humulene synthase cDNA reported here provides direct and unequivocal proof for this earlier, prescient biosynthetic proposal (60, 61).

Sequence comparison between the delta -selinene synthase and the gamma -humulene synthase indicates that the two enzymes are very similar, but with the similarity decreasing toward the carboxyl terminus of the proteins. This observation is consistent with the conclusions drawn from domain swapping experiments with related sesquiterpene synthases (54) which suggest that the amino-terminal regions of the proteins are involved in the initial, common steps of the cyclization reactions and that the more carboxyl-terminal regions are responsible for determining the specific product outcome. The two gymnosperm sesquiterpene synthases clearly resemble in sequence the angiosperm terpenoid synthases (roughly 55% similarity and 30% identity), with levels of conservation similar to those observed between the angiosperm sesquiterpene and diterpene synthases and the monoterpene synthases of this plant class (9, 18). The regions of highest similarity between the various terpenoid synthases are clustered and likely represent those elements responsible for common cyclization chemistry (e.g. ionization, charge stabilization, and deprotonation). The more variable regions likely impart the specific shape of the active site that enforces substrate and intermediate conformation and thus dictates the specific product outcome. The crystal structures of two sesquiterpene cyclases have recently been described for pentalenene synthase from Streptomyces UC5319 (63) and epi-aristolochene synthase from tobacco (64). Both enzymes have been shown to possess very similar fold structures related to farnesyl diphosphate synthase (52) and to consist of mostly antiparallel alpha -helices that form a large central cavity. Modeling studies with other terpenoid cyclases have been initiated (64), and it should soon be possible to compare the predicted structures of the multiple product sesquiterpene synthases of grand fir to these defined single product synthases and to perhaps reveal the structural basis for fidelity (or the lack thereof) in these cyclization reactions.

The cDNAs encoding delta -selinene synthase and gamma -humulene synthase provide tools for evaluating the transcriptional regulation of sesquiterpene biosynthesis in the context of constitutive oleoresin formation and, along with bacterial expression systems, the means for examining structure-function relationships in these mechanistically fascinating catalysts. These cDNAs should also provide access to genomic clones to allow comparison of intron/exon structure of these genes to their angiosperm counterparts (40, 65). Grand fir is the first plant from which cDNA species encoding representative monoterpene, sesquiterpene, and diterpene synthases have been isolated (8, 9). Although the sequence comparisons are in themselves instructive, the availability of these clones should permit a more highly refined understanding of oleoresinosis and lead to the manipulation of this defensive secretion in the protection of conifer species against the devastating environmental and economic effects of bark beetle predation (1, 2, 66, 67).

    ACKNOWLEDGEMENTS

We thank Larry Cool, Ron Binder, Robert Adams, Margaret Essenberg, and Rudolf Hopp for the gifts of sesquiterpene reference standards; Jack Alexander of the Harvard Arnold Arboretum for the gift of A. alba tissue; Joyce Tamura-Brown for typing the manuscript; and Thom Koehler for raising the trees. We thank Eva Katahira for technical assistance and Gerhard Munske of the Laboratory for Biotechnology and Bioanalysis for DNA sequencing. We are especially grateful to Larry Cool (Forest Products Laboratory, University of California, Berkeley) for expert assistance in the identification of the sesquiterpenes from grand fir oleoresin.

    FOOTNOTES

* This work was supported in part by National Institutes of Health Grant GM 31354, Dept. of Agriculture NRI Grant 97-35302-4432, the Tode Foundation, and Project 0268 from the Agricultural Research Center, Washington State University.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) U92266 and U92267.

Dagger The first two co-authors share equal credit in this investigation.

§ Present address: Plant Biology Division, S. R. Noble Foundation, Ardmore, OK 73402.

Feodor Lynen Fellow of the Alexander von Humboldt Foundation.

par To whom correspondence should be addressed: Institute of Biological Chemistry, Washington State University, Pullman, WA 99164-6340. Tel.: 509-335-1790; Fax: 509-335-7643; E-mail: croteau{at}mail.wsu.edu.

1 The abbreviations used are: GLC, gas-liquid chromatography; MS, mass spectrometry (spectra); aa, amino acid(s); bp, base pair(s); PCR, polymerase chain reaction; RACE, rapid amplification of cDNA ends.

2 C. L. Steele, S. Katoh, J. Bohlmann, and R. Croteau, manuscript submitted for publication.

3 L. Cool, personal communication.

    REFERENCES
Top
Abstract
Introduction
Procedures
Results
Discussion
References

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