Physiological and biochemical effects of <i>Lantana camara</i> L. allelochemicals on the seed germination of <i>Avena sativa</i> L.

Gindri, Diego Medeiros; Coelho, Cileide Maria Medeiros; Uarrota, Virgilio Gavicho

doi:10.1590/1983-40632020v5062546

ABSTRACT

Lantana camara (L.) is considered one of the main weeds of agricultural crops, and allelochemicals produced by this species may be a source for the development of natural herbicides. In this study, phytotoxic effects of L. camara aqueous extracts on seed germination and seedling growth of Avena sativa (L.) were assessed. The experimental design was completely randomized, in a 2 x 5 factorial scheme, with treatments resulting from two assays, testing five concentrations of the extract (0 %, 2.5 %, 5.0 %, 7.5 % and 10 %; vv^-1). During the seed germination, physiological (e.g., seed imbibition, germination and vigor) and biochemical (e.g., catalase, ascorbate peroxidase, proline, phenols, malondialdehyde and hydrogen peroxide) proprieties were evaluated. The leaf extracts of L. camara affected the response variables on A. sativa by reducing the germination speed index (phases I and II) and seed viability (phase III of germination), thus causing a solute leakage and increasing the production of reactive oxygen forms and, finally, lipid peroxidation. Extract concentrations above 2.5 % inhibit the growth of epicotyls. Therefore, the studied allelochemicals showed potential to be exploited in the development of natural herbicides.

KEYWORDS:
Antioxidant system; bioactive compounds; seed physiology; phytotoxicity

RESUMO

Lantana camara (L.) é considerada uma das principais plantas invasoras de culturas agrícolas, e aleloquímicos produzidos por essa espécie podem ser fonte para o desenvolvimento de herbicidas naturais. Avaliaram-se efeitos fitotóxicos de extratos aquosos de L. camara sobre a germinação de sementes e o crescimento de plântulas de Avena sativa (L.). O delineamento experimental foi completamente randomizado, em esquema fatorial 2 x 5, com tratamentos resultantes de dois ensaios, testando-se cinco concentrações do extrato (0 %, 2,5 %, 5,0 %, 7,5 % e 10 %; vv^-1). Durante a germinação das sementes, foram avaliadas propriedades fisiológicas (e.g., embebição, germinação e vigor de sementes) e bioquímicas (e.g., catalase, ascorbato peroxidase, prolina, fenóis, malondialdeído e peróxido de hidrogênio). Os extratos foliares de L. camara afetaram as variáveis respostas em A. sativa, reduzindo o índice de velocidade de germinação (fases I e II) e a viabilidade das sementes (fase III da germinação), provocando, então, vazamento de soluto e aumento da produção de formas reativas de oxigênio e, finalmente, peroxidação lipídica. Concentrações de extrato acima de 2,5 % inibem o crescimento de epicótilos. Portanto, os aleloquímicos estudados mostraram potencial para exploração no desenvolvimento de herbicidas naturais.

PALAVRAS-CHAVE:
Sistema antioxidante; compostos bioativos; fisiologia de sementes; fitotoxicidade

INTRODUCTION

Allelochemicals are mainly secondary metabolites produced by plants or with microbial origin, which influence the growth or development of biological systems (IAS 1996).

Lantana camara (L.), as a perennial aromatic shrub of the Verbenaceae family, is considered worldwide as a major invasive plant (Chengxu et al. 2011CHENGXU, W.; MINGXING, Z.; XUHUI, C.; BO, Q. Review on allelopathy of exotic invasive plants. Procedia Engineering, v. 18, n. 1, p. 240-246, 2011.).

Among the metabolites found in L. camara, 1,8-cineol, β-pinene, dipentene, lantadene A and lantadene D have been cited as important intermediate sources for herbicide development (Kegge & Pierik 2010KEGGE, W.; PIERIK, R. Biogenic volatile organic compounds and plant competition. Trends in Plant Science, v. 15, n. 3, p. 126-132, 2010., Mishra 2015MISHRA, A. Allelopathic properties of Lantana camara. International Research Journal of Basic and Clinical Studies, v. 3, n. 1, p. 13-28, 2015. , Latif et al. 2017LATIF, S.; CHIAPUSIO, G.; WESTON, L. A. Allelopathy and the role of allelochemicals in plant defence. In: BECARD, G. (ed.). Advances in botanical research. Wagga Wagga: Academic Press, 2017. p. 19-54., Gindri et al. 2020GINDRI, D. M.; COELHO, C. M. M.; UARROTA, V. G.; REBELO, A. M. Herbicidal bioactivity of natural compounds from Lantana camara on the germination and seedling growth of Bidens pilosa. Pesquisa Agropecuária Tropical, v. 50, e57746, 2020.).

Allelopathic compounds (e.g., phenolics, terpenoids, alkaloids and their derivatives) are reported to inhibit seed germination and reduce the germination speed index and seedling growth (Abu-Romman et al. 2010, Hussain & Reigosa 2011HUSSAIN, M. I.; REIGOSA, M. J. Allelochemical stress inhibits growth, leaf water relations, PSII photochemistry, non-photochemical fluorescence quenching, and heat energy dissipation in three C3 perennial species. Journal of Experimental Botany, v. 62, n. 13, p. 4533-4545, 2011.). Such phytotoxity effects occur because of their action on cellular degradation processes through the production of reactive oxygen species, resulting in cellular oxidative stress (Bogatek & Gniazdowska 2007BOGATEK, R.; GNIAZDOWAKA, A. ROS and phytohormons in plant-plant allelopathic interaction. Plant Signaling & Behavior, v. 2, n. 4, p. 317-318, 2007., Qian et al. 2009QIAN, H.; XU, X.; CHEN, W.; JIANG, H.; JIN, Y.; LIU, W.; FU, Z. Allelochemical stress causes oxidative damage and inhibition of photosynthesis in Chlorella vulgaris. Chemosphere, v. 75, n. 3, p. 368-375, 2009. ).

The mechanisms that define how the allelochemicals of L. camara act have not been described yet. The response to alelochemicals leads to the induction of adaptive changes in the biochemical and gene expression of plants, such as induction of the enzymatic and non-enzymatic antioxidant defense system. The ability of the cell to cope with the oxidative stress produced by alellochemicals will largely depend on the endogenous free radical scavenging capacity of the species (Mittler 2017MITTLER, R. ROS are good. Trends in Plant Science, v. 22, n. 1, p. 11-19, 2017.).

In general, abiotic and biotic stresses will induce perturbations in the fruit cellular homeostasis, which will then result in an increased generation of reactive oxygen species. When the free radicals scavenging capacity exceeds the endogenous scavenging, reactive oxygen species interact with sensors that will initiate cascade reactions and also up-regulation of transcription factors (Toivonen & Hodges 2011TOIVONEN, P. M. A.; HODGES, D. M. Abiotic stress in harvested fruits and vegetables. In: SHANKER, A. (ed.). Abiotic stress in plants: mechanisms and adaptations. Croatia: InTech, 2011. p. 39-58. ), resulting in oxidative stress.

Studies on enzymatic activity, free radical content, cell membrane system integrity and other tests routinely used for seed vigor and germination may be important tools in elucidating the action mechanisms of allelopathic compounds. Moreover, despite the extensive literature about the effects of L. camara allelochemicals, studies regarding such effects on Avena sativa are still scarce. In this research, it was hypothesized that L. camara extracts affect physiological and biochemical proprieties of A. sativa seed germination and, therefore, have a potential to be used in the development of natural herbicides. This study aimed to evaluate such effects.

MATERIAL AND METHODS

Commercial seeds of A. sativa were obtained from the seed laboratory of the Universidade do Estado de Santa Catarina and stored in a dry and cold chamber (50 ± 5 % relative humidity and 8 ± 2 ºC), until analysis, and L. camara leaves were collected from wild plants in the city of Lages, Santa Catarina state, Brazil. Leaves were then washed using distilled water and dried in an oven with air circulation at 40 ºC, for 72 h. After drying, the leaves were shredded and stored in a dry and cold chamber (50 ± 5 % relative humidity and 8 ± 2 ºC), until analysis. The extracts were prepared by mixing 10 g of leaf powder in 90 mL of distilled water (25 ºC, for 24 h). The mixture was filtered and then centrifuged at 3,600 rpm, for 10 min. The resulting supernatant (crude extract) was diluted in distilled water to obtain the different tested extract concentrations: 0 %, 2.5 %, 5.0 %, 7.5 % and 10 % (vv^-1).

