Changes in hormonal balance as key to reserve degradation after dormancy overcoming in <i>Annona macroprophyllata</i> and <i>Annona purpurea seeds</i>

Ferreira, Gisela; De-la-Cruz-Chacón, Ivan; González-Esquinca, Alma Rosa

doi:10.1590/0100-29452020664

Abstract

Studies on the effect of the applying of phytoregulators to overcome seed dormancy have been carried out in Annonaceae species, thus the endogenous relationship between abscisic acid and gibberellins after the application of phytoregulators needs to be known in these species. Considering the importance of hormonal balance in dormancy mechanisms, the aim of this research was to elucidate how endogenous ABA and GA concentrations change after the application of phytoregulators in seeds and how these changes affect reserve degradation during germination of Annona macroprophyllata and A. purpurea seeds. Seeds were submitted to three conditions: - no soaking, soaking-in-water and soaking-in-GA4+7+benzyladenine. ABA, GA, lipids, proteins, and total soluble sugars were quantified at 0, 2, 5, 10, and 15 days after the beginning of treatments. The application of phytoregulators led change of the hormonal balance inducing increase in endogenous GA and reduction in ABA levels since seed soaking. During imbibition, the degradation of seed reserves (breaks proteins first, and then soluble sugars and finally lipids) was observed and complete germination was obtained after 10 days, with primary root emission. In both species, dormancy can be broken soon after seed dispersal when the balance between GA and ABA is endogenously changed (by exogenous application of phytoregulators), leading to metabolic reserve degradation and germination.

Index terms
abscisic acid; gibberellins; germination; lipids; proteins; soluble sugars; plant growth regulators; phytoregulators

Resumo

Estudos sobre o efeito da aplicação de reguladores vegetais para a superação da dormência de sementes têm sido realizados em espécies de Annonaceae, deste modo a relação endógena entre o ácido abscísico e as giberelinas, após a aplicação de reguladores vegetais, necessita ser mais bem estudada nesta família. Considerando a importância do balanço hormonal nos mecanismos de dormência, o objetivo deste trabalho foi elucidar como as concentrações endógenas de ABA e GA se modificam após a aplicação de reguladores vegetais em sementes durante a superação da dormência e como essas alterações afetam a degradação de reservas durante a germinação de sementes de Annona macroprophyllata e A. purpurea logo após tal superação. As sementes foram submetidas a três condições: - sem imersão; imersão em água, e imersão em GA4+7+benzyladenina. ABA, GA, lipídios, proteínas e açúcares solúveis totais foram quantificados aos 0; 2; 5; 10 e 15 dias após o início dos tratamentos. A aplicação dos reguladores levou à alteração do balanço hormonal, induzindo aumento do GA endógeno e redução dos níveis de ABA desde a embebição das sementes. Durante a embebição, foi observada a degradação de reservas das sementes (primeiro proteínas, depois os açúcares e finalmente os lipídios), e a germinação completa foi obtida após 10 dias do início dos tratamentos, com emissão da raiz primária. Em ambas as espécies, a dormência pode ser quebrada logo após a dispersão das sementes, quando o equilíbrio entre GA e ABA endógeno é alterado (pela aplicação exógena de reguladores vegetais), levando à degradação de reservas e à germinação.

Termos para indexação
ácido abscísico; giberelinas; germinação; lipidios; proteínas; açúcares solúveis; hormônios vegetais; reguladores vegetais

Introduction

The Annonaceae family has approximately 135 genera and 2500 species, with evolutionary, ecological, and pharmaceutical importance, in addition to its application in the food industry (CHATROU et al., 2012 CHATROU, L.W.; PIRIE, M.D.; ERKENS, R.H.J.; COUVREUR, T.L.P.; NEUBIG, K.M.; ABBOTT, J.R.; MOLS, J.B.; MAAS, J.W.; SAUNDERS, R.M.K.; CHASE, M.W. A new subfamilial and tribal classification of the pantropical flowering plant family Annonaceae informed by molecular phylogenetics. Botanical Journal of the Linnean Society, Londres, v.169, p.5-40, 2012. ). Annonaceae seeds have acquired different dormancy mechanisms during evolution - morphological (RIZZINI, 1973 RIZZINI, C.T. Dormancy in seeds of Annona crassiflora Mart. Journal of Experimental Botany, Oxford, v. 24, p.17-123, 1973. ); physiological (SILVA et al., 2007 SILVA, E.A.A. da; MELO, D.L.B.; DAVIDE, A.C.; BODE, N.; ABREU, G.B.; FARIA, J.M.R.; HILHORST, H.W.M. Germination ecophysiology of Annona crassiflora seeds. Annals of Botany, Oxford, v. 99, n.5, p.823–830, 2007. ) and/ or morphophysiological (BRAGA et al., 2010 BRAGA, J.F.; FERREIRA, G.; PINHO, S.Z.; BRAGA, L.F.; SOUSA, M.P. Germination of atemoya (Annona cherimola Mill. x A. squamosa L.) CV. Gefner seeds subjected to treatments with plant growth regulators. International Journal of Science and Nature, Daca, v.1, n.2, p.120-126, 2010. ; COSTA et al., 2011 COSTA, P.N.; BUENO, S.S.C.; FERREIRA, G. Fases da germinação de sementes de Annona emarginata (Schltdl.) H. Rainer em diferentes temperaturas. Revista Brasileria de Fruticultura, Jaboticabal, v.33, n.1, p.253-260, 2011 ). Such mechanisms still need to be studied in several species, including Annona macroprophyllata and A. purpurea. Seed dispersal occurs at the end of the rainy season, with dormancy during the entire drought period (approximately 6 months) to Annona macroprophyllata (GONZALEZ-ESQUINCA et al., 2015 GONZÁLEZ-ESQUINCA, A.R.; DE-LA-CRUZ-CHACÓN, I.; DOMÍNGUEZ-GUTÚ, L.M. Dormancy and germination of Annona macroprophyllata (Annonaceae): the importance of the micropylar plug and seed position in the fruits. Botanical Sciences, Ciudad de México, v. 93, n.3, p.1-7, 2015. ) and more than six months to A. purpurea (GOMÉZ-CASTAÑEDA et al., 2003 GOMÉZ-CASTAÑEDA, J.A.; RAMIREZ, H; BENAVIDES-MENDOZA, A.; ENCINA-RODRIGUEZ, L.I. Germinación y crecimiento de plántula en chincuya (Annona purpurea Moc y Sessé) y su relación con los niveles de giberelinas y ácido abscísico. Revista Chapingo, Chapingo, v.9, n.2,p. 243-253, 2003. ).

