PLoS ONEplosplosonePLOS ONE1932-6203Public Library of ScienceSan Francisco, CA USA10.1371/journal.pone.0192872PONE-D-17-42550Research ArticleBiology and life sciencesPlant sciencePlant anatomyLeavesBiology and life sciencesOrganismsEukaryotaPlantsFlowering plantsLettuceBiology and life sciencesOrganismsEukaryotaPlantsVegetablesLettuceBiology and life sciencesCell biologyCellular structures and organellesChloroplastsChlorophyllBiology and life sciencesCell biologyPlant cell biologyChloroplastsChlorophyllBiology and life sciencesPlant sciencePlant cell biologyChloroplastsChlorophyllBiology and life sciencesCell biologyCellular typesPlant cellsChloroplastsChlorophyllBiology and life sciencesCell biologyPlant cell biologyPlant cellsChloroplastsChlorophyllBiology and life sciencesPlant sciencePlant cell biologyPlant cellsChloroplastsChlorophyllPhysical sciencesMaterials scienceMaterials by attributePigmentsOrganic pigmentsChlorophyllPhysical sciencesChemistryChemical compoundsPhenolsPhysical sciencesChemistryChemical compoundsAcidsOrganic acidsBiology and life sciencesPlant sciencePlant anatomyFruit and seed anatomyPlant embryo anatomyRadicleBiology and life sciencesPlant sciencePlant anatomyPlant embryo anatomyRadicleBiology and life sciencesDevelopmental biologyEmbryogenesisPlant embryogenesisPlant embryo anatomyRadicleBiology and life sciencesDevelopmental biologyPlant growth and developmentPlant developmentPlant embryogenesisPlant embryo anatomyRadicleBiology and life sciencesPlant sciencePlant growth and developmentPlant developmentPlant embryogenesisPlant embryo anatomyRadiclePhysical sciencesPhysicsElectromagnetic radiationLuminescenceFluorescenceBiology and life sciencesPlant sciencePlant anatomySeedsUnravelling the bioherbicide potential of Eucalyptus globulus Labill: Biochemistry and effects of its aqueous extractUnravelling the bioherbicide potential of E. globulus aqueous extracthttp://orcid.org/0000-0002-4596-8571PuigCarolina G.ConceptualizationData curationFormal analysisInvestigationMethodologyVisualizationWriting – original draft1*ReigosaManuel J.Funding acquisitionMethodologyResourcesSupervisionValidationWriting – review & editing1‡ValentãoPatríciaFunding acquisitionMethodologyResourcesSupervision2‡AndradePaula B.Funding acquisitionMethodologyResourcesSupervision2‡PedrolNuriaConceptualizationFormal analysisFunding acquisitionInvestigationMethodologyProject administrationResourcesSupervisionValidationWriting – review & editing1Department of Plant Biology and Soil Science, University of Vigo, Vigo, SpainREQUIMTE/LAQV, Laboratory of Pharmacognosy, Department of Chemistry, University of Porto, Porto, PortugalCimminoAlessioEditorUniversita degli Studi di Napoli Federico II, ITALY
The authors have declared that no competing interests exist.
‡ These authors also contributed equally to this work.
* E-mail: cgpuig@uvigo.es13220182018132e0192872412201731120182018Puig et alThis is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
In the worldwide search for new strategies in sustainable weed management, the use of plant species able to produce and release phytotoxic compounds into the environment could be an effective alternative to synthetic herbicides. Eucalyptus globulus Labill. is known to be a source of biologically active compounds responsible for its phytotoxic and allelopathic properties. Our previous results demonstrated the bioherbicide potential of eucalyptus leaves incorporated into the soil as a green manure, probably through the release of phytotoxins into the soil solution. Thus, the aims of this study were to understand the phytotoxicity of the eucalyptus leaves aqueous extract applied in pre- and post-emergence, and to identify and quantify its potentially phytotoxic water-soluble compounds. The effects were tested on the germination and early growth of the model target species Lactuca sativa and Agrostis stolonifera, and on physiological parameters of L. sativa adult plants after watering or spraying application. Dose-response curves and ED50 and ED80 values for eucalyptus aqueous extracts revealed pre-emergence inhibitory effects on both target species, effects being comparable to the herbicide metolachlor. While spraying treatment reduced the aerial and root biomass and increased the dry weight/fresh weight ratio of lettuce adult plants, watering application reduced protein contents and chlorophyll concentrations with respect to control, reflecting different modes of action depending on the site of phytotoxin entry. Via HPLC analyses, a total of 8 phenolic compounds (chlorogenic, two ρ-coumaric derivatives, ellagic, hyperoside, rutin, quercitrin, and kaempferol 3-O-glucoside) and other 5 low weight organic acids (citric, malic, shikimic, succinic and fumaric acids) were obtained from aqueous extract, the latter being identified for the first time in E. globulus. Despite some phytotoxic effects were found on lettuce adult plants, the use of eucalyptus aqueous extract would be discarded in post-emergence, whereas it was promising as a pre-emergence bioherbicide.
http://dx.doi.org/10.13039/501100003329Ministerio de Economía y CompetitividadCGL2016-78660-RPedrolNuriahttp://dx.doi.org/10.13039/501100003176Ministerio de Educación, Cultura y DeporteAP2009-4809http://orcid.org/0000-0002-4596-8571PuigCarolina G.This work was supported by the Spanish Ministry of Education for the FPU grant AP2009-4809 (CGP) and by the Spanish Ministry of Economy and Competitiveness (http://www.mineco.gob.es/; BIOINPUT (CGL2016-78660-R)) (NP). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.Data AvailabilityAll relevant data are within the paper.Introduction
During the past years, an increasing demand for the environmental safety of pesticides has led to looking for new nonsynthetic management methods in agriculture. In this context, sustainable weed management is one of the main challenges for both organic and conventional agriculture [1]. However, the existing products on the market targeting weeds are weakly developed compared with those targeting other pests and diseases [1]. Hence, in the necessary search for new strategies for weed control in organic agriculture, the use of plant species able to produce and release phytotoxic compounds could be an effective tool.
The first step to find possible candidates as bioherbicides consists in assessing the phytotoxic activity of plant material aqueous extracts on morpho-physiological parameters of model target species, by in vitro bioassays. Phenolic compounds, together with other low molecular weight organic acids, are present in plant aqueous extracts because of their water-soluble nature, and several studies have demonstrated their phytotoxic potential against different target species [2,3]. The differential allelopathic effect of each plant species would depend on the type and amount of individual phytotoxic compound as well as on the mixture of compounds present in the plant extract [4,5]. Therefore, chemical identification procedures such as chromatographic techniques for analysis of phenolic compounds have been thoroughly improved in the last years [6].