For the viability and vigor tests, four replications of 25 seeds were sown in acrylic boxes (12 cm x 12 cm), on three sheets of germitest paper moistened 2.5 times the weight of the dry paper with water and extracts in the different concentrations. The boxes were transferred to a biochemical oxygen demand (BOD) chamber at 25 ºC and 12-h photoperiod.

The samples for seed imbibition assessment were prepared in the same way; but, after the seed preparation at each different time (0, 3, 6, 9, 12, 18, 24, 36, 48, 72 and 96 h), two samples of 25 seeds were kiln dried (105 ºC, for 24 h) to determine the moisture. The imbibition curve was obtained by using the difference of humidity between the times.

For seed germination, after preparation, the seeds remained in water (control) or in each one of the L. camara extract concentrations, until seven days after sowing. Also, in the beginning of the germination phase III (root protrusion), a part of the seeds previously exposed only to water at the germination phases I and II were transferred to boxes containing the extract at different concentrations; and those previously exposed to the extract were transferred to boxes with water. The results were expressed as percentage of normal seedlings.

The germination speed index (GSI) was evaluated by counting, every 12 h of the assay, the total number of germinated seeds (root protrusion of 2 mm), until a constant number of germinated seeds. Thus, it was calculated according to following equation: $GSI (%) = \sum [G_{S 1} / C_{1}) + (G_{S 2} / C_{2}) + \dots + (G_{Sn} / C_{n})] \times 100$ , where: $C_{1}, C_{2} \dots C_{n}$ represent the first, second and n^th seed counts, and $G_{S 1}, G_{S 2} \dots G_{Sn}$ are the respective numbers of germinated seeds at these counts (Souza-Filho et al. 2010).

To evaluate the vigor by electrical conductivity, four replications of 50 seeds were previously weighed and soaked (1 h) in the different extract concentrations (0 %, 2.5 %, 5.0 %, 7.5 % and 10 %). After imbibition, the seeds were washed in distilled water, transferred to a cylindrical flat bottom beaker containing distilled water (50 mL) and stored in a BOD chamber (20 ºC/24 h). The electrical conductivity was evaluated after 24 h, with results expressed as µS cm^-1 g^-1 of seeds (Vieira & Carvalho 1994VIEIRA, R. D.; CARVALHO, N. M. Testes de vigor em sementes. Jaboticabal: Funep, 1994.).

In the evaluation of vigor by initial seedling growth, after preparation, the hypocotyl and root length, as well as the presence of secondary roots, were then measured. The results were expressed as growth inhibition rate and presence of secondary roots rate (Nakagawa 1999NAKAGAWA, J. Testes de vigor baseados no desempenho de plântulas. In: KRZYZANOWSKI, F. C.; VIEIRA, R. D.; FRANÇA NETO, J. B. (ed.). Vigor de sementes: conceitos e testes. 2. ed. Londrina: Abrates, 1999. p. 1-24.).

The biochemical properties measured in this study were contents of malondialdehyde (MDA) and hydrogen peroxide (H₂O₂), enzymatic activities of catalase and ascorbate peroxidase, as well as proline and total phenolic compounds contents.

For the MDA and H₂O₂ determination, seed samples (200 mg) were macerated in liquid nitrogen and homogenized in 2 mL of trichloroacetic acid (TCA) 0.1 %. The homogenate was centrifuged at 3,600 rpm, for 15 min, and the supernatant recovered. For MDA, the assay mixture consisted of 20 % of TCA and 0.5 % of thiobarbituric acid. The reaction was performed by mixing 250 µL of supernatant and 1 mL of the mixture, followed by incubation in water bath (95 ºC) for 30 min. Then, the reaction was stopped on ice (10 min). The samples were left to stand at room temperature for 10 min, and absorbance was measured using a spectrophotometer at 600 nm and 535 nm. The results were expressed as µmol g^-1 of fresh mass (Heath & Packer 1968HEATH, R. L.; PACKER, L. Photoperoxidation in isolated chloroplasts: I. Kinetics and stoichiometry of fatty acid peroxidation. Archives in Biochemistry and Biophysics, v. 125, n. 1, p. 189-198, 1968.).

The reaction mixture for H₂O₂ consisted of 200 µL of supernatant, 800 µL of potassium iodide and 200 µL of phosphate buffer (0.1 M; pH 7.5), followed by incubation on ice during 1 h. Then, the samples were left to stand at room temperature for 5 min and absorbance readings were recorded using a spectrophotometer at 390 nm, with results expressed as nmol g^-1 of fresh mass (Alexieva et al. 2001ALEXIEVA, V.; SERGIEV, I.; MAPELLI, S.; KARANOV, E. The effect of drought and ultraviolet radiation on growth and stress markers in pea and wheat. Plant Cell Environment, v. 24, n. 12, p. 1337-1344, 2001. ). Both assays were performed with three replicates.

To enzyme extraction and protein determination, fresh samples collected at 24, 48, 72 and 120 h of germination were macerated in a mortar using liquid nitrogen, and 1 g of sample was homogenized with 1.8 mL of 100 mM potassium phosphate buffer (pH 7.8) containing 0.1 mM of ethylenediaminetetraacetic acid (EDTA) and 20 % of polyvinylpolypyrrolidone (PVPP). The extract was centrifuged at 13,000 g/20 min (4 ºC) and the supernatant was used to determine the enzymatic activities (Bradford 1976BRADFORD, M. M. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Analytical Biochemistry, v. 72, n. 1-2, p. 248-254, 1976. ).

The catalase activity (CAT - EC 1.11.1.6) was assayed spectrophotometrically at 25 ºC, in a reaction mixture containing 1 mL of 100 mM potassium phosphate buffer (pH 7.5) plus 2.5 µL of H₂O₂ (25 % solution), prepared immediately before its use. The reaction was started by the addition of 25 µL of plant extract, and the catalase activity was monitored by H₂O₂ degradation at 240 nm, over a 1-min period (Azevedo et al. 1988).

The ascorbate peroxidase activity (APX - EC 1.11.1.11) was assayed by monitoring the oxidation rate of ascorbate during 2 min at 290 nm (ε = 2.80 x 103 M^-1 cm^-1). The reaction mixture consisted of 13 mL of 100 mM potassium phosphate buffer (pH 7.0), 2 mL of 0.5 mM ascorbic acid and 2 mL of 1 mM EDTA. The reaction was started by adding 1,780 µL of the reaction medium, 200 µL of 0.1 mM H₂O₂ and 20 µL of the enzyme extract. The results, such as for the catalase, were expressed as µmol min^-1 mg prot^-1 (Nakano & Asada 1981NAKANO, Y.; ASADA, K. Hydrogen peroxide is scavenged by ascorbate-specific peroxidase in spinach chloroplasts. Plant Cell Physiology, v. 22, n. 5, p. 867-880, 1981.).

To quantify the proline content, seed samples (0.3 mg) were macerated in liquid nitrogen and homogenized in 6 mL of sulfosalicylic acid (3 %). The homogenate was centrifuged at 3,600 rpm for 30 min and the supernatant was used. Proline was determined by mixing 2 mL of the supernatant, 2 mL of an acidic ninhydrin solution and 2 mL of glacial acetic acid. The reaction mixture was incubated in water bath (100 ºC, for 60 min) and left to stand on ice for 10 min. After that, 2 mL of toluene were added and the mixture rested for 20 min at room temperature, for phase separation. The upper phase was collected and absorbance readings were performed spectrophotometrically at 520 nm. The results were expressed as µmol g^-1 of fresh mass (Bates et al. 1973BATES, L. S.; WALDREN, R. P.; TEARE, I. D. Rapid determination of free proline for water stress studies. Plant and Soil, v. 39, n. 1, p. 205-207, 1973. ).

The total phenolic compounds were similarly quantified from the seed samples (0.3 mg), also macerated in liquid nitrogen, homogenized in 3 mL of acidified methanol (1 mL of hydrochloric acid + 100 mL of methanol at 80 %) and centrifuged (3,600 rpm, for 30 min). Thus, the supernatant (100 µL) was mixed with 700 µL of Folin-Ciocalteau (0.25 M) and incubated in the dark for 3 min. Then, 700 µL of Na₂CO₃ (0.2 M) were added and incubated in the dark for 30 min. The absorbance readings were carried out spectrophotometrically at 725 nm. The results were expressed as mg GAE (gallic acid equivalent) g^-1 of fresh mass (Folin & Ciocalteu 1927).

