Influence of Precursor Availability on Alkaloid Accumulation by Transgenic Cell Line of Catharanthus roseus

doi:10.1104/pp.116.2.853

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Influence of Precursor Availability on Alkaloid Accumulation by Transgenic Cell Line of Catharanthus roseus¹

Serap Whitmer, Camilo Canel²^,^*, Didier Hallard, Cecilia Gonçalves, and Robert Verpoorte

Department of Pharmacognosy, Gorlaeus Laboratories, Leiden University, P.O. Box 9502, 2300 RA Leiden, The Netherlands

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

We have used a transgenic cell line of Catharanthus roseus (L.) G. Don to study the relative importance of the supply of biosyntheticprecursors for the synthesis of terpenoid indole alkaloids. LineS10 carries a recombinant, constitutively overexpressed versionof the endogenous strictosidine synthase (Str) gene. Various concentrationsand combinations of the substrate tryptamine and of loganin, theimmediate precursor of secologanin, were added to suspension culturesof S10. Our results indicate that high rates of tryptamine synthesiscan take place under conditions of low tryptophan decarboxylaseactivity, and that high rates of strictosidine synthesis are possiblein the presence of a small tryptamine pool. It appears that theutilization of tryptamine for alkaloid biosynthesis enhances metabolicflux through the indole pathway. However, a deficiency in thesupply of either the iridoid or the indole precursor can limitflux through the step catalyzed by strictosidine synthase. Precursorutilization for the synthesis of strictosidine depends on theavailability of the cosubstrate; the relative abundance of theseprecursors is a cell-line-specific trait that reflects the metabolicstatus of the cultures.

INTRODUCTION

Top
Abstract
Introduction
Methods
Results
Discussion
References

The tropical plant Catharanthus roseus (L.) G. Don (Apocynaceae) produces TIAs of high medicinal and economic value, suchas ajmalicine, catharanthine, vindoline, and the bisindoles vinblastineand vincristine. Cell cultures of C. roseus have long been consideredto be sources of medicinally important TIAs, but have sufferedfrom their characteristically low productivity (Verpoorte et al.,1993). The optimization of medium composition, including the supplyof biosynthetic precursors, and genetic engineering are amongthe various strategies that have been followed to increase alkaloidproduction in vitro. The precursors for the synthesis of TIAsare obtained from the shikimate and mevalonate pathways, whichsupply the indole tryptamine and the iridoid secologanin, respectively(Fig. 1). Tryptamine is synthesized from Trp, a step catalyzedby TDC, whereas secologanin is obtained from loganin, which isderived from the monoterpenoid geraniol. The first committed stepin the biosynthesis of TIAs is the condensation of secologaninand tryptamine, catalyzed by STR, which results in the formationof strictosidine, the universal precursor of TIAs.

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Figure 1. Biosynthesis of strictosidine in C. roseus.

There are numerous reports of experiments in which precursors have been added to cell cultures of C. roseus. The reportedeffects of feeding various indole and terpenoid building blocksare largely inconsistent. Exogenous Trp has been reported to increasetryptamine content without affecting TIA production (Mérillonet al., 1986; Facchini and Di Cosmo, 1991); it has also been reportedto cause a nearly 3-fold increase in alkaloid production in onecell line, and to reduce production in a daughter line (Zenk etal., 1977). Exogenous Trp and tryptamine negatively affected alkaloidaccumulation in one study (Döller et al., 1976), whereas tryptaminehad a stimulating effect in another (Krueger and Carew, 1978).Exogenous secologanin has also been shown both to have no effecton and to enhance alkaloid production (Zenk et al., 1977; Kruegerand Carew, 1978; Facchini and Di Cosmo, 1991; Moreno et al., 1993).These apparently contradictory results underscore the difficultiesassociated with the study of a complex metabolic pathway.

We report a series of experiments designed to study the effect of feeding precursors under conditions of high-STR activityand iridoid availability. We have used cell line S10 of C. roseus,an experimental system in which flux through the crucial metabolicstep of strictosidine synthesis is always unimpeded. The patternsof alkaloid accumulation and enzymatic activities of S10 are wellcharacterized; S10 is a transgenic line that constitutively expressesthe Str gene at high levels, resulting in high STR activity andthe accumulation of large quantities of TIAs, including ajmalicine,catharanthine, serpentine, and tabersonine (Canel et al., 1998).We have thus been able to assess the relative importance of thetwo pathways that converge at the STR-catalyzed step and the influenceof TDC activity on TIA production.