Evidence of the allelopathic activity and chemical composition of different species of the genus Eucalyptus (Myrtaceae) have been widely reported. Plants of the genus Eucalyptus possess strong pesticide potential due to the presence of a wide array of biologically active compounds, especially from their essential oils rich in terpenoids [7,8]. The phytotoxic effects of Eucalyptus globulus Labill. aqueous extracts or leachates have been demonstrated on the germination and radicle growth of some crops such as sorghum (Sorghum vulgare) [9], Brassica sp. [10], eggplant (Solanum melongena) [11], barley (Hordeum vulgare) [12] or fingermillet (Eleusine coracana) [13], as well as on weed species: purple nutsedge (Cyperus rotundus) and bermudagrass (Cynodon dactylon) [14], or redroot pigweed (Amaranthus retroflexus) and barnyardgrass (Echinochloa crus-galli) [15]. Our previous results in greenhouse conditions demonstrated the bioherbicide potential of eucalyptus leaves incorporated into the soil as a green manure, pointing out different modes of action for target species and attributing the phytotoxic effects probably to the release of water-soluble compounds into the soil solution [15]. Therefore, it is time to detail the chemical composition of E. globulus aqueous extract and to determine the primary physiological processes affected in target species.
Several studies on the phenolic composition of E. globulus leaf aqueous extracts revealed the presence of different hydroxycinnamic and hydroxybenzoic acids: caffeic, ferulic, and chlorogenic, as well as some flavonoids: rutin, quercitin, hyperoside and ellagic acid, but these studies were usually related to an antioxidant activity [6,16–19]. However, only some isolated reports deal with the relation between the phenolic composition of the leaf extracts and their allelopathic properties [20–22]. To our knowledge, no reports have been done to study the organic acid composition from E. globulus leaf aqueous extract. Furthermore, the important stock of eucalyptus plantations, mainly devoted to paper industry, present in the agroecosystems (and the fact that it is one of the most world widespread species) makes E. globulus biomass an optimal candidate for its potential use as a bioherbicide.
For this work, E. globulus aqueous extract was evaluated for its allelopathic potential as natural herbicide, by the following objectives: i) to assess the phytotoxicity of aqueous extract applied in pre- and post-emergence, and to determine the primary physiological processes affected; and ii) to identify potentially phytotoxic compounds present in the aqueous extract.
Materials and methodsPlant material and aqueous extracts
Fresh eucalyptus adult leaves from Eucalyptus globulus Labill. were collected from several 10 years old plantations surrounding University of Vigo (Galicia, NW Spain, 42.09°N, 8.25°W), and slashed in 1 cm2-sized pieces immediately after collection. Extractions were performed in 2-L Erlenmeyer flasks at a plant dry weight/distilled water volume ratio of 66.7 g L-1 (the maximum ratio to keep a volume of chopped plant material completely soaked). Dry weight/fresh mass ratio was obtained by drying aliquots of fresh material at 70°C for 72 h. Flasks were maintained in the dark at room temperature for 24 h, being gently soaked every 6 h. The aqueous extracts were filtered through cellulose membrane 0.45 μm pore size to clear impurities and then through 0.2 μm to sterilize the extract. The extracts were then frozen at -20°C in sterile plastic bottles until bioassayed.
For the bioassays, lettuce (Lactuca sativa L. cv. `Great Lakes´) and bentgrass (Agrostis stolonifera L. cv. Penncross) were chosen respectively as dicot- and monocotyledon ‘standard target species’ (STS), thoroughly used in literature for their fast germination, genetic homogeneity, and high sensitivity to allelochemicals [23,24], thus allowing comparisons for many different compounds [25]. Seeds of lettuce and bentgrass were purchased from Fitó S. A. (Barcelona, Spain) and Rocalba S. A. (Girona, Spain), respectively.
Pre-emergence dose-response bioassays
The crude aqueous extract was successively diluted in distilled water to get five final concentrations, those corresponding to 66.7, 33.3, 16.7, 6.7 and 0 g L-1 on a dry mass basis. Values for pH (CrisonMicropH 2001 pH-meter), electrical conductivity (EC, Crison CDTM-523 conductivity meter), and osmolarity (Gonotec OSMOMAT 030 cryoscopic osmometer) corresponding to each dilution were: 4.75, 4.44, 4.62, 4.87 and 6.55; 1.37, 0.70, 0.40, 0.16 and 0.00 dS m-1; and 0.064, 0.037, 0.016, 0.006 and 0.000 osmol kg-1, respectively. The synthetic pre-emergence herbicide S-metolachlor 960 g L-1 (Dual Gold®, Syngenta Agro S.A., Madrid, Spain) was prepared at 0.153 g L-1 (540 μM) in such a way attaining the label dose (LD, 0.96 kg ha-1), and used as positive control. Values of pH, EC and osmolarity were 6.14, 0.02 dS m-1 and 0.099 osmol kg-1. Lettuce seeds were incubated in 6-well dishes, at a rate of 15 seeds per well for germination bioassay, and placed on a filter paper wetted with 600 μL of solution. Dishes were sealed with Parafilm and incubated in the dark at 27°C and a relative humidity of 75% during 48 hours. The number of germinated seeds (rupture of seed coats and the emergence of radicle ≥ 1 mm [26]) was counted every 24 hours until no further seeds germinated. Total percentage of germinated seeds (Gt) was calculated from the cumulative germination data [27]. For radicle growth bioassay, lettuce seeds were pre-germinated on wet filter paper in plastic trays filled with perlite watered at saturation with can water and incubated at 27°C for 24 h. After incubation, ten pre-germinated seeds (radicle length between 1–3 mm [26]) were transferred to each well dish as described above and placed in a growth chamber at 25/20°C, 18/6 h light/dark. After 48 h of incubation, radicle length was measured. Each treatment was replicated five times.
Phytotoxicity bioassays with bentgrass were carried out according to the procedure described by Dayan et al. [28]. Twelve mg of A. stolonifera seeds were placed on a Whatman 3 MM Chr filter paper in each well of a 24-well plate. Two hundred fifty μL of the different aqueous extract concentrations and metolachlor were added at random to different wells. Plates were incubated at 27°C in continuous light. Phytotoxicity was evaluated by visually comparing the germination and seedling growth in each well after 12 days. The phytotoxicity was rated on a scale ranging from 0 to 5. Ratings of 0 meant no effect and of 5 complete inhibition. Each treatment was repeated seven times.