The data for all variables were summarized, subjected to normality (Shapiro-Wilk) and homogeneity (Levene) tests, and analyses of variance (Anova) were conducted. Two independent analyses were performed, because the statistical results showed no significant differences between the experiments. The results are presented as mean and standard deviation of all replicates, and the response variables were submitted to regression analysis. The best models displayed in graphics were selected according to the higher R-squared and lower Akaike Information Criterium (AIC). All statistical analyses were performed by the R software (R Core Team 2019).

RESULTS AND DISCUSSION

The reduction of water potential during seed germination may result in lower germination rates, or even its inhibition (Cardoso 2004CARDOSO, V. J. M. Germinação. In: KERBAUY, G. B. (ed.). Fisiologia vegetal. 2. ed. Rio de Janeiro: Guanabara Koogan, 2004. p. 386-407.). Under full water availability, the imbibition of A. sativa seeds presents a three-phase curve. In the phase I, the water content in the seed increases rapidly, what is followed by a stabilization in the phase II, until the protrusion of the radicle, thus starting the phase III, with another increase in water content due to the growth of the embryo (Bewley et al. 2013BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. Germination. In: BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. (ed.). Seeds: physiology of development, germination and dormancy. 3. ed. New York: Springer, 2013. p. 133-182.).

The three-phase seed germination pattern was observed for all treatments in the imbibition curve, with a rapid absorption of water up to 9 h, a phase of low water absorption between 9 h and 36 h, and a recovery in the water absorption rate after 48 h. The results indicate that the osmotic potential of aqueous solutions of L. camara leaves did not interfere in the water absorption of the seeds.

The germination of A. sativa seeds, expressed as percentage of normal seedlings, was not affected by the aqueous extract concentrations of L. camara leaves, when exposed to the phases I and II of germination (Figure 1A). However, the germination of the seeds, when they were exposed to the extract in the phase III, was significantly affected at all concentrations of the extract (Figure 1B). In the phase III, the seed germination from 78 ± 5 % in the control treatment was reduced to 54 % ± 1, 43 % ± 12, 14 % ± 8 and 6 % ± 6, respectively, at aqueous extract concentrations of 2.5 %, 5 %, 7.5 % and 10 % (vv^-1). Also, when A. sativa seeds were exposed to the extract during all the germination phases (I, II and III), there was a reduction of the percentage of normal seedlings for all extract concentrations (Figure 1C). In these treatments, because of the longer exposure time to the extract (from phase I to III), there was a greater damage to seed germination. The seed germination was completely inhibited at the aqueous extract concentration of 10 % (vv^-1).

Figure 1
Regressions for the percentage of normal seedlings, when Avena sativa seeds were exposed to the Lantana camara extract, at different concentrations (%; vv^-1), in the germination phases I and II (A), III (B) or during the three phases (C). The bars for observed points are the mean standard deviations.

According to Kupidlowska et al. (1994)KUPIDLOWSKA, E.; DOBRZYNSKA, K.; PARYS, E.; ZOBEL, A. M. Effect of coumarin and xanthotoxin on mitochondrial structure, oxygen uptake, and succinate dehydrogenase activity in onion root cells. Journal of Chemical Ecology, v. 20, n. 10, p. 2471-2480, 1994., the phyto-chemical coumarin found in L. camara leaves by Yi et al. (2006)YI, Z.; ZHANG, M.; LING, B.; XU, D.; YE, J. Inhibitory effects of Lantana camara and its contained phenolic compounds in Eichhornia crassipes growth. Journal of Applied Ecology, v. 17, n. 9, p. 1637-1640, 2006. causes necrosis and inhibition of root growth in seedlings. Atrophied and necrotic roots were the main anomalies found in seeds exposed to these phytochemicals, although the phytotoxic damages of the extract to the seed metabolism were not sufficient to promote the death of the seedlings.

DNA synthesis, mitotic divisions and mobilization of reserve substances occur after the embryo growth begins, in the phase III of germination (Cardoso 2004CARDOSO, V. J. M. Germinação. In: KERBAUY, G. B. (ed.). Fisiologia vegetal. 2. ed. Rio de Janeiro: Guanabara Koogan, 2004. p. 386-407., Bewley et al. 2013BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. Germination. In: BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. (ed.). Seeds: physiology of development, germination and dormancy. 3. ed. New York: Springer, 2013. p. 133-182.). The results indicate that the phytochemicals of L. camara present in the extract interfere in these metabolic processes.

The aqueous extract of L. camara caused a reduction in the germination speed index at all tested concentrations (Figure 2A). The germination speed index values were reduced from 13.8 % ± 0.3 to 11.7 % ± 0.8, 10.5 % ± 0.5, 9.17 % ± 0.3 and 8.4 % ± 0.2, respectively, at the concentrations of 2.5 %, 5 %, 7.5 % and 10 %. The delay in the radicle emission may be explained by the interference in the growth of the allelochemicals present in the extract, such as reactivation of mitochondrial Krebs cycle enzymes and oxidative phosphorylation, as well as protein synthesis from substrates (enzymes, mRNA, etc.), that occur during the germination phases I and II (Cardoso 2004CARDOSO, V. J. M. Germinação. In: KERBAUY, G. B. (ed.). Fisiologia vegetal. 2. ed. Rio de Janeiro: Guanabara Koogan, 2004. p. 386-407., Bewley et al. 2013BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. Germination. In: BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. (ed.). Seeds: physiology of development, germination and dormancy. 3. ed. New York: Springer, 2013. p. 133-182.).

Figure 2
Regressions for the germination speed index (A; %) and electrical conductivity (B; μS cm^-1 g^-1) of Avena sativa seeds, as a function of Lantana camara extract at different concentrations (%; vv^-1). The bars for observed points are the mean standard deviations.

Allelochemicals may rapidly depolarize the cell membrane, increasing the permeability and inducing lipid peroxidation (Yu et al. 2003YU, J.; YE, S.; ZHANG, M.; HU, W. Effects of root exudates and aqueous root extracts of cucumber (Cucumis sativus) and allelochemicals, on photosynthesis and antioxidant enzymes in cucumber. Biochemical Systematics and Ecology, v. 31, n. 2, p. 129-139, 2003.). Previous reports have shown that the increase of electrolyte flow may be one of the consequences of membrane integrity damage (Poonpaiboonpipat et al. 2013POONPAIBOONPIPAT, T.; PANGNAKORN, U.; SUVUNNAMEK, U.; TEERARAK, M.; CHAROENYING, P.; LAOSINWATTANA, C. Phytotoxic effects of essential oil from Cymbopogon citratus and its physiological mechanisms on barnyardgrass (Echinochloa crus-galli). Industrial Crops and Products, v. 41, n. 2, p. 403-407, 2013.). A significant seed solute leakage was observed when exposed to the extract. The solute leakage increased with the increase of extract concentration (Figure 2B); hence, it may be stated that there is damage to the repair system of cell membranes during seed imbibition, caused by the allelochemicals present in the extract. Aumonde et al. (2013)AUMONDE, T.; MARTINAZZO, E.; PEDÓ, T.; BORELLA, J.; AMARANTE, L.; VILLELA, F. A.; MORAES, D. M. Respostas fisiológicas de sementes e plântulas de alface submetidas ao extrato de Philodendron bipinnatifidum. Semina: Ciências Agrárias, v. 34, n. 6, p. 3181-3192, 2013. also reported a higher release of lettuce seed electrolytes with an increase in the concentration of the aqueous extract of Philodendron bipinnatifidum.

The exposure of the aqueous extract of L. camara during seed germination at the phases I and II did not affect the epicotyl and root development of the A. sativa seedlings. The seeds submitted to the extract during the phase III of germination had their growth negatively affected. The extracts reduced the epicotyl growth by 57 %, 66 %, 84 % and 90 % (Figure 3A) and root growth by 28 %, 43 %, 57 % and 62 % (Figure 3B), respectively, at concentrations of 2.5 %, 5 %, 7.5 % and 10 %. The exposure of the seeds to the extract during all phases of seed germination (I, II and III) caused the greatest damage to the epicotyl and root growth, reaching 99 % of inhibition. The reductions reached 57 %, 81 %, 89 % and 99 % for epicotyls (Figure 3C) and 41 %, 58 %, 74 % and 99 % for roots (Figure 3D), respectively, at concentrations of 2.5 %, 5 %, 7.5 % and 10 %.

Figure 3
Regressions for the epicotyl and root growth inhibition at the phase III (A-B) and phases I, II and III (C-D) of germination of Avena sativa seeds, as a function of Lantana camara extract at different concentrations (%; vv^-1). The bars for observed points are the mean standard deviations.