	MATERIALS AND METHODS

Top Abstract Introduction Methods Results Discussion References

Culture Media and Components

MS58 (per liter) consisted of: Murashige and Skoog salts (Murashige and Skoog, 1962

), 0.1 g of myo-inositol, 0.4 mg of thiamine,2 mg of NAA, 0.2 mg of kinetin, and 30 g of Suc; and PM consistedof: Murashige and Skoog salts devoid of phosphate and nitrate,0.1 g of myo-inositol, 0.4 mg of thiamine, and 80 g of Suc. Sucwas purchased from Duchefa (Haarlem, The Netherlands); salts,vitamins, and hormones from Merck; loganin from Extrasynthese(Genay, France); and tryptamine-HCl from Aldrich. Secologaninwith a purity of 96% was obtained from crude acetone extractsof berries of Symphoricarpus sp. by elution from a silica column(Kieselgel 60, Merck) with acetone:ethyl acetate (Stevens, 1994

Cell Lines and Culture Conditions

The transgenic cell line S10 was generated by Agrobacterium-mediated transformation of leaves of Catharanthus roseus (L.)G. Don, var Morning Mist (Blokker, The Netherlands), as describedpreviously (Canel et al., 1998

). The line carries a T-DNA constructedin binary vector pMOG22 (Mogen, Leiden, The Netherlands), whichconfers resistance to the antibiotic hygromycin, and containsa gus reporter gene and a recombinant version of the endogenousStr gene (accession no. X61932) under the control of the strongconstitutive cauliflower mosaic virus 35S promoter. Line S10 wasmaintained in medium MS58 containing 50 mg/L hygromycin B for4 months after its initiation from transgenic callus in July 1995,and has since been grown in antibiotic-free MS58. Wild-type lineCRPM was established from seeds of C. roseus in 1983. Lines weremaintained by periodic subculture (every 7-10 d) into 250-mL wide-mouthedErlenmeyer flasks fitted with silicon foam stoppers (Shin Etsu,Tokyo, Japan) containing 50 mL of liquid medium in a 1:2 to 1:4ratio. Cultures were placed on gyratory shakers (110-120 rotationsper min) at 25 ± 1°C, in continuous light (2000-3600 lux). Togenerate sufficient biomass for inoculation of a large numberof flasks, cell cultures were sequentially scaled up to 0.5- and2-L flasks containing 100 and 500 mL of MS58, respectively. Cellsin stationary phase (7-10 d old) were inoculated at the rate of5.0 ± 0.1 g fresh weight per 50 mL of PM in 250-mL flasks. Loganinand tryptamine were added from filter-sterilized 100-mM solutions.Treated and control cultures were harvested in duplicate or triplicate;extraction and analysis were carried out after pooling the replicatesamples.

Enzyme Assays

Soluble proteins were extracted from 350 mg of frozen biomass by homogenization in 350 µL of extraction buffer (0.1 m sodiumphosphate, pH 7.0, 2 mm EDTA, and 4 mm DTT) in the presence of17.5 mg of polyvinylpolypyrrolidone. Homogenization was performedin 1.5-mL microfuge tubes using hand-held plastic micropestles(Van Oostermerssen, Rijswijk, The Netherlands). A clear supernatantcontaining the enzymes of interest was obtained by centrifugationof the homogenate at 16,000g at 4°C for 30 min. Protein concentrationwas determined using the protein-staining reagent and 3550-UVMicroplate Reader (Bio-Rad) and BSA as the standard. The proceduresto assay the activities of STR and TDC have been described (Penningset al., 1987

, 1989

Detection of Alkaloids and Precursors

Tryptamine was extracted from 50 mg of freeze-dried biomass using 5 mL of dichloromethane (Schripsema and Verpoorte, 1992

)and detected by HPLC (Van der Heijden et al., 1987

). Secologaninwas extracted from 100 mg of freeze-dried biomass by incubationin 2 mL of boiling water for 2 min. Secologanin was quantifiedas strictosidine by HPLC (Pennings et al., 1989

), after in vitroconversion in 100 µL of 0.1 mm sodium phosphate, pH 6.8, containing>15 pkat STR, 1 mm tryptamine, 1 mm EDTA, and 3 mm DTT at 30°Cfor 30 min (D. Hallard and R. Van der Heijden, unpublished data).For extraction of TIAs, 100 mg of freeze-dried biomass was homogenizedin 15 mL of absolute ethanol. After centrifugation at 3,500g for30 min, 10 mL of the extract was dried under reduced pressure,and the residue was dissolved in 1 mL of 1 m H₃PO₄. Followingcentrifugation of the acidic alkaloid solution at 16,000g for5 min, 50 µL of the supernatant was analyzed by HPLC. The identityof the analytes was established by photodiode-array detectionof their UV spectra (Van der Heijden et al., 1987