Dose-response curves were obtained for seed germination and radicle growth, and the ED50 and ED80 (concentrations required to obtain 50% and 80% inhibition, respectively) were estimated.
Post-emergence bioassays: Watering vs. spraying
Lettuce seeds were germinated in plastic trays with 5 cm depth layer perlite watered with half-strength Hoagland nutrient solution [29] every other day. Seedlings were grown in a growth chamber at 75% relative humidity and 12 h light at 18°C and 12 h dark at 8°C for three weeks. Plants with three fully expanded leaves were transferred to pots containing perlite watered with half-strength Hoagland nutrient solution to stimulate root system development, and left to acclimate. One week later, plants were exposed to the different post-emergence treatments: control vs. eucalyptus aqueous extract. Treatments were applied in two different forms: watering vs. spraying, with the aim to determine the differing effects of entry through the root compared to damage by contact.
For the watering treatment, the aqueous extract prepared at 66.7 g L-1 in half-strength Hoagland nutrient solution was applied daily until percolation, using plants watered with half-strength Hoagland solution as a negative control. For the spraying treatment, plants were sprayed once a day with crude extract prepared at 66.7 g L-1 in distilled water, using plants sprayed with distilled water as negative control. Lettuce plants were sprayed until all the leaves were covered with small droplets, just before the point of runoff. Sprayed plants were as well watered daily with half-strength Hoagland solution during the experiment. Six replicates per treatment and application form were prepared.
Chlorophyll a fluorescence measurement
The effects of the imposed treatments were sequentially measured on the photosynthetic efficiency of three lettuce plants per treatment chosen at random, by using a Maxi Imaging PAM Chlorophyll Fluorescence System from Walz (Effeltrich, Germany). Immediately before aqueous extract treatment and every 24 h during 5 days, chlorophyll fluorescence parameters were obtained (Table 1). At each measuring time, a dark acclimation period of 5 min was imposed on the plants to allow all reaction centers to open and minimize fluorescence associated with the energization of the thylakoid membrane [30]. After that, whole plants were successively illuminated at an intensity of 0.5 μmol m-2 s-1 for the measurement of Fo, and with a saturating pulse of 2700 μmol m-2 s-1 intensity for the measurement of Fm. Finally, plants were exposed for 5 min to actinic illumination at 110 μmol m-2 s-1 (measuring the corresponding fluorescence level, F) which was interrupted every 20 s with 800 ms saturating pulses of 2700 μmol m-2 s-1 for the measurement of Fm´. From these parameters, other variables (Table 1) were calculated by the instrument software using different formula according to Bilger and Björkman [31], Demmig-Adams et al. [32], Genty et al. [33] and Kramer et al. [34]. Fifteen measurements were obtained for each variable at each measuring time, which yielded a kinetic plot for each parameter along time. The average of the area was calculated from the kinetic measurement for the three replicates in every treatment.
10.1371/journal.pone.0192872.t001
Chlorophyll fluorescence parameters measured with the Maxi Imaging PAM fluorometer.
F
Fluorescence yield
Fo
Dark fluorescence yield
Fo´
Fluorescence yield of light-adapted leaves
= Fo / (Fv / Fm + Fo / Fm´)
Fm
Maximal fluorescence yield of dark-adapted leaves
Fm´
Maximal fluorescence yield of light-adapted leaves
Fv
Variable fluorescence yield of dark-adapted leaves
= Fm − Fo
Fv´
Variable fluorescence yield of light-adapted leaves
= Fm´ − Fo´
Fv/Fm
Maximal (photosystem II) PSII efficiency
= (Fm − Fo)/ Fm
φII
Effective (photosystem II) PSII quantum yield
= (Fm´−F)/ Fm´
φNPQ
Quantum yield of regulated energy dissipation
= 1- φII -1/ (φNPQ +1+qL(Fm / Fo -1))
φNO
Quantum yield of non-regulated energy dissipation
= 1/ (φNPQ +1+ qL (Fm / Fo -1))
qN
Coefficient of non-photochemical quenching
= (Fm − Fm´)/ (Fm − Fo´)
qL
Coefficient of photochemical quenching
= (Fm´-F)/ (Fm´ -Fo´) · Fo´/ F
ETR
Estimated rate of photosynthetic electron transport
= 0.5· φII ·PARa·Abs.μequivalents m-2s-1
a PAR, Photosynthetic Active Radiation
Photosynthetic pigments content
After 5 days of treatment, each plant measured for chlorophyll fluorescence was analyzed for photosynthetic pigments. Pigments were extracted from 100 mg of fresh material per replicate in 1.5 mL methanol and centrifuged at 3500 g for 5 minutes. Then, 0.5 mL of the supernatant were diluted with extra 0.5 mL of methanol, and chlorophyll a (Chl a), chlorophyll b (Chl b) and carotenoid contents were determined spectrophotometrically (WPA Lightwave Diode-Array UV/Vis) after Wellburn [35].
Protein content determination
Total proteins were quantified by using the spectrophotometric Bradford assay as described by Pedrol et al. [36], in the same 3 lettuce seedlings used for pigment determination. For each replicate, 100 mg of fresh leaves were homogenized in 0.8 mL of 0.05 M Tris buffer containing 0.05 g of the antioxidant polyvinyl polypyrrolidone (PVPP). The homogenates were centrifuged at 4°C and 14000 gn for 20 min. Then, 0.1 mL of the supernatant was mixed with 2 mL of Bradford´s reagent and absorbance was measured at 595 nm against a dose-response curve of commercial bovine seroalbumin (BSA).
Growth parameters
The remaining three lettuce plants from each treatment were used to determine the fresh and dry weights of aerial and root biomass, and the length of roots. Fresh leaves and fresh roots from each replicate were weighted before and after being dried at 70°C for 72 h. The dry weight/fresh mass ratio was obtained for aerial biomass.
Chemical analyses of aqueous extractReagents and standards
Formic and sulphuric acids and methanol were obtained from LiChrosolv® (Darmstadt, Germany). Phenolic acids and flavonoid standards were purchased from Extrasynthèse (Genay, France), and organic acids from Sigma-Aldrich (St. Louis, MO, USA). The water was treated in a Mili-Q water purification system (Millipore, Bedford, MA).