Seedling growth is known to depend on DNA synthesis, mitotic divisions and seed reserve mobilization (Cardoso 2004CARDOSO, V. J. M. Germinação. In: KERBAUY, G. B. (ed.). Fisiologia vegetal. 2. ed. Rio de Janeiro: Guanabara Koogan, 2004. p. 386-407., Bewley et al. 2013BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. Germination. In: BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. (ed.). Seeds: physiology of development, germination and dormancy. 3. ed. New York: Springer, 2013. p. 133-182.). Mitotic divisions can be reduced by the action of allelochemicals (Ladhari et al. 2014LADHARI, A.; OMEZZINE, F.; HAOUALA, R. The impact of Tunisian Capparidaceae species on cytological, physiological and biochemical mechanisms in lettuce. South African Journal of Botany, v. 93, n. 1, p. 222-230, 2014.), compromising the normal plant development. Romagni et al. (2000)ROMAGNI, J. G.; ALLEN, S. N.; DAYAN, F. E. Allelopathic effects of volatile cineoles on two weedy plant species. Journal of Chemical Ecology, v. 26, n. 1, p. 303-313, 2000. reported that the compound 1,8-cineol is present as a mitotic index and root growth reducer. The phytochemical 1,8-cineol is present in L. camara extracts (Singh et al. 2012SINGH, R. K.; TIWARI, B.; SHARMA, D. K.; SINGH, S. P. Comparative study of chemical composition of Lantana camara leaf, flower & fruit essential oil. International Journal of Pharmaceutical and Chemical Sciences, v. 1, n. 1, p. 895-899, 2012.) and may be involved in the phytotoxic action of the aqueous extract of L. camara leaves in A. sativa seedlings. Kenany & Darier (2013)KENANY, E.; DARIER, S. Suppression effects of Lantana camara L. aqueous extracts on germination efficiency of Phalaris minor Retz. and Sorghum bicolor L. (Moench). Journal of Taibah University for Science, v. 7, n. 2, p. 64-71, 2013. did not identify the compounds involved; however, they reported that the extract of L. camara leaves is able to inhibit the root and stem elongation during the seed germination of Phalaris minor and Sorghum bicolor.

The malondialdehyde (MDA) levels, at 24 and 48 h of germination, were not affected by the exposure to the allelochemicals in the extract concentration of 5 % (vv^-1). After 48 h of germination, the MDA levels remained stable in the control; however, there was an increase in the MDA levels at 72 h of germination of the seeds exposed to phytochemicals (3.0 ± 0.1 µmol g^-1), and they were also high at 120 h of germination (2.7 ± 0.1 µmol g^-1) (Figure 4A). When the seeds were removed from the water and exposed to the extract within 48 h of germination, there was a large increase in the MDA levels at 72 h of germination (3.6 ± 0.1 µmol g^-1), indicating a phytotoxic action. Conversely, the seeds removed from the extract within 48 h of germination had reduced MDA levels by 72 h of germination (1.8 ± 0.2 µmol g^-1). The phase III of germination is more sensitive to allelochemicals, as observed by the higher levels of oxidative stress markers. Increases in the MDA levels related to phytochemical stress are also reported in lettuce (Ladhari et al. 2014LADHARI, A.; OMEZZINE, F.; HAOUALA, R. The impact of Tunisian Capparidaceae species on cytological, physiological and biochemical mechanisms in lettuce. South African Journal of Botany, v. 93, n. 1, p. 222-230, 2014.), soybean (Haddadchi & Gerivani 2009HADDADCHI, G. R.; GERIVANI, Z. Effects of phenolic extracts of canola (Brassica napuse L.) on germination and physiological responses of soybean (Glycin max L.) seedlings. International Journal of Plant Production, v. 3, n. 1, p. 63-67, 2009. ), mustard (Oracz et al. 2007ORACZ, K.; BAILLY, C.; GNIAZDOWSKA, A.; CÔME, D.; CORBINEAU, F.; BOGATEK, R. Induction of oxidative stress by sunflower phytotoxins in germinating mustard seeds. Journal of Chemical Ecology, v. 33, n. 2, p. 251-264, 2007. ), maize, pea and radish (Gmerek & Politycka 2011GMEREK, J.; POLITYCKA, B. Response of maize, pea and radish roots to allelochemical stress. Acta Biologica Cracoviensia Series Botanica, v. 53, n. 1, p. 32-37, 2011. ). Gmerek & Politycka (2011) attribute the lipid peroxidation to the phytochemicals ferulic and p-coumaric acids present in L. camara extracts (Yi et al. 2006YI, Z.; ZHANG, M.; LING, B.; XU, D.; YE, J. Inhibitory effects of Lantana camara and its contained phenolic compounds in Eichhornia crassipes growth. Journal of Applied Ecology, v. 17, n. 9, p. 1637-1640, 2006.).

Figure 4
Regressions for malondialdehyde (A; μmol g^-1 of fresh mass) and hydrogen peroxide (B; nmol g^-1) contents, during the germination period (in hours) of Avena sativa seeds, when kept in water (0) or exposed to Lantana camara extract at the concentration of 5 % (vv^-1) (5), and with induction (0_5) or removal (5_0) of the phytotoxic stress. The bars for observed points are the mean standard deviations.

Malondialdehyde (MDA) is one of the final products of polyunsaturated fatty acids peroxidation in the cells. The MDA content is commonly known as a marker of oxidative stress (Gawel et al. 2004GAWEL, S.; WARDAS, M.; NIEDWOROK, E.; WARDAS, P. Malondialdehyde (MDA) as a lipid peroxidation marker.Wiadomości Lekarskie, v. 57, n. 9-10, p. 453‐455, 2004.). Kurek et al. (2019)KUREK, K.; PLITTA-MICHALAK, B.; RATAJCZAK, E. Reactive oxygen species as potential drivers of the seed aging process. Plants, v. 8, n. 6, p. 174-186, 2019. reported that the genomic integrity considerably affects the seed viability and vigor. Quinones and phenols (groups of allelochemical compounds) are thought to have a toxic effect, because of their ability to form semiquinone radicals that donate electrons to molecular oxygen, forming reactive oxygen species (Hammond-Kosak & Jones 1996).

The H₂O₂ levels increased throughout the period of seed germination; however, there were no differences between the control and the seeds exposed to the extract (Figure 4B). Contrary to our results, allelopathic metabolites increase the H₂O₂ levels in some plant species, such as Sinapis alba (Oracz et al. 2007ORACZ, K.; BAILLY, C.; GNIAZDOWSKA, A.; CÔME, D.; CORBINEAU, F.; BOGATEK, R. Induction of oxidative stress by sunflower phytotoxins in germinating mustard seeds. Journal of Chemical Ecology, v. 33, n. 2, p. 251-264, 2007. ) and Chlorella vulgaris (Qian et al. 2009QIAN, H.; XU, X.; CHEN, W.; JIANG, H.; JIN, Y.; LIU, W.; FU, Z. Allelochemical stress causes oxidative damage and inhibition of photosynthesis in Chlorella vulgaris. Chemosphere, v. 75, n. 3, p. 368-375, 2009. ). The non-increase of H₂O₂ levels may be related to an efficient antioxidant defense system of A. sativa.

Lower levels of catalase activity, between 48 and 120 h of germination, were observed in the seeds exposed to the extract (5 %; vv^-1), when compared to the control (0 %; vv^-1) (Figure 5A). The reduction in the levels of catalase enzyme in the seeds exposed to the extract is possibly related to the action of the enzyme in neutralizing reactive oxygen species, accumulated by the phytotoxic effect of the extract.

Figure 5
Regressions for the enzymatic activities (μmol min^-1 mg prot^-1) of catalase (A) and ascorbate peroxidase (B), during the germination period (in hours) of Avena sativa seeds, when kept in water (0) or exposed to Lantana camara extract at the concentration of 5 % (vv^-1) (5), and with induction (0_5) or removal (5_0) of the phytotoxic stress. The bars for observed points are the mean standard deviations.

When the seeds were removed from the water (0 %; vv^-1) and exposed to the phytotoxic extract at the concentration of 5 % (vv^-1) (treatment denoted as “0_5”), a high increase in the catalase activity was observed, with a subsequent rapid reduction (Figure 5A). This indicates a metabolic response of reactive oxygen species for neutralization. In seeds removed from the phytotoxic stress (extract at the concentration of 5 %) to water, here denoted as “5_0”, an increase in the catalase activity was also observed, although less than for the treatment “0_5”, signaling, in this case, the interruption of the phytotoxic action.