Several studies have been conducted to determine the factors involved with seed dormancy, including studies on tegument impermeability and embryo immaturity (FERREIRA et al., 2019 FERREIRA, G.; DE-LA-CRUZ-CHACÓN, I.; BOARO, C.S.F.; BARON, D.; LEMOS, E.E.P.D. Propagation of Annonaceous plants. Revista Brasileira de Fruticultura, Jaboticabal, v. 41, n.1, e-500, 2019. ). Studies on impermeability have demonstrated that seeds of both species (A. macroprophyllata and A. purpurea) present low imbibition rate, but are not impermeable (FERREIRA et al., 2014 FERREIRA, G.; GONZÁLEZ-ESQUINCA, A.R.; DE-LA-CRUZ-CHACÓN, I. Water uptake by Annona diversifolia Saff. and A. purpurea Moc. e Sessé ex Dunal seeds (Annonaceae). Revista Brasileria de Fruticultura, Jaboticabal, v.36, n.1, p.288-295, 2014. Número Especial. ). Gonzalez-Esquinca et al. (2015) found that the tissues of embryos are differentiated at the time of seed dispersal, indicating absense the morphological problem in seed to germination. In another work, Campbell and Popenoe (1968) CAMPBELL, C.W. ; POPENOE, J. Effect of gibberellic acid on seed dormancy of Annona diversifolia Saff. Tropical Region American Society for Horticultural Science, Mount Vermon, v.11, p.33-36, 1968. report the use of GA3 to overcome the dormancy of Annona diversifolia seeds. Similarly with A. macroprophyllata and A. purpurea seeds, Ferreira et al. (2016) FERREIRA, G.; DE-LA-CRUZ-CHACON, I.; GONZALEZ-ESQUINCA, A. R. Overcoming seed dormancy in Annona macroprophyllata and Annona purpurea using plant growth regulators. Revista Brasileira de Fruticultura, Jaboticabal, v. 38, n. 3, e-234, 2016. observed that at the time of dispersion, seeds only germine with the application of plant growth regulators and the use of giberellins asociated with cytokinin (GA4+7 + N-(phenylmethyl)-aminopurine (benzyladenine - BA)) was more effective than giberellin GA3 to break dormancy in both seed species.

The effect of gibberellins and cytokinins to overcome dormancy caused by abscisic acid (ABA) is well known (KOORNEEF et al., 2002 KOORNNEEF, M.; BENTSINK, L.; HILHORST, H. Seed dormancy and germination. Current Opinion Plant Biology, London, v. 5, p. 33-36, 2002. ; GUBLER et al., 2005 GUBLER, F.; MILLAR, A.A.; JACOBSEN, J.V. Dormancy release, ABA and pre-harvest sprouting. Current Opinion in Plant Biology, Saint Louis, v. 8, p.183-187, 2005. ; BEWLEY et al., 2013 BEWLEY, J.D.; BRADFORD, K.J.; HILHORST, H.W.M.; NONOGAKI, H. Seeds: physiology of development, germination and dormancy. 3rd ed. London: Springer, 2013. 392p. ). Since dormancy is overcome, gibberellins promote the biosynthesis of hydrolytic enzymes that act in reserve degradation, releasing energy and substrate for germination (MIRANSARI; SMITH, 2014 MIRANSARI, M.; SMITH, D.L. Plant hormones and seed germination. Environmental and Experimental Botany, Oxford, v.99, p.110-121, 2014. ). Cytokinins act at the various germination stages, inducing reserve degradation by increasing amylolytic and proteolytic activity (BEWLEY et al., 2013 BEWLEY, J.D.; BRADFORD, K.J.; HILHORST, H.W.M.; NONOGAKI, H. Seeds: physiology of development, germination and dormancy. 3rd ed. London: Springer, 2013. 392p. ), also acting on cell division during germination (HEYL et al., 2012 HEYL, A.; RIEFLER, M.; ROMANOV, G.A.; SCHMÜLLING, T. Properties, functions and evolution of cytokinin receptors. European Journal of Cell Biology, Zurich, v.9, n.4, p. 246-256. ).