Phenolic compounds identification and quantification by high performance liquid chromatography coupled with a diode array detector (HPLC-DAD)
The crude aqueous extract was freeze-dried (model 4.5 Freezone apparatus, Labconco, Kansas City, MO), obtaining a yield rate of 6.46 g of lyophilized per liter. Twenty-five mg of lyophilized were dissolved in 1 mL of methanol and then filtered by 0.45 μm PTFE membrane. Separation of the phenolic compounds was achieved by analyzing 20 μL of the methanol extract on an analytical HPLC unit (Gilson), with a reversed-phase Spherisorb ODS2 column (250 x 4.6 mm, 5 μm particle size; Waters, Milford, MA, USA) with a C18 guard column. The solvent system used was carried out according to a procedure described by Almeida et al. [16], using a mixture of water/formic acid (19:1 vol/vol; solvent A) and methanol (solvent B). The gradient was as follows: 0 min, 5% B; 3 min, 15% B; 13 min, 25% B; 25 min, 30% B; 35 min, 35% B; 39 min, 45% B; 42 min, 45% B; 44 min, 50% B; 57 min, 55% B; 60 min, 70% B; 66 min, 75% B; and 70 min, 100% B; 75 min, 100% B; 76 min, 5% B. Elution was performed at a solvent flow rate of 1 mL/min. Detection was achieved with a Gilson diode array detector. Spectral data from all peaks were collected in the range of 200–400 nm and chromatograms were recorded at 320 nm and at 350 nm, as these correspond to highest absorption of the identified phenolic acids and flavonoids, respectively. The data were processed by Unipoint System software (Gilson Medical Electronics, Villiers le Bel, France). The compounds were identified by comparing their elution order and UV-vis spectra with authentic standards. Peak purity was checked by the software contrast facilities. Phenolic compounds quantification was achieved by the absorbance recorded in the chromatograms relative to external standards, using the following equation:
C(c)=A(c)A(st)×C(st)
Where C(c) is the concentration of the compound in the sample, A(c) is the peak area of the compound in the sample chromatogram, C(st) is the concentration of the standard in the reference solution and A(st) is the area of the peak for the standard in the reference chromatogram. This procedure was performed in triplicate. Data presented are the mean values of three independent measurements.
Organic acids identification and quantification by HPLC-UV
Twenty five mg of lyophilized aqueous extract were dissolved in 1 mL 0.01 N H2SO4, followed by filtration by a 0.45 μm Nylon membrane. The separation and quantification of organic acids were carried out according to the procedure described by Oliveira et al. [37], in a system consisting of an analytic HPLC unit (Gilson Inc., Middleton, WI) with an ion exclusion Nucleogel Ion 300 OA (300×7.7 mm; Macherey-Nagel, Düren, Germany) column. Elution was performed in isocratic mode with H2SO4 (0.01 N), at a flow rate of 0.2 mL/min. Detection was achieved with a UV detector set at 214 nm. Organic acids quantification was done by measuring the absorbance recorded in the chromatograms relative to external standards. This procedure was performed in triplicate. Data presented are the mean values of three independent measurements.
Statistical analyses
Replicated experiments were conducted in a completely randomized design. After testing for normality by Kolmogorov-Smirnov test and for homogeneity of variance by Levene´s test, means were analyzed using independent samples Student´s t-test or one-way ANOVA at P ≤0.05. LSD test (P = 0.05) was used for multiple comparisons of means. In the case of heteroscedasticity, Kruskal-Wallis test and U of Mann-Whitney were used. Semi-quantitative data obtained from A. stolonifera was subjected to Median test regarding the discontinuity of values, besides U of Mann-Whitney for post hoc comparisons. Dose-response curves were modeled by regression analysis with mathematical models, and the most appropriate model was selected for each case on the basis of the determination coefficient [3]. Statistical analyses were performed using the IBM SPSS Statistics 19 software (IBM SPSS Inc., Chicago, IL, USA).
ResultsPre-emergence dose-response bioassays
The aqueous extract of E. globulus affected significantly the germination and radicle length of lettuce in a concentration-dependent manner (Fig 1). Using the best-fit equation based on the coefficient of determination (r2), the obtained ED50 and ED80 values for germination and radicle growth of lettuce are shown in Table 2.
10.1371/journal.pone.0192872.g001
Dose-response curves for E. globulus aqueous extract on (A) germination and (B) radicle length of L. sativa.
Mean values labeled with distinct letters are significantly different at P ≤ 0.05 (LSD post hoc multiple comparisons). Symbols represent mean values of four replicates ± SD. Met., metolachlor (label dose); % r.c., percentage with respect to the control.
10.1371/journal.pone.0192872.t002
E. globulus leaf aqueous extract ED values for germination and radicle length of L. sativa.
Regression equation
r2a
ED50b (g dw L-1)
ED80c (g dw L-1)
Total germination
y = 0.016 x2–2.161 x + 99.93
[1]
0.963
29.6
o.r. d
Radicle length
y = 0.016 x2–2.214 x + 104.1
[2]
0.941
31.7
o.r. d
ar2 = determination coefficient
b ED50, c ED80 = concentration required to obtain 50% and 80% germination, radicle or shoot length inhibition, respectively.
d o.r. = out of range
Mean Gt and radicle growth values of the different eucalyptus concentrations (Fig 1) ranged from 82 to 30% and 90 to 33% of control, respectively, with a highly significant effect of concentration (ANOVA, P ≤ 0.01 for Gt; P ≤ 0.001 for growth). Regardless no concentration attained the ED80 value (Table 2), eucalyptus concentrations above 20 g dw L-1 were significantly more inhibitory of growth than metolachlor: eucalyptus at 33.3 to 66.7 g dw L-1 inhibited 60 to 68% of control, whereas the synthetic herbicide at 0.153 g L-1 attained 28% inhibition (Fig 1).
Results of phytotoxicity assessment against the model monocotyledon A. stolonifera are shown in Fig 2. Analysis of semi-quantitative data showed also highly significant effects of concentration (Median test, P ≤ 0.001) on this STS. Statistical comparisons with control revealed very significant growth reductions at 33.3 g dw L-1 for eucalyptus extract, and a highly significant inhibition at 66.7 g dw L-1 similar to that imposed by metolachlor 0.153 g L-1, which did not completely inhibit the growth of bentgrass seedlings as well.
10.1371/journal.pone.0192872.g002
Effects of E. globulus aqueous extract at different concentrations and metolachlor (label dose) on the growth of A. stolonifera ranking from 0 to 5: 0, no effect; 5, total inhibition. Count cases, n = 7.
Asterisks indicate significant differences between control and each treatment (*P ≤ 0.05, **P ≤ 0.01, ***P ≤ 0.001, n.s. not significant P > 0.05; Mann-Whitney U test).