Oracz et al. (2007)ORACZ, K.; BAILLY, C.; GNIAZDOWSKA, A.; CÔME, D.; CORBINEAU, F.; BOGATEK, R. Induction of oxidative stress by sunflower phytotoxins in germinating mustard seeds. Journal of Chemical Ecology, v. 33, n. 2, p. 251-264, 2007. reported increases in the catalase activity in Sinapis alba L. seeds subjected to Helianthus annuus L. extract up to eight days of germination, while Pandey et al. (2005)PANDEY, D.; MISHRA, N.; SINGH, P. Relative phytotoxicity of hydroquinone on rice (Oryza sativa L.) and associated aquatic weed green musk chara (Chara zeylanica Willd.). Pesticide Biochemistry and Physiology, v. 83, n. 2-3, p. 82-96, 2005. in Chara zeylanica and Lin et al. (2000)LIN, W. X.; KIM, K. U.; SHIN, D. H. Rice allelopathic potential and its modes of action on barnyardgrass (Echinochloa crus-galli). Allelopathy Journal, v. 7, n. 2, p. 215-224, 2000. in Echinochloa crus-galli found a reduction in the catalase activity in plants subjected to allelopathic extract. Such differences may be explained by plant-specific mechanisms to scavenge the production of reactive oxygen species.

The activity of ascorbate peroxidase in seeds under normal germination conditions (0 %; vv^-1) remains stable during the phases I and II (up to 48 h), gradually increasing during the seedling growth and development (Figure 5B). However, in seeds exposed to allelochemicals (5 %; vv^-1), the levels of ascorbate peroxidase increase rapidly during the germination phases I and II (up to 48 h) and decrease rapidly during the seedling growth and development phase (after 48 h).

The increase and reduction in the levels of the ascorbate peroxidase enzyme, in seeds exposed to the extract, are possibly related to the metabolic response of production and action of the enzyme to neutralize the reactive oxygen species, accumulated by the phytotoxic effect of the extract. The treatments “0_5” and “5_0” did not present significant changes in the ascorbate peroxidase activity.

The results corroborate those by Pandey et al. (2005)PANDEY, D.; MISHRA, N.; SINGH, P. Relative phytotoxicity of hydroquinone on rice (Oryza sativa L.) and associated aquatic weed green musk chara (Chara zeylanica Willd.). Pesticide Biochemistry and Physiology, v. 83, n. 2-3, p. 82-96, 2005., who reported a reduced ascorbate peroxidase activity in C. zeylanica plants. Muscolo et al. (2001)MUSCOLO, A.; PANUCCIO, M. R.; SIDARI, M. The effect of phenols on respiratory enzymes in seed germination: respiratory enzyme activities during germination of Pinus laricio seeds treated with phenols extracted from different forest soils. Plant Growth Regulation, v. 35, n. 1, p. 31-35, 2001. reported that phenolic compounds such as vanillic, p-coumaric and p-hydroxybenzoic acids are able to inhibit the enzymatic activity in seedlings. These substances are present in leaves of L. camara (Yi et al. 2006YI, Z.; ZHANG, M.; LING, B.; XU, D.; YE, J. Inhibitory effects of Lantana camara and its contained phenolic compounds in Eichhornia crassipes growth. Journal of Applied Ecology, v. 17, n. 9, p. 1637-1640, 2006., Mishra 2015MISHRA, A. Allelopathic properties of Lantana camara. International Research Journal of Basic and Clinical Studies, v. 3, n. 1, p. 13-28, 2015. ).

It was observed that, during the phases I and II of germination (up to 48 h), all treatments showed a rapid increase in the proline levels (Figure 6A). During the seedling growth and development (phase III), there was a reduction in the level of proline in the control seedlings (without stress). However, it is observed that the proline level remained high in the seedlings subjected to phytochemical stress. Higher levels of proline, during the phase III of germination, were also observed in the treatments that suffered stress, either only during the phase III (treatment “0_5”) or just before it (treatment “5_0”) (Figure 6A).

Figure 6
Regression for the contents of proline (A; μmol g^-1 of fresh mass) and total phenolic compounds [B; mg GAE (gallic acid equivalent] g^-1 of fresh mass), during the germination period (in hours) of Avena sativa seeds, when kept in water (0) or exposed to Lantana camara extract at the concentration of 5 % (vv^-1) (5), and with induction (0_5) or removal (5_0) of the phytotoxic stress. The bars for observed points are the mean standard deviations.

According to Singh & Rao (2003)SINGH, D.; RAO, Y. B. Allelopathic evaluation of Andrograhis paniculata aqueous leachates on rice (Oryza sativa). Allelopathy Journal, v. 11, n. 1, p. 71-76, 2003., proline protects proteins from denaturing, what may explain the elevation and maintenance of high levels in stressed seedlings, as an attempt to defend seedlings against allelochemical damage. An increase in the proline content was also recorded in Triticum turgidum and Pisum sativum, as a response to phytochemical coumarin (Abenavoli et al. 2006ABENAVOLI, M. R.; CACCO, G.; SORGONÀ, A.; MARABOTTINI, R.; PAOLACCI, A. R.; CIAFFI, M.; BADIANI, M. The inhibitory effects of coumarin on the germination of durum wheat (Triticum turgidum ssp. durum, cv. Simeto) seeds. Journal of Chemical Ecology, v. 32, n. 2, p. 489-506, 2006. ); Tagetes erecta under treatment with Jatropha curcas extract (Wang et al. 2009WANG, J. C.; WU, Y.; WANG, Q.; PENG, Y. L.; PAN, K. W.; LUO, P.; WU, N. Allelopathic effects of Jatropha curcas on marigold (Tagetes erecta L.). Allelopathy Journal, v. 24, n. 1, p. 123-130, 2009.); and Triticum aestivum leaves with aqueous extract of Zea mays leaves (Ibrahim et al. 2013IBRAHIM, M.; AHMAD, N.; SHINWARI, Z. K.; BANO, A.; ULLAH, F. Allelopathic assessment of genetically modified and non-modified maize (Zea mays L.) on physiology of wheat (Triticum aestivum L.). Pakistan Journal of Botany, v. 45, n. 13, p. 235-240, 2013.). After that, Ladhari et al. (2014LADHARI, A.; OMEZZINE, F.; HAOUALA, R. The impact of Tunisian Capparidaceae species on cytological, physiological and biochemical mechanisms in lettuce. South African Journal of Botany, v. 93, n. 1, p. 222-230, 2014.) also reported an accumulation of proline in lettuce leaves, in response to the methanolic extract of Cleome arabica; however, this accumulation was reduced in the roots.

The levels of total phenolic compounds were reduced throughout the germination of seeds in all treatments; however, the levels remained higher than for the control in the treatments exposed to allelochemicals (Figure 6B). Djanaguiraman et al. (2005)DJANAGUIRAMAN, M.; PANDIYAN, M.; DEVI, D. D. Physiological responses of Eucalyptus globulus leaf leachate on seedling physiology of rice, sorghum and blackgram. International Journal of Agricultural and Biological Engineering, v. 7, n. 1, p. 35-38, 2005. reported that allelochemicals increase the phenolic content in Sorghum bicolor and Phaseoulus vulgaris. Ladhari et al. (2014)LADHARI, A.; OMEZZINE, F.; HAOUALA, R. The impact of Tunisian Capparidaceae species on cytological, physiological and biochemical mechanisms in lettuce. South African Journal of Botany, v. 93, n. 1, p. 222-230, 2014. stated that allelochemicals increase the phenolic content in lettuce roots, but reduce it in lettuce leaves; while Pandey et al. (2005)PANDEY, D.; MISHRA, N.; SINGH, P. Relative phytotoxicity of hydroquinone on rice (Oryza sativa L.) and associated aquatic weed green musk chara (Chara zeylanica Willd.). Pesticide Biochemistry and Physiology, v. 83, n. 2-3, p. 82-96, 2005. reported a reduction in the phenolic content of C. zeylanica exposed to allelochemicals.

CONCLUSION

Concentrations of the aqueous extract of Lantana camara leaves above 2.5 % (vv^-1) impair the physiological development of Avena sativa seeds during germination. The extract affects the phases I and II of germination, damaging cellular membranes and delaying the radicle emission, and, at the phase III, it causes abnormalities in the seedling development. In addition, this phytotoxic effect triggers the enzymatic and non-enzymatic antioxidant metabolism of A. sativa seeds during germination. Hence, this study corroborates the potential of L. camara allelochemicals for the development of natural herbicides.