	RESULTS

Top Abstract Introduction Methods Results Discussion References

Control cultures of S10 showed the patterns of enzymatic activity and alkaloid accumulation that are characteristic of thishighly productive line. TDC activity was induced upon inoculationinto PM, reaching maxima between d 3 and 5, and decreased to basallevels for the rest of the culture period. STR activity was alwaysvery high (>500 pkat/mg of soluble protein), ranging from 10 to50 times the level found in wild-type cultures. Inoculation intoPM was followed by a short lag period of about 3 d, during whichthe relatively high amount of TIAs already present in the inoculumincreased only slightly. The rate of accumulation then increaseduntil reaching a plateau around d 12. Tryptamine content was highestduring the first few days of the production phase; it decreasedrapidly as TIAs began to accumulate, and increased slightly atthe end of the production period, when the rate of TIA accumulationdecreased. The addition of precursors did not affect the growthof the cell cultures, as determined by measuring the amount ofbiomass obtained at the end of the test period. Control culturesreached 18.5 ± 3.5 g dry weight L¹ (n = 6), whereas treated cultures reached 18.6 ± 3.1 g/L (n =19); the dry weight to fresh weight ratio was always in the rangeof 0.11 to 0.13. Loganin was chosen over secologanin because thelatter is inefficiently utilized for strictosidine synthesis whenadded to the medium. Exogenous secologanin appears to be compartmentalizeddifferently from endogenous secologanin, including that synthesizedfrom exogenous loganin; in contrast, exogenous loganin is usedin toto by C. roseus (Naudascher et al., 1989a, 1989b).

The first experiment consisted of feeding 500 µm loganin to a set of cultures either at the time of inoculation (d 0) withharvesting on d 3, or on d 11 with harvesting on d 14. Nonfedcontrol cultures were harvested on d 3, 11, and 14. Exogenousloganin had a depleting effect on tryptamine content, which wasequally dramatic on either of the two feeding dates, and was accompaniedby a 2- to 4-fold increase in TIA content in the treated cells(Table I). The steady-state level of tryptamine was a small fraction,in molar equivalents, of the amount by which alkaloid contentincreased. From d 0 to 3, treated cells accumulated 126 µmol/LTIAs, whereas the alkaloid content of the control cultures increasedonly slightly; the difference in tryptamine content between thetwo sets of cultures at the end of that period was 6.8 µmol/L.More strikingly, in the 3-d period between d 11 and 14, duringwhich low levels of tryptamine prevail, cells fed loganin on d11 produced 140 µmol/L TIAs more than control cells, whereas thedifference between their tryptamine content was only 5.0 µmol/L.Iridoids did not accumulate in any of the cultures.

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Table I. Effect of feeding loganin on tryptamine and TIA content of cultured C. roseus cells

Treatment consisted of addition of 500 µm loganin. Triplicate cultures were pooled upon harvesting and analyzed as singlesamples.

For the second experiment, we used cell cultures of S10 showing a reduced capacity to synthesize tryptamine. We have observeda significant correlation between culture browning and low tryptaminebiosynthetic capacity during the course of experiments not relatedto precursor feeding. Nine out of 12 independently initiated culturesharvested at the onset of browning had a tryptamine content nogreater than 1.5 µmol/L (mean = 1.6 ± 2.2 µmol/L), compared witha content of 6.8 ± 1.3 µmol/L measured in healthy cultures. Culturebrowning results from the oxidation of phenolic compounds. Browningis commonly associated with increased flux through branches ofthe shikimate pathway, leading to the synthesis of phenolic acidsand phenylpropanoids, which compete with the indole branch forprecursors and consequently impair the ability of the cells tomaintain a high rate of tryptamine synthesis. We do not know thereason for the occasional spontaneous browning of the cultures,a phenomenon that is not unique to S10. Nevertheless, culturebrowning in S10 is valuable for indicating the occurrence of reducedtryptamine biosynthetic capacity, which provides the opportunityto carry out experiments under conditions of low tryptamine availability.The experiment was performed with 27 cultures, which remainedhealthily colored, out of a total of 51 that were started fromthe same inoculum. The remaining cultures turned brown shortlyafter inoculation and were discarded as browning developed. Thehealthy sister cultures were divided into control and treatedgroups. The TDC activity of the control cultures followed thenormal pattern of induction upon inoculation into PM. The levelof tryptamine dropped from 5.1 µmol/L on d 0 to 0.4 µmol/L ond 3. Tryptamine content remained below 1.0 µmol/L thereafter,most notably at the end of the culture period when the calculatedrate of increase of TIA content was low (<10 µmol L¹ d¹). The reduced capacity to synthesize tryptamine was most apparentduring the 2nd week of culture. Whereas addition of 50, 100, or500 µm loganin on d 0 increased alkaloid content, it did not havea significant effect when done on d 11 (Fig. 2); rather, feedingloganin on d 11 resulted in the accumulation of secologanin. Alkaloidcontent rose considerably when tryptamine was supplied along withloganin (Fig. 2). Addition of tryptamine alone, however, did notincrease TIA content.