Post-emergence bioassays: Watering vs. sprayingChlorophyll a fluorescence measurement
E. globulus aqueous extract affected the photochemical and non-photochemical status of the treated plants, with interactions depending on the mode of application (Fig 3). In eucalyptus-watered plants, in vivo measurements at the first 24 h after application revealed an initial damage (Fig 3) related to significant increases in fluorescence emission (φNO) (P ≤ 0.01) to the detriment of heat dissipation (φNPQ and qN). There were significant reductions in photochemical quenching (φII) and ETR (P ≤ 0.01) at 48 h, with concomitant increases in φNPQ and qN values. This increase was followed by a stimulation of the photosynthetic activity (qL) after 72 h and 96 h of treatment, which dropped significantly at the end of the assay (φII,qL and ETR), whereas φNPQ and qN increased again. The maximum PSII efficiency (Fv/Fm) was not affected. Nonetheless, in sprayed plants, the photosynthetic activity (φII, ETR and Fv/Fm) fell during the first 72 h, and then Fv/Fm recovered.
10.1371/journal.pone.0192872.g003
Significative differences of photosynthetic parameters on L. sativa adult plants treated with E. globulus aqueous extract by spraying vs. watering.
Positive (+) and negative (-) signs indicate increase or decrease with respect to the control. The number of signs indicates the level of statistical significance: one, P ≤ 0.05; two, P ≤ 0.01; three, P ≤ 0.001; independent samples t-test.
Growth parameters, photosynthetic pigments, and protein contents
Parameters measured on lettuce plants after harvesting are summarized in Fig 4. Eucalyptus-treated plants suffered conspicuous effects on morphological and biochemical variables measured at 5 days of treatment. When applied by spraying, eucalyptus aqueous extract had a significant effect on growth, reducing the aerial and root biomass (Fig 4A and 4C) and increasing the dry weight/fresh weight ratio (Fig 4B). When applied by watering, eucalyptus plants had similar or higher mean values of root biomass (Fig 4C) and length (Fig 4D) than those of control, whereas differences did not achieve statistical signification. However, the application by watering produced significant effects on the measured metabolites, thus reducing protein contents (Fig 4E) and chlorophyll concentrations (Fig 4F) with respect to control. Statistical analysis also revealed significant differences between application methods for dw/fw ratio of aerial biomass (P ≤ 0.001) in lettuce plants treated with eucalyptus aqueous extract (Fig 4B). Finally, no significant effects on carotenoid levels were observed between treatments or modes of application and neither visual symptoms of damage as leaf chlorosis or necrosis.
10.1371/journal.pone.0192872.g004
Phytotoxic effects of eucalyptus aqueous extracts on growth and physiological parameters of lettuce seedlings.
Bars represent mean values of three replicates ± SD. For each mode of application, mean values labeled with distinct letters are significantly different (P ≤ 0.05; independent samples t-test). For each treatment, asterisks indicate significant differences between watering and spraying (*P ≤ 0.05;**P ≤ 0.01;***P ≤ 0.001; independent samples t-test).
Chemical composition of eucalyptus aqueous extracts
From the HPLC analyses, 8 phenolic compounds and 5 organic acids were identified (Table 3). The phenolic profile of eucalyptus extract revealed the presence of three hydroxycinnamic acids (chlorogenic and two ρ-coumaric derivatives), and five flavonoids (ellagic acid, hyperoside, rutin, quercitrin, and kaempferol 3-O-glucoside). In relation to organic acids, shikimic and succinic acids were the major compounds (55.4%). For these two compounds, as well as for ellagic acid and kaempferol 3-O-glucoside, the HPLC-DAD did not throw a well-defined separation, making them not quantifiable as single compounds.
10.1371/journal.pone.0192872.t003
Chemical profile of Eucalyptus globulus aqueous extract.
Compound
RT a
Content (μg ·g-1 of lyophilized extract) b
Content (μg ·mL-1 of extract) c
% of each compound respect to the total
Phenolic compounds
Chlorogenic acid
15.6
1808.6 ± 1.6
11.7 ± 0.01
15.3
ρ-coumaric acid derivative ‘1’
17.5
242.3 ± 1.7
1.6 ± 0.01
2.1
ρ-coumaric acid derivative ‘2’
19.9
174.2 ± 0.2
1.1 ± 0.001
1.5
Hyperoside
38.1
2997.9 ± 9.4
19.4 ± 0.06
25.4
Rutin
39.6
1713.5 ± 10.8
11.1 ± 0.07
14.5
Quercitrin
43.2
648.2 ± 28.4
4.2 ± 0.18
5.5
Ellagic acid + Kaempferol 3-O-glucoside
43.7
not quantifiable
61.6
Organic acids
Citric acid
30
22493.2 ± 1745.6
145.3 ± 11.3
24.4
Malic acid
36.1
13891.9 ± 630.6
89.7 ± 4.1
15.1
Shikimic + Succinic acid
47.3
not quantifiable
55.4
Fumaric acid
62.1
4676 ± 164.5
30.2 ± 1.1
5.1
a RT = retention time in min
b Content (μg ·g-1 of lyophilized extract) = quantity of each compound present in 1 gram of lyophilized extract
c Content (μg ·mL-1 of extract) = quantity of each compound present in 1 mL of extract according with the yield of the lyophilized
Discussion
Germination and growth bioassays on lettuce and bentgrass as model target species, as well as tests measuring biochemical parameters and photosynthetic activity, have been frequently used to assess phytotoxicity of plant extracts [38–40]. In the same scenario, the measurement of physicochemical properties of aqueous extracts is commonly explored, since they can cause changes in cellular processes that could be misled as a possible phytotoxic effect. Taking into account that pH values between 5 and 7 [25], EC values below 2 dS m−1 [41] or osmolarity values of PEG lower than 0.1 osmol kg-1 [42] do not affect lettuce development, any inhibitory effect observed in our pre and post-emergence bioassays could be attributed a priori to the phytotoxins present in the plant aqueous extract. In our pre-emergence bioassays, the observed phytotoxicity confirmed the previous reports by Souto et al. [22] and Yamagushi et al. [10] wherein E. globulus aqueous extract inhibited lettuce germination and radicle growth. A progressive increase in inhibition of germination and radicle length was observed concomitantly to increase in extract concentration. For these cases, dose-response curves are useful for estimating parameters ED50 and ED80, which are important because they establish a frame of reference to which subsequent tests can be compared [28]. Furthermore, the identification of the phytotoxic dose of an aqueous extract could be useful for further bioassays in greenhouse and field conditions.