ACKNOWLEDGMENTS

The first author (D. M. Gindri) thanks the Companhia Integrada de Desenvolvimento Agrícola de Santa Catarina (CIDASC), for contributing to its Ph.D. in Crop Production, as well as the Universidade do Estado de Santa Catarina (UDESC), for providing research facilities; C. M. M. Coelho thanks the CNPq/Capes, for the research fellowships; and V. G. Uarrota thanks the FONDECYT-CONICYT (Project number 3190055) and the Vicerrectoria de Investigacion y Estudios Avanzados of the Pontificia Universidade Católica de Valparaiso, for research facilities.

REFERENCES

ABENAVOLI, M. R.; CACCO, G.; SORGONÀ, A.; MARABOTTINI, R.; PAOLACCI, A. R.; CIAFFI, M.; BADIANI, M. The inhibitory effects of coumarin on the germination of durum wheat (Triticum turgidum ssp. durum, cv. Simeto) seeds. Journal of Chemical Ecology, v. 32, n. 2, p. 489-506, 2006.
ABU-ROMMAN, S.; SHATNAWI, M.; SHIBLI, R. Allelopathic effects of spurge (Euphorbia hierosolymitana) on wheat (Triticum durum). American Eurasian Journal of Agricultural & Environmental Sciences, v. 7, n. 3, p. 298-302, 2010.
ALEXIEVA, V.; SERGIEV, I.; MAPELLI, S.; KARANOV, E. The effect of drought and ultraviolet radiation on growth and stress markers in pea and wheat. Plant Cell Environment, v. 24, n. 12, p. 1337-1344, 2001.
AUMONDE, T.; MARTINAZZO, E.; PEDÓ, T.; BORELLA, J.; AMARANTE, L.; VILLELA, F. A.; MORAES, D. M. Respostas fisiológicas de sementes e plântulas de alface submetidas ao extrato de Philodendron bipinnatifidum Semina: Ciências Agrárias, v. 34, n. 6, p. 3181-3192, 2013.
AZEVEDO, R. A.; ALAS, R. M.; SMITH, R. J. Response of antioxidant enzymes to transfer from elevated carbon dioxide to air and ozone fumigation, in the leaves and roots of wild-type and a catalase-deficient mutant of barley. Physiologia Plantarum, v. 104, n. 2, p. 280-292, 1998.
BATES, L. S.; WALDREN, R. P.; TEARE, I. D. Rapid determination of free proline for water stress studies. Plant and Soil, v. 39, n. 1, p. 205-207, 1973.
BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. Germination. In: BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. (ed.). Seeds: physiology of development, germination and dormancy. 3. ed. New York: Springer, 2013. p. 133-182.
BOGATEK, R.; GNIAZDOWAKA, A. ROS and phytohormons in plant-plant allelopathic interaction. Plant Signaling & Behavior, v. 2, n. 4, p. 317-318, 2007.
BRADFORD, M. M. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Analytical Biochemistry, v. 72, n. 1-2, p. 248-254, 1976.
CARDOSO, V. J. M. Germinação. In: KERBAUY, G. B. (ed.). Fisiologia vegetal 2. ed. Rio de Janeiro: Guanabara Koogan, 2004. p. 386-407.
CHENGXU, W.; MINGXING, Z.; XUHUI, C.; BO, Q. Review on allelopathy of exotic invasive plants. Procedia Engineering, v. 18, n. 1, p. 240-246, 2011.
DJANAGUIRAMAN, M.; PANDIYAN, M.; DEVI, D. D. Physiological responses of Eucalyptus globulus leaf leachate on seedling physiology of rice, sorghum and blackgram. International Journal of Agricultural and Biological Engineering, v. 7, n. 1, p. 35-38, 2005.
FOLIN, O.; CIOCALTEU, V. On tyrosine and tryptophane determinations in proteins. Journal of Biological Chemistry, v. 73, n. 2, p. 627-650, 1927.
GAWEL, S.; WARDAS, M.; NIEDWOROK, E.; WARDAS, P. Malondialdehyde (MDA) as a lipid peroxidation marker.Wiadomości Lekarskie, v. 57, n. 9-10, p. 453‐455, 2004.
GINDRI, D. M.; COELHO, C. M. M.; UARROTA, V. G.; REBELO, A. M. Herbicidal bioactivity of natural compounds from Lantana camara on the germination and seedling growth of Bidens pilosa Pesquisa Agropecuária Tropical, v. 50, e57746, 2020.
GMEREK, J.; POLITYCKA, B. Response of maize, pea and radish roots to allelochemical stress. Acta Biologica Cracoviensia Series Botanica, v. 53, n. 1, p. 32-37, 2011.
HADDADCHI, G. R.; GERIVANI, Z. Effects of phenolic extracts of canola (Brassica napuse L.) on germination and physiological responses of soybean (Glycin max L.) seedlings. International Journal of Plant Production, v. 3, n. 1, p. 63-67, 2009.
HAMMOND-KOSACK, K. E.; JONES, J. D. G. Resistance gene-dependent plant defense responses. The Plant Cell, v. 10, n. 10, p. 1773-1791, 1996.
HEATH, R. L.; PACKER, L. Photoperoxidation in isolated chloroplasts: I. Kinetics and stoichiometry of fatty acid peroxidation. Archives in Biochemistry and Biophysics, v. 125, n. 1, p. 189-198, 1968.
HUSSAIN, M. I.; REIGOSA, M. J. Allelochemical stress inhibits growth, leaf water relations, PSII photochemistry, non-photochemical fluorescence quenching, and heat energy dissipation in three C3 perennial species. Journal of Experimental Botany, v. 62, n. 13, p. 4533-4545, 2011.
IBRAHIM, M.; AHMAD, N.; SHINWARI, Z. K.; BANO, A.; ULLAH, F. Allelopathic assessment of genetically modified and non-modified maize (Zea mays L.) on physiology of wheat (Triticum aestivum L.). Pakistan Journal of Botany, v. 45, n. 13, p. 235-240, 2013.
INTERNATIONAL ALLELOPATHY SOCIETY (IAS). World congress on allelopathy: a science for the future: book of abstracts. Cadiz: Universidad de Cadiz; International Allelopathy Society, 1996.
KEGGE, W.; PIERIK, R. Biogenic volatile organic compounds and plant competition. Trends in Plant Science, v. 15, n. 3, p. 126-132, 2010.
KENANY, E.; DARIER, S. Suppression effects of Lantana camara L. aqueous extracts on germination efficiency of Phalaris minor Retz. and Sorghum bicolor L. (Moench). Journal of Taibah University for Science, v. 7, n. 2, p. 64-71, 2013.
KUPIDLOWSKA, E.; DOBRZYNSKA, K.; PARYS, E.; ZOBEL, A. M. Effect of coumarin and xanthotoxin on mitochondrial structure, oxygen uptake, and succinate dehydrogenase activity in onion root cells. Journal of Chemical Ecology, v. 20, n. 10, p. 2471-2480, 1994.
KUREK, K.; PLITTA-MICHALAK, B.; RATAJCZAK, E. Reactive oxygen species as potential drivers of the seed aging process. Plants, v. 8, n. 6, p. 174-186, 2019.
LADHARI, A.; OMEZZINE, F.; HAOUALA, R. The impact of Tunisian Capparidaceae species on cytological, physiological and biochemical mechanisms in lettuce. South African Journal of Botany, v. 93, n. 1, p. 222-230, 2014.
LATIF, S.; CHIAPUSIO, G.; WESTON, L. A. Allelopathy and the role of allelochemicals in plant defence. In: BECARD, G. (ed.). Advances in botanical research Wagga Wagga: Academic Press, 2017. p. 19-54.
LIN, W. X.; KIM, K. U.; SHIN, D. H. Rice allelopathic potential and its modes of action on barnyardgrass (Echinochloa crus-galli). Allelopathy Journal, v. 7, n. 2, p. 215-224, 2000.
MISHRA, A. Allelopathic properties of Lantana camara International Research Journal of Basic and Clinical Studies, v. 3, n. 1, p. 13-28, 2015.
MITTLER, R. ROS are good. Trends in Plant Science, v. 22, n. 1, p. 11-19, 2017.
MUSCOLO, A.; PANUCCIO, M. R.; SIDARI, M. The effect of phenols on respiratory enzymes in seed germination: respiratory enzyme activities during germination of Pinus laricio seeds treated with phenols extracted from different forest soils. Plant Growth Regulation, v. 35, n. 1, p. 31-35, 2001.
NAKAGAWA, J. Testes de vigor baseados no desempenho de plântulas. In: KRZYZANOWSKI, F. C.; VIEIRA, R. D.; FRANÇA NETO, J. B. (ed.). Vigor de sementes: conceitos e testes. 2. ed. Londrina: Abrates, 1999. p. 1-24.
NAKANO, Y.; ASADA, K. Hydrogen peroxide is scavenged by ascorbate-specific peroxidase in spinach chloroplasts. Plant Cell Physiology, v. 22, n. 5, p. 867-880, 1981.
ORACZ, K.; BAILLY, C.; GNIAZDOWSKA, A.; CÔME, D.; CORBINEAU, F.; BOGATEK, R. Induction of oxidative stress by sunflower phytotoxins in germinating mustard seeds. Journal of Chemical Ecology, v. 33, n. 2, p. 251-264, 2007.
PANDEY, D.; MISHRA, N.; SINGH, P. Relative phytotoxicity of hydroquinone on rice (Oryza sativa L.) and associated aquatic weed green musk chara (Chara zeylanica Willd.). Pesticide Biochemistry and Physiology, v. 83, n. 2-3, p. 82-96, 2005.
POONPAIBOONPIPAT, T.; PANGNAKORN, U.; SUVUNNAMEK, U.; TEERARAK, M.; CHAROENYING, P.; LAOSINWATTANA, C. Phytotoxic effects of essential oil from Cymbopogon citratus and its physiological mechanisms on barnyardgrass (Echinochloa crus-galli). Industrial Crops and Products, v. 41, n. 2, p. 403-407, 2013.
QIAN, H.; XU, X.; CHEN, W.; JIANG, H.; JIN, Y.; LIU, W.; FU, Z. Allelochemical stress causes oxidative damage and inhibition of photosynthesis in Chlorella vulgaris Chemosphere, v. 75, n. 3, p. 368-375, 2009.
R CORE TEAM. R: a language and environment for statistical computing. Vienna: R Foundation for Statistical Computing, 2019.
ROMAGNI, J. G.; ALLEN, S. N.; DAYAN, F. E. Allelopathic effects of volatile cineoles on two weedy plant species. Journal of Chemical Ecology, v. 26, n. 1, p. 303-313, 2000.
SINGH, D.; RAO, Y. B. Allelopathic evaluation of Andrograhis paniculata aqueous leachates on rice (Oryza sativa). Allelopathy Journal, v. 11, n. 1, p. 71-76, 2003.
SINGH, R. K.; TIWARI, B.; SHARMA, D. K.; SINGH, S. P. Comparative study of chemical composition of Lantana camara leaf, flower & fruit essential oil. International Journal of Pharmaceutical and Chemical Sciences, v. 1, n. 1, p. 895-899, 2012.
SOUZA-FILHO, A.; GUILHON, G.; SANTOS, L. Metodologias empregadas em estudos de avaliação da atividade alelopática em condições de laboratório: revisão crítica. Planta Daninha, v. 28, n. 3, p. 689-697, 2010.
TOIVONEN, P. M. A.; HODGES, D. M. Abiotic stress in harvested fruits and vegetables. In: SHANKER, A. (ed.). Abiotic stress in plants: mechanisms and adaptations. Croatia: InTech, 2011. p. 39-58.
VIEIRA, R. D.; CARVALHO, N. M. Testes de vigor em sementes Jaboticabal: Funep, 1994.
WANG, J. C.; WU, Y.; WANG, Q.; PENG, Y. L.; PAN, K. W.; LUO, P.; WU, N. Allelopathic effects of Jatropha curcas on marigold (Tagetes erecta L.). Allelopathy Journal, v. 24, n. 1, p. 123-130, 2009.
YI, Z.; ZHANG, M.; LING, B.; XU, D.; YE, J. Inhibitory effects of Lantana camara and its contained phenolic compounds in Eichhornia crassipes growth. Journal of Applied Ecology, v. 17, n. 9, p. 1637-1640, 2006.
YU, J.; YE, S.; ZHANG, M.; HU, W. Effects of root exudates and aqueous root extracts of cucumber (Cucumis sativus) and allelochemicals, on photosynthesis and antioxidant enzymes in cucumber. Biochemical Systematics and Ecology, v. 31, n. 2, p. 129-139, 2003.