Although studies on dormancy have been carried out for several Annonaceae species (SILVA et al., 2007 SILVA, E.A.A. da; MELO, D.L.B.; DAVIDE, A.C.; BODE, N.; ABREU, G.B.; FARIA, J.M.R.; HILHORST, H.W.M. Germination ecophysiology of Annona crassiflora seeds. Annals of Botany, Oxford, v. 99, n.5, p.823–830, 2007. ; GONZÁLEZ-ESQUINCA et al., 2015 GONZÁLEZ-ESQUINCA, A.R.; DE-LA-CRUZ-CHACÓN, I.; DOMÍNGUEZ-GUTÚ, L.M. Dormancy and germination of Annona macroprophyllata (Annonaceae): the importance of the micropylar plug and seed position in the fruits. Botanical Sciences, Ciudad de México, v. 93, n.3, p.1-7, 2015. ), studies have demonstrated the effect of the application of plant growth regulators on seed germination (STENZEL, 2003 STENZEL, N.M.C.; MURATA, I.M.; NEVES, C.S.V.J. Superação da dormência em sementes de atemóia e fruta-do-conde. Revista Brasileira de Fruticultura, Jaboticabal, v.25, n.2, p.305-308, 2003. ; OLIVEIRA et al., 2010 OLIVEIRA, M.C.; FERREIRA, G.; GUIMARÃES, V.F.; DIAS, G.B. Germinação de sementes de atemoia (Annona cherimola Mill. x A. squamosa L.) cv ‘Gefner’submetidas a tratamentos com ácido Giberélico (GA3) e ethephon. Revista Brasileria de Fruticultura, Jaboticabal, v.32, n.2, p.544-554, 2010. ; SOKOLOWSKI; CICERO, 2011 SOCOLOWSKI, F.; CICERO, S.M. Use of growth regulators to overcome seed dormancy in Xylopia aromatica (Annonaceae). Seed Science and Technology, Zurich, v.39, p.21-28, 2011. ). The relationship between endogenous abscisic acid (ABA) and gibberellins (GA) after the application of plant growth regulators is well known in other botanical families (CHEN et al., 2010 CHEN, S.Y.; CHIEN, C.T.; BASKIN, J.M.; BASKIN, C.C. Storage behavior and changes in concentrations of abscisic acid and gibberellins during dormancy break and germination in seeds of Phellodendron amurense var. wilsonii (Rutaceae). Tree Physiology, Oxford, v.30, n.2, p.275-284, 2010. ).

Studies on the germination and dormancy aspects of Annonaceae seeds are relatively scarce, especially when the study is about the metabolic processes that occur during germination. It is known that in other species, the balance between ABA and GA is responsible for controlling dormancy and germination, which has not been discussed for Annonaceae.

Considering the importance of hormonal balance in dormancy mechanisms, the present study aimed at elucidating how endogenous ABA and GA concentrations change after the application of plant growth regulators in seeds and how these changes affect reserve degradation during germination of Annona macroprophyllata and A. purpurea seeds.

Materials and methods

Experimental design, treatments and evaluations Annona macroprophyllata Donn.Sm. (≡ Annona diversifolia Saff.) and Annona purpurea Moc. e Sessé ex Dunal fruits were obtained at the municipality of San Lucas, Chiapas, Mexico, from 18 and 12 trees, respectively, from non-commercial orchards. About 90 and 60 fruits of each species were collected and obtained, on average, 50 and 70 seeds per fruit, respectively. Seeds were manually extracted, washed with distilled water and maintained in the shade at 25 °C (+ 2 ºC) during seven days for superficial drying. The water content of seeds (9% to A.macroprophyllata and 16% to A. purpurea) was determined using four replicates of 25 seeds (GOMES et al., 2019 GOMES, R.L.; PASSOS, J.R.S.; GIMENEZ, J.I.; SOUSA, M.C.;DE-PIERI-OLIVEIRA, M.F., MIMI, C.O.; FERREIRA, G. Optimum Sample Size in the gerrmination of Atemoya seeds (Annona× atemoya Mabb.). Journal of Agricultural Science, Cambridge, v.11, n.7, p.239-245, 2019. ) by the method of drying at 105 ºC for 24 hours (BRASIL, 2009 BRASIL. Ministério da Agricultura. Regras para análise de sementes. Brasilia (DF): Departamento de Produção Vegetal, 2009. 398 p. ). To verify seed viability, the tetrazolium test was performed in four replicates of 25 seeds. Seeds were longitudinally cut and immersed in tetrazolium solution (1% concentration) in black germination boxes (10 x 10 x 2 cm) for 2 hours under constant temperature of 30 °C ± 2 °C (GIMENEZ et al., 2014 