To determine the effect of post-emergence-applied aqueous extract, “the measurement of chlorophyll a fluorescence emitted by intact, attached leaves is thought to be a reliable, non-invasive method for monitoring photosynthesis and for judging the physiological status of the plant” [43]. For the assessment of post-emergence bioherbicide potential, the test performed with lettuce adult plants was useful to study the possible sites of action of the plant extracts, considering that their effects and mechanisms of action can be completely different in adult plants than in seedling metabolism, as well as depending on the application method [44]. Chlorophyll contents are closely related to the absorption and emission of energy, and any change in them is expected to lead a change in photosynthesis [45]. As stated Zhou and Yu [45], photoinhibition of photosynthesis by allelochemicals is typically characterized as a reduction in quantum yield of PSII photochemistry and a decrease in Chl fluorescence. Reduction in quantum yield can be evaluated by the ratio of variable to maximum fluorescence (Fv/Fm). If a plant cannot emit the excess energy received from the sun, this excess energy is transferred to oxygen via chlorophyll, resulting in photo-oxidation damage. Excessive damage leads to membranes destruction and chlorophyll oxidation. In our bioassay, watering application of eucalyptus aqueous extract revealed more general conspicuous phytotoxic effects than the spraying method. A reduction in photochemical quenching (φII) and ETR, with the decline of chlorophyll a + b was detected in watered-plants, which indicates that the biochemical phase of photosynthesis was directly affected by the exogenous application of eucalyptus; however, lettuce plants could activate mechanisms of regulated energy dissipation in the form of heat (increase in φNPQ and qN) and then acclimate [43]. In agreement with our results, Batish et al. [46] found that total chlorophyll content and respiratory activity were reduced in response to eucalypt oil in all tested species. Similarly, extracts of abscised leaves of eucalyptus have been shown to reduce chlorophyll content on crops, effect that was related to a possible poor photosynthesis and, as a result, a poor plant growth [21]. Together with the effects described on photosynthesis and chlorophyll contents, protein concentration was also significantly reduced in our eucalyptus-watered plants. Those effects might indicate an inhibition of the synthesis of these compounds in the leaves as a symptom of early stress caused by phytotoxicity, which is still not reflected at whole plant growth level. These results are in conformity with those of Djanaguiraman et al. [47], who detected reductions in chlorophyll and protein content in blackgram, rice and sorghum seedlings by E. globulus leachates assayed at different concentrations. In our case of spraying application, and differently to watering, eucalyptus aqueous extract significantly inhibited plant growth, and increased dry weight/fresh weight ratio of aerial biomass, without affecting protein or chlorophyll contents. Such decrease in growth can be a consequence of the early inhibition of photosynthetic efficiency measured as Fv/Fm, which was then restored as a symptom of acclimation. Root biomass resulted as well diminished in sprayed-plants, suggesting a systemic behavior. Such observations could be reflecting different modes of action depending on the site of phytotoxins entry, growth and morphological parameters being early affected by spraying on leaves, and physiological traits more affected by watering.
Despite the conspicuous inhibition or reduction detected for some physiological and/or morphological parameters, external symptoms of damage as chlorosis or necrosis were absent in lettuce adult plants. So, the lack of remarkable effects on lettuce, being a standard target species chosen for its high sensitivity to allelochemicals, led us to discard the use of eucalyptus aqueous extract as a post-emergence bioherbicide, which effects would be agronomically irrelevant in the context of weed control.
In the present study, we have used natural aqueous extracts because water is the extraction solvent in nature, so the use of aqueous extraction simulated the natural release of water-soluble phytotoxins into the environment. Moreover, the advantage in utilizing aqueous extracts is given by the joint action of several compounds present in them and not only by a simple compound, considering that many authors demonstrated that a mixture of compounds could be more phytotoxic than their respective individual compounds [3,48,49]. Most of the germination and growth inhibitors present in aqueous extracts are phenolic compounds [50], and have been widely reported to affect many physiological processes [45,51], viz. phytohormone activity, mineral uptake, plant water balance and stomatal function, photosynthesis, respiration, organic synthesis of certain compounds and flow of carbon [52]. Via HPLC analysis, the major phytotoxic substances identified in our eucalyptus leaf aqueous extract were hyperoside and the mixtures of ellagic acid-kaempferol 3-O-glucoside and shikimic-succinic acids. Of these, hyperoside was also found as the main flavonoid in the E. globulus phenolic profile by Deszi et al. [18], and the presence of ellagic acid is in conformity with Almeida et al. [16], Amakura et al. [17], Boulekbache-Makhlouf et al. [6] or Souto et al. [22]. Most of the compounds identified here are well-known phytotoxins, so their occurrence in our aqueous extract can explain the phytotoxic effects described when applied both in pre- and post-emergence on the STS. Moreover, the release of these and other compounds can underlie the herbicidal activity observed when E. globulus leaves are incorporated into the soil as a green manure [15]. Chon et al. [49] detected chlorogenic and ρ-coumaric acids in Xanthium occidentale water fraction and correlated their presence and amount with the phytotoxicity observed from the extract. Mersie and Singh [53] also found an inhibition of photosynthesis in Abutilon theophrasti leaf cells by the action of these phenolic acids. Rutin was suggested as the major allelochemical in buckwheat by Golisz et al. [54], while Fujii et al. [55] observed a significant inhibitory activity when tested against lettuce seedlings. In another report, the effect of ellagic acid on Arabidopsis fresh weight appeared to be mainly due to root damage [56].
Regarding other low molecular weight organic acids, from our knowledge, this is the first time that the organic acid composition from E. globulus leaf aqueous extract is reported. In other frameworks, Silva et al. [57] showed the presence of succinic, fumaric, malic and citric acids in root tips of six eucalyptus species, and suggested that their synthesis and root exudation could contribute to the adaptation of these species to acid Al-toxic soils. Zhang et al. [58] showed that both malic and citric acid inhibited SOD activity and reduced the fresh weight of melon, the latter being also an inhibitor of radicle and hypocotyl growth. On the other hand, An et al. [48] concluded that succinic acid showed weak phytotoxic strength, however, it was considered as one of the quantity-dominant compounds which makes it as a high contributor to phytotoxicity. Besides the occurrence of these organic acids probably contributing to phytotoxicity, the presence of high amounts of shikimic acid in the eucalyptus extract could be an indication of a high potential for secondary metabolites production, since it is a key intermediate in the formation of numerous types of secondary compounds (including phenolic acids and flavonoids) [59,60].