Publication Dates

Publication in this collection
24 Aug 2020
Date of issue
2020

History

Received
16 Mar 2020
Accepted
29 May 2020
Published
27 July 2020

This 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 work is properly cited

[1] ABENAVOLI, M. R.; CACCO, G.; SORGONÀ, A.; MARABOTTINI, R.; PAOLACCI, A. R.; CIAFFI, M.; BADIANI, M. The inhibitory effects of coumarin on the germination of durum wheat (Triticum turgidum ssp. durum, cv. Simeto) seeds. Journal of Chemical Ecology, v. 32, n. 2, p. 489-506, 2006.

[2] ABU-ROMMAN, S.; SHATNAWI, M.; SHIBLI, R. Allelopathic effects of spurge (Euphorbia hierosolymitana) on wheat (Triticum durum). American Eurasian Journal of Agricultural & Environmental Sciences, v. 7, n. 3, p. 298-302, 2010.

[3] ALEXIEVA, V.; SERGIEV, I.; MAPELLI, S.; KARANOV, E. The effect of drought and ultraviolet radiation on growth and stress markers in pea and wheat. Plant Cell Environment, v. 24, n. 12, p. 1337-1344, 2001.

[4] AUMONDE, T.; MARTINAZZO, E.; PEDÓ, T.; BORELLA, J.; AMARANTE, L.; VILLELA, F. A.; MORAES, D. M. Respostas fisiológicas de sementes e plântulas de alface submetidas ao extrato de Philodendron bipinnatifidum Semina: Ciências Agrárias, v. 34, n. 6, p. 3181-3192, 2013.

[5] AZEVEDO, R. A.; ALAS, R. M.; SMITH, R. J. Response of antioxidant enzymes to transfer from elevated carbon dioxide to air and ozone fumigation, in the leaves and roots of wild-type and a catalase-deficient mutant of barley. Physiologia Plantarum, v. 104, n. 2, p. 280-292, 1998.

[6] BATES, L. S.; WALDREN, R. P.; TEARE, I. D. Rapid determination of free proline for water stress studies. Plant and Soil, v. 39, n. 1, p. 205-207, 1973.

[7] BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. Germination. In: BEWLEY, J.; BRADFORD, K.; HILHORST, H.; NONOGAKI, H. (ed.). Seeds: physiology of development, germination and dormancy. 3. ed. New York: Springer, 2013. p. 133-182.

[8] BOGATEK, R.; GNIAZDOWAKA, A. ROS and phytohormons in plant-plant allelopathic interaction. Plant Signaling & Behavior, v. 2, n. 4, p. 317-318, 2007.

[9] BRADFORD, M. M. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Analytical Biochemistry, v. 72, n. 1-2, p. 248-254, 1976.

[10] CARDOSO, V. J. M. Germinação. In: KERBAUY, G. B. (ed.). Fisiologia vegetal 2. ed. Rio de Janeiro: Guanabara Koogan, 2004. p. 386-407.

[11] CHENGXU, W.; MINGXING, Z.; XUHUI, C.; BO, Q. Review on allelopathy of exotic invasive plants. Procedia Engineering, v. 18, n. 1, p. 240-246, 2011.

[12] DJANAGUIRAMAN, M.; PANDIYAN, M.; DEVI, D. D. Physiological responses of Eucalyptus globulus leaf leachate on seedling physiology of rice, sorghum and blackgram. International Journal of Agricultural and Biological Engineering, v. 7, n. 1, p. 35-38, 2005.

[13] FOLIN, O.; CIOCALTEU, V. On tyrosine and tryptophane determinations in proteins. Journal of Biological Chemistry, v. 73, n. 2, p. 627-650, 1927.

[14] GAWEL, S.; WARDAS, M.; NIEDWOROK, E.; WARDAS, P. Malondialdehyde (MDA) as a lipid peroxidation marker.Wiadomości Lekarskie, v. 57, n. 9-10, p. 453‐455, 2004.

[15] GINDRI, D. M.; COELHO, C. M. M.; UARROTA, V. G.; REBELO, A. M. Herbicidal bioactivity of natural compounds from Lantana camara on the germination and seedling growth of Bidens pilosa Pesquisa Agropecuária Tropical, v. 50, e57746, 2020.