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Figure 2. Effect of feeding loganin on TIA accumulation under conditions of low tryptamine availability. White bars represent culturestreated on d 0 and sampled on d 3; shaded bars represent culturestreated on d 11 and harvested on d 14. The concentration of exogenouslyadded precursors is expressed in micromoles. L+T indicates thatboth loganin and tryptamine were added. Triplicate cultures werepooled upon harvesting and analyzed as single samples.

To investigate the influence of TDC activity on alkaloid production, when secologanin supply is not limiting, an experimentwas performed in which one set of cultures was kept under conditionsof loganin abundance for the entire production period. Two timecourses of 14 d were carried out: one with loganin-fed cells andthe other without feeding. Beginning on d 0, 200 µm loganin wasadded daily to a different set of flasks, which was harvestedthe following day, along with a set of control, nonfed cultures.Alkaloid accumulation was higher in fed cultures at all pointsduring the production test (Fig. 3A). Tryptamine content followedthe normal pattern, reaching a maximum of 2.4 µmol/L on d 3 incontrol cultures and of 1.5 µmol/L on d 2 in fed cultures. TDCactivity also followed the normal pattern and was very similarin both sets of cultures, indicating that the presence of exogenousloganin did not affect the amount of active enzyme in the cells.The daily increase in alkaloid content showed a downward trend,which paralleled, but was not proportional to, the drop in TDCactivity. The difference in alkaloid content between control andfed cultures was rather constant (67.4 ± 9.3 µmol/L), and wasnot affected by fluctuations in tryptamine content nor by changesin the level of TDC activity (Fig. 3B). Feeding 200 µm tryptaminealong with loganin did not significantly increase alkaloid contentrelative to cultures fed only loganin, whether performed at thebeginning (d 2) or near the end (d 10) of the culture period.

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Figure 3. Time course of alkaloid production (A) and TDC activity (B) under normal conditions ( $open circle$ ) and in the presence of 200 µm exogenousloganin ( $bullet$ ). $Delta$ , Daily difference in alkaloid content between treatedand control cultures. Duplicate or triplicate cultures were pooledupon harvesting and analyzed as single samples.

Loganin utilization was generally low; only 25 to 35% of the exogenous loganin was converted into alkaloids. Still, loganinfeeding was far more effective than secologanin feeding. The capacityto utilize exogenous secologanin (500 µm) was tested in a smallnumber of cultures, which showed an increase in TIA content thatwas only 10% of that achieved with loganin. Cultures of the wild-typeline CRPM were also supplied with precursors. CRPM does not normallyaccumulate TIAs, but it did utilize exogenous loganin for alkaloidproduction, even more so when fed tryptamine concurrently. Thealkaloid content of CRPM, however, reached levels much lower thanin the transgenic line (<40 µmol/L), suggesting that other factors,possibly including the characteristically low STR activity, limitits biosynthetic capacity. The C. roseus cultures did not accumulatetryptamine and secologanin concurrently; no evidence of the existenceof separate accumulation sites for these precursors was thus obtained.Alkaloids were never detected in the culture medium.

	DISCUSSION

Top Abstract Introduction Methods Results Discussion References

Thanks to the constitutively elevated levels of STR activity that characterize transgenic line S10, induction of the indoleand iridoid pathways can be readily detected in S10 cultures bymeasuring tryptamine and TIA content, and the level of utilizationof exogenous precursors. Induction of tryptamine synthesis takesplace very rapidly after transfer to PM, whereas the iridoid pathwaytakes longer to become fully activated. The rapid utilizationof the small tryptamine pool for TIA biosynthesis signals theflux of iridoids through to the strictosidine synthesis step.High rates of TIA accumulation can occur when TDC activity, ameasure of the amount of active enzyme present in the cells, andtryptamine availability are low (Table I; Fig. 3). This indicatesthat the rate of TIA biosynthesis depends on the rapid turnoverof tryptamine rather than on its accumulation, and that high levelsof TDC are not required for this rapid turnover to occur. Underregular conditions tryptamine accumulation, as well as the rateand degree of TIA accumulation, are all independent of TDC activity;this is also the case when iridoid precursors are abundant (Fig.3B). Our results are consistent with the lack of correlation betweenTDC activity and TIA biosynthesis generally found in cell cultures(Knobloch and Berlin, 1983; Mérillon et al., 1986; Eilert etal., 1987; Facchini and Di Cosmo, 1991; Islas et al., 1994). Apparently,factors other than TDC activity, such as the availability of Trpand secologanin, the activity of other tryptamine-utilizing enzymes,and tryptamine transport across the tonoplast, more strongly influenceflux through the indole pathway. However, it has been reportedthat TDC activity in developing seedlings of Cinchona ledgerianaincreases after a large pool of Trp has formed, and falls to undetectablelevels once the Trp has been converted into tryptamine (Aertset al., 1990), suggesting that, unlike in cell cultures, preciselytimed changes in the level of TDC activity do play a role in alkaloidbiosynthesis in the intact plant.