Conclusions
The combination of methods carried out in this study has demonstrated that aqueous extract from E. globulus leaves exhibit phytotoxic effects on germination, growth and some physiological parameters of standard target species. Despite some phytotoxic effects were found on lettuce adult plant physiology and morphology, the use of eucalyptus aqueous extract will be discarded in post-emergence but can be promising as a pre-emergence bioherbicide. It is concluded that E. globulus synthesizes a cocktail of phytotoxic compounds that can be released from leaf residues applied to the soil, and then interfere with the germination and development of other species.
The authors thank the people from Laboratory of Pharmacognosy, especially Rui Gonçalves, for his constant and reliable assistance in chemical analyses.
ReferencesCordeauS, TrioletM, WaymanS, SteinbergC, GuilleminJP. Bioherbicides: dead in the water? A review of the existing products for integrated weed management. . 2016; 87: 44–49.ReigosaMJ, SoutoXC, GonzálezL. Effect of phenolic compounds on the germination of six weed species. . 1999; 28: 83–89.ReigosaMJ, Pazos-MalvidoE. Phytotoxic effects of 21 plant secondary metabolites on Arabidopsis thaliana germination and root growth. . 2007; 33: 1456–1466. doi: 10.1007/s10886-007-9318-x17577597GerigTM, BlumU, MeierK. Statistical analysis of the joint inhibitory action of similar compounds. . 1989; 15 (10): 2403–2412. doi: 10.1007/BF0102037124271537Inderjit. Plant Phenolics in Allelopathy. . 1996; 62 (2): 186–202.Boulekbache-MakhloufL, MeudecE, MazauricJP, MadaniK, CheynierV. Qualitative and semi-quantitative analysis of phenolics in Eucalyptus globulus leaves by high-performance liquid chromatography coupled with diode array detection and electrospray ionisation mass spectrometry. . 2013; 24: 162–170. doi: 10.1002/pca.239622930658BatishDR, SinghHP, KohliRK, KaurS. Eucalyptus essential oil as a natural pesticide. . 2008; 256: 2166–2174.ZhangJ, AnM, WuH, StantonR, LemerleD. Chemistry and bioactivity of Eucalyptus essential oils. . 2010; 25: 313–330.BagavathyS, XavierGSA. Effects of aqueous extract of Eucalyptus globulus on germination and seedling growth of sorghum. . 2007; 20: 395–402.YamagushiMQ, GusmanGS, VestenaS. Allelopathic effect of aqueous extracts of Eucalyptus globulus Labill. and of Casearia sylvestris Sw. on crops. . 2011; 32:1361–1374.DejamM, KhaleghiSS, AtaollahiR. Allelopathic effects of E. globulus Labill. on seed germination and seedling growth of eggplant (Solanum melongena L.). . 2014; 3 (1): 81–86.MorsiMM, AbdelmigidHM. Allelopathic activity of Eucalyptus globulus leaf aqueous extract on Hordeum vulgare growth and cytogenetic behavior. . 2016; 10 (11): 1551–1556.PadhyB, PatnaikPK, TripathyAK. Allelopathic potential of Eucalyptus leaf litter leachates on germination and seedling growth of fingermillet. . 2000; 7: 69–78.BabuRC, KandasamyOS. Allelopathic effect of Eucalyptus globulus Labill. on Cyperus rotundus L. and Cynodon dactylon L. Pers. . 1997. 179: 123–126.PuigCG, Álvarez-IglesiasL, ReigosaMJ, PedrolN. Eucalyptus globulus leaves incorporated as green manure for weed control in maize. . 2013; 61: 154–161.AlmeidaIF, FernandesE, LimaJLFC, ValentãoP, AndradePB, SeabraRM, et al. Oxygen and nitrogen reactive species are effectively scavenged by Eucalyptus globulus leaf water extract. . 2009; 12: 175–183. doi: 10.1089/jmf.2008.004619298212AmakuraY, YoshimuraM, SugimotoN, YamazakiT, YoshidaT. Marker constituents of the natural antioxidant eucalyptus leaf extract for the evaluation of food additives. . 2009; 75: 1060–1065.DezsiS, BadarauAS, BischinC, VodnarDC, Silaghi-DumitrescuR, GheldiuAM, et al.Antimicrobial and antioxidant activities and phenolic profile of Eucalyptus globulus Labill. and Corymbia ficifolia (F. Muell.) K. D. Hill & L. A. S. Johnson leaves. . 2015; 20: 4720–4734. doi: 10.3390/molecules2003472025786160GullónB, GullónP, Lú-ChauTA, MoreiraMT, LemaJM, EibesG. Optimization of solvent extraction of antioxidants from Eucalyptus globulus leaves by response surface methodology: Characterization and assessment of their bioactive properties. . 2017; 108: 649–659.El-RokiekKG, MessihaNK, El-MasryRR, Saad El-DinSA. Evaluating the leaf residues of Eucalyptus globulus and Mangifera indica on growth of Cynodon dactylon and Echinochloa colonum. . 2011; 7: 1793–1799.JayakumarM, EyiniM, Pannirselvam. Allelopathic effect of Eucalyptus globulus Labill. in groundnut and corn. . 1990; 15 (3): 109–113.SoutoXC, GonzálezL, ReigosaMJ. Comparative-analysis of allelopathic effects produced by 4 forestry species during decomposition process in their soils in Galicia (NW Spain). . 1994; 20: 3005–3015. doi: 10.1007/BF0209840524241931XuanTD, ShinkichiT, KhanhTD, ChungIM. Biological control of weeds and plant pathogens in paddy rice by exploiting plant allelopathy: An overview. . 2005; 24 (3): 197–206.DayanFE, DukeSO. Clues in the search for new herbicides. In: ReigosaMJ, PedrolN, GonzálezL, editors. . Springer, Dordrecht, Netherlands. 2006. pp: 63–84.MacíasFA, CastellanoD, MolinilloJMG. Search for a standard phytotoxic bioassay for allelochemicals. Selection of standard target species. . 2000; 48: 2512–2521. 10888578MayerAM, Poljakoff-MayberA. . Pergamon Press, New York. 1963.ChiapusioG, SánchezAM, ReigosaMJ, GonzálezL, PellissierF. Do germination indices adequately reflect allelochemical effects on the germination process? . 1997; 23: 2445–2453.DayanFE, RomagniJG, DukeSO. Investigating the mode of action of natural phytotoxins. . 