[16] GMEREK, J.; POLITYCKA, B. Response of maize, pea and radish roots to allelochemical stress. Acta Biologica Cracoviensia Series Botanica, v. 53, n. 1, p. 32-37, 2011.

[17] HADDADCHI, G. R.; GERIVANI, Z. Effects of phenolic extracts of canola (Brassica napuse L.) on germination and physiological responses of soybean (Glycin max L.) seedlings. International Journal of Plant Production, v. 3, n. 1, p. 63-67, 2009.

[18] HAMMOND-KOSACK, K. E.; JONES, J. D. G. Resistance gene-dependent plant defense responses. The Plant Cell, v. 10, n. 10, p. 1773-1791, 1996.

[19] HEATH, R. L.; PACKER, L. Photoperoxidation in isolated chloroplasts: I. Kinetics and stoichiometry of fatty acid peroxidation. Archives in Biochemistry and Biophysics, v. 125, n. 1, p. 189-198, 1968.

[20] HUSSAIN, M. I.; REIGOSA, M. J. Allelochemical stress inhibits growth, leaf water relations, PSII photochemistry, non-photochemical fluorescence quenching, and heat energy dissipation in three C3 perennial species. Journal of Experimental Botany, v. 62, n. 13, p. 4533-4545, 2011.

[21] IBRAHIM, M.; AHMAD, N.; SHINWARI, Z. K.; BANO, A.; ULLAH, F. Allelopathic assessment of genetically modified and non-modified maize (Zea mays L.) on physiology of wheat (Triticum aestivum L.). Pakistan Journal of Botany, v. 45, n. 13, p. 235-240, 2013.

[22] INTERNATIONAL ALLELOPATHY SOCIETY (IAS). World congress on allelopathy: a science for the future: book of abstracts. Cadiz: Universidad de Cadiz; International Allelopathy Society, 1996.

[23] KEGGE, W.; PIERIK, R. Biogenic volatile organic compounds and plant competition. Trends in Plant Science, v. 15, n. 3, p. 126-132, 2010.

[24] KENANY, E.; DARIER, S. Suppression effects of Lantana camara L. aqueous extracts on germination efficiency of Phalaris minor Retz. and Sorghum bicolor L. (Moench). Journal of Taibah University for Science, v. 7, n. 2, p. 64-71, 2013.

[25] KUPIDLOWSKA, E.; DOBRZYNSKA, K.; PARYS, E.; ZOBEL, A. M. Effect of coumarin and xanthotoxin on mitochondrial structure, oxygen uptake, and succinate dehydrogenase activity in onion root cells. Journal of Chemical Ecology, v. 20, n. 10, p. 2471-2480, 1994.

[26] KUREK, K.; PLITTA-MICHALAK, B.; RATAJCZAK, E. Reactive oxygen species as potential drivers of the seed aging process. Plants, v. 8, n. 6, p. 174-186, 2019.

[27] LADHARI, A.; OMEZZINE, F.; HAOUALA, R. The impact of Tunisian Capparidaceae species on cytological, physiological and biochemical mechanisms in lettuce. South African Journal of Botany, v. 93, n. 1, p. 222-230, 2014.

[28] LATIF, S.; CHIAPUSIO, G.; WESTON, L. A. Allelopathy and the role of allelochemicals in plant defence. In: BECARD, G. (ed.). Advances in botanical research Wagga Wagga: Academic Press, 2017. p. 19-54.

[29] LIN, W. X.; KIM, K. U.; SHIN, D. H. Rice allelopathic potential and its modes of action on barnyardgrass (Echinochloa crus-galli). Allelopathy Journal, v. 7, n. 2, p. 215-224, 2000.

[30] MISHRA, A. Allelopathic properties of Lantana camara International Research Journal of Basic and Clinical Studies, v. 3, n. 1, p. 13-28, 2015.

[31] MITTLER, R. ROS are good. Trends in Plant Science, v. 22, n. 1, p. 11-19, 2017.

[32] MUSCOLO, A.; PANUCCIO, M. R.; SIDARI, M. The effect of phenols on respiratory enzymes in seed germination: respiratory enzyme activities during germination of Pinus laricio seeds treated with phenols extracted from different forest soils. Plant Growth Regulation, v. 35, n. 1, p. 31-35, 2001.

[33] NAKAGAWA, J. Testes de vigor baseados no desempenho de plântulas. In: KRZYZANOWSKI, F. C.; VIEIRA, R. D.; FRANÇA NETO, J. B. (ed.). Vigor de sementes: conceitos e testes. 2. ed. Londrina: Abrates, 1999. p. 1-24.

[34] NAKANO, Y.; ASADA, K. Hydrogen peroxide is scavenged by ascorbate-specific peroxidase in spinach chloroplasts. Plant Cell Physiology, v. 22, n. 5, p. 867-880, 1981.

[35] ORACZ, K.; BAILLY, C.; GNIAZDOWSKA, A.; CÔME, D.; CORBINEAU, F.; BOGATEK, R. Induction of oxidative stress by sunflower phytotoxins in germinating mustard seeds. Journal of Chemical Ecology, v. 33, n. 2, p. 251-264, 2007.

[36] PANDEY, D.; MISHRA, N.; SINGH, P. Relative phytotoxicity of hydroquinone on rice (Oryza sativa L.) and associated aquatic weed green musk chara (Chara zeylanica Willd.). Pesticide Biochemistry and Physiology, v. 83, n. 2-3, p. 82-96, 2005.

[37] POONPAIBOONPIPAT, T.; PANGNAKORN, U.; SUVUNNAMEK, U.; TEERARAK, M.; CHAROENYING, P.; LAOSINWATTANA, C. Phytotoxic effects of essential oil from Cymbopogon citratus and its physiological mechanisms on barnyardgrass (Echinochloa crus-galli). Industrial Crops and Products, v. 41, n. 2, p. 403-407, 2013.

[38] QIAN, H.; XU, X.; CHEN, W.; JIANG, H.; JIN, Y.; LIU, W.; FU, Z. Allelochemical stress causes oxidative damage and inhibition of photosynthesis in Chlorella vulgaris Chemosphere, v. 75, n. 3, p. 368-375, 2009.

[39] R CORE TEAM. R: a language and environment for statistical computing. Vienna: R Foundation for Statistical Computing, 2019.

[40] ROMAGNI, J. G.; ALLEN, S. N.; DAYAN, F. E. Allelopathic effects of volatile cineoles on two weedy plant species. Journal of Chemical Ecology, v. 26, n. 1, p. 303-313, 2000.

[41] SINGH, D.; RAO, Y. B. Allelopathic evaluation of Andrograhis paniculata aqueous leachates on rice (Oryza sativa). Allelopathy Journal, v. 11, n. 1, p. 71-76, 2003.

[42] SINGH, R. K.; TIWARI, B.; SHARMA, D. K.; SINGH, S. P. Comparative study of chemical composition of Lantana camara leaf, flower & fruit essential oil. International Journal of Pharmaceutical and Chemical Sciences, v. 1, n. 1, p. 895-899, 2012.

[43] SOUZA-FILHO, A.; GUILHON, G.; SANTOS, L. Metodologias empregadas em estudos de avaliação da atividade alelopática em condições de laboratório: revisão crítica. Planta Daninha, v. 28, n. 3, p. 689-697, 2010.

[44] TOIVONEN, P. M. A.; HODGES, D. M. Abiotic stress in harvested fruits and vegetables. In: SHANKER, A. (ed.). Abiotic stress in plants: mechanisms and adaptations. Croatia: InTech, 2011. p. 39-58.

[45] VIEIRA, R. D.; CARVALHO, N. M. Testes de vigor em sementes Jaboticabal: Funep, 1994.

[46] WANG, J. C.; WU, Y.; WANG, Q.; PENG, Y. L.; PAN, K. W.; LUO, P.; WU, N. Allelopathic effects of Jatropha curcas on marigold (Tagetes erecta L.). Allelopathy Journal, v. 24, n. 1, p. 123-130, 2009.

[47] YI, Z.; ZHANG, M.; LING, B.; XU, D.; YE, J. Inhibitory effects of Lantana camara and its contained phenolic compounds in Eichhornia crassipes growth. Journal of Applied Ecology, v. 17, n. 9, p. 1637-1640, 2006.

[48] YU, J.; YE, S.; ZHANG, M.; HU, W. Effects of root exudates and aqueous root extracts of cucumber (Cucumis sativus) and allelochemicals, on photosynthesis and antioxidant enzymes in cucumber. Biochemical Systematics and Ecology, v. 31, n. 2, p. 129-139, 2003.

Brasil