The utilization of tryptamine for TIA production appears to induce the cells to synthesize more tryptamine. Control cellsthat were not accumulating large amounts of alkaloids at the endof the production period did not show high tryptamine content,but their capacity to rapidly synthesize tryptamine became apparentupon addition of loganin. Tryptamine has been proposed to feedbackinhibit TDC activity (Noé et al., 1984); its utilization maytherefore have a de-inhibitory effect. We consistently detectedsimilar levels of TDC activity in cells that were actively synthesizingalkaloids and cells that were not. The possibility that any positiveinfluence that tryptamine utilization may have on flux throughthe indole pathway affects an earlier step leading to increasedTrp availability merits further study.

Our results, particularly those obtained when using the tryptamine-deficient cultures (Fig. 2), show that an abundant supplyof both precursors, tryptamine and secologanin, must exist forhigh rates of strictosidine synthesis to occur. Exogenous loganinincreases alkaloid content when tryptamine is not limiting; additionof loganin causes the rapid utilization of tryptamine, at whichpoint addition of tryptamine may have a positive effect. Loganindeficiency is limiting when tryptamine is abundant, and vice versa.This model accounts for the observations reported in the literature,except for the occasional negative effects of Trp and tryptamineon TIA accumulation, and accurately predicts the outcome of ourexperiments. The relative rate of biosynthesis of tryptamine andsecologanin, and therefore also the limitation in the supply ofeither precursor, are cell-line-specific phenomena. The effectof feeding precursors depends on the metabolic status of the subjectcell line, which is a function of a large number of variablesthat affect the steady-state concentration of a particular metabolite.Cell cultures will thus constitute more useful experimental systemswhen at least some of those variables can be assigned a value.The influence of the shikimate pathway on TIA biosynthesis willbe more fully understood if we are able to manipulate relevantenzymatic activities in a high-STR-activity background, such asfound in S10, under conditions of iridoid abundance. A numberof genes encoding enzymes of the shikimate pathway are availablefrom other plant species, constituting starting points to furtherstudy TIA biosynthesis in C. roseus.

	FOOTNOTES

¹   This work was supported by the National Science Foundation under a grant awarded to C.C. in 1995.
²   Present address: U.S. Department of Agriculture, Agricultural Research Service, Natural Products Center, Room 2021, University,MS 38677.
^*   Corresponding author; e-mail CCanel{at}olemiss.edu; fax 1-601-232-1035.

Received June 23, 1997; accepted September 19, 1997.

ABBREVIATIONS

Abbreviations: PM, production medium. STR, strictosidine synthase. TDC, Trp decarboxylase. TIA, terpenoid indole alkaloid.

	LITERATURE CITED

Top Abstract Introduction Methods Results Discussion References

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Pennings EJM, Hegger I, Vander Heijden R, Duine JA, Verpoorte R (1987) Assayof tryptophan decarboxylase from Catharanthus roseus cell culturesby high-performance liquid chromatography. AnalBiochem 165: 33-136 [CrossRef][Medline]

Pennings EJM, Van den Bosch RA, Vander Heijden R, Stevens LH, Duine JA, Verpoorte R (1989) Assayof strictosidine synthase from plant cells by high-performanceliquid chromatography. AnalBiochem 176: 412-415 [CrossRef][ISI][Medline]

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Influence of Precursor Availability on Alkaloid Accumulation by Transgenic Cell Line of Catharanthus roseus1

Copyright Clearance Center: 0032-0889/98/116/0853/05 © 1998 American Society of Plant Physiologists

Influence of Precursor Availability on Alkaloid Accumulation by Transgenic Cell Line of Catharanthus roseus¹

Copyright Clearance Center: 0032-0889/98/116/0853/05

© 1998 American Society of Plant Physiologists