2000; 26:2079–2094.HoaglandDR, ArnonDI. The water-culture method of growing plants without soil. . Univ. of California, Berkeley, CA. 1950.KrauseGH, VernotteC, BriantaisJM. Photoinduced quenching of chlorophyll fluorescence in intact chloroplasts and algae. . 1982; Acta 679:16–24.BilgerW, BjörkmanO. Role of the xanthophyll cycle in photoprotection elucidated by measurements of light-induced absorbance changes, fluorescence and photosynthesis in Hedera camariensis. . 1990; 25:173–185. doi: 10.1007/BF0003315924420348Demmig-AdamsB, AdamsWWIII, LoganBA, VerhoevenAS. Xanthophyll-cycle-dependent energy dissipation and flexible photosystem II efficiency in plants acclimated to light stress. . 1995; 22: 249–260.GentyB, BriantaisJ-M, BakerNR. The relationship between quantum yield of photosynthetic electron transport and quenching of chlorophyll fluorescence. . 1989; 990: 87–92.KramerDM, JohnsonG, KiiratsO, EdwardsGE. New fluorescence parameters for the determination of QA redox state and excitation energy fluxes. . 2004; 79: 209–218. doi: 10.1023/B:PRES.0000015391.99477.0d16228395WellburnAR. The spectral determination of chlorophylls a and b, as well as total carotenoids, using various solvents with spectrophotometers of different resolution. . 1994; 144: 307–313.PedrolN, RamosP, ReigosaMJ. Phenotypic plasticity and acclimation to long-term water deficits in velvetgrass: a greenhouse experiment. Changes in leaf morphology, photosynthesis and stress-induced metabolites. . 2000; 157: 383–393.OliveiraAP, ValentãoP, PereiraJA, SilvaBM, TavaresF, AndradePB. Ficusarica L.: Metabolic and biological screening. . 2009; 47: 2841–2846. doi: 10.1016/j.fct.2009.09.00419747518AliottaG, CafieroG, Martínez-OteroA. Weed germination, seedling growth and their lesson for allelopathy in agriculture. In: ReigosaMJ, PedrolN, GonzálezL, editors. . Springer, Netherland; 2006. pp: 285–297.de Jesus JatobaL, VarelaRM, MolinilloJMG, Ud DinZ, Juliano GualtieriSC, Rodrigues-FilhoE, et al. Allelopathy of Bracken Fern (Pteridium arachnoideum): New Evidence from Green Fronds, Litter, and Soil. . 2016; 11(8): e0161670. doi: 10.1371/journal.pone.016167027552161HoaglandRE, WilliamsRD. Bioassays—Useful Tools for the Study of Allelopathy. In: MacíasFA, GalindoJCG, MolinilloJMG, CutlerHG, editors. . CRC-Press, Boca-Raton, Florida. 2004. pp: 315–351.SouzaLS, VeliniED, Maiomoni-RodellaRCS. Allelopathic effect of weeds and concentrations of Brachiaria decumbens on the initial development of eucalyptus (Eucalyptus grandis). . 2003; 21: 343–354.Álvarez-IglesiasL, PuigCG, GarabatosA, ReigosaMJ, PedrolN. Vicia faba aqueous extracts and plant material can supress weeds and enhance crops. . 2014; 34: 299–314.EfeoğluB, EkmekçiY, ÇiçekN. Physiological responses of three maize cultivars to drought stress and recovery. . 2009; 75: 34–42.GrañaE, SoteloT, Díaz-TielasC, ReigosaMJ, Sánchez-MoreirasA. The phytotoxic potential of the terpenoid citral on seedlings and adult plants. . 2013; 61: 469–481.ZhouYH, YuJQ. Allelochemicals and photosynthesis. In: ReigosaMJ, PedrolN, GonzálezL, editors. . Springer, Netherland. 2006; pp: 127–156.BatishDR, SetiaN, SinghHP, KohliRK. Phytotoxicity of lemon-scented eucalypt oil and its potential use as a bioherbicide. . 2004; 23: 1209–1214.DjanaguiramanM, VaidyanathanR, SheebaJA, DeviDD, BangarusamyU. physiological responses of Eucalyptus globulus leaf leachate on seedling physiology of rice, sorghum and blackgram. 2005; 7(1): 35–38.AnM, PratleyJE, HaigT. Phytotoxicity of vulpia residues: III. Biological activity of identified allelochemicals from Vulpia myuros. . 2001; 27 (2): 383–394. 14768822ChonSU, KimYM, LeeJC. Herbicidal potential and quantification of causative allelochemicals from several Compositae weeds. . 2003; 43:444–450.RiceEL. . 2nd ed. Academic Press, Orlando. 1984. pp: 189.MacíasFA, MolinilloJMG, VarelaRM, GalindoJCG. Allelopathy—a natural alternative for weed control. . 2007; 63:327–348. doi: 10.1002/ps.134217348068EinhelligFA. Mode of allelochemical action of phenolic compounds. In: MacíasFA, GalindoJCG, MolinilloJMG, CutlerHG, editors. . CRC Press, Boca Raton, Florida. 2004. pp: 217–238.MersieW, SinghM. Phenolic acids affect photosynthesis and protein synthesis by isolated leaf cells of velvet-leaf. . 1993; 19:1293–1301. doi: 10.1007/BF0098487624249162GoliszA, LataB, GawronskiSW, FujiiY. Specific and total activities of allelochemicals identified in buckwheat. . 2007; 7: 164–171.Fujii Y, Golisz A, Furubayashi A, Iqbal Z, Nasir H. Allelochemicals from buckwheat and Tartary buckwheat and practical weed control in the field. Proceedings of the 20th Asian-Pacific Weed Science Society Conference. Ho Chi Minh City, Vietnam. 2005; 227–223.QinB, PerryLG, BroecklingCD, DuJ, StermitzFR, PaschkeMW, et al. Phytotoxic allelochemicals from roots and root exudates of leafy spurge (Euphorbia esula L.). . 2006; 1(6): 323–327. 19517003SilvaIR, NovaisRF, JhamGN, BarrosNF, GebrimFO, NunesFN, et al. Responses of eucalypt species to aluminum: the possible involvement of low molecular weight organic acids in the Al tolerance mechanism. . 2004; 24: 1267–1277. 15339736ZhangZZ, SunZH, ChenWH, LinWX. Allelopathic effects of organic acid allelochemicals on melon. . 2013; 33: 4591–4598.HerrmannKM, WeaverLM. The shikimate pathway. . 1999; 50: 473–503.SeiglerDS. Basic pathways for the origin of allelopathic compounds. In: ReigosaMJ, PedrolN, GonzálezL, editors. . Springer, Netherland. 2006. pp: 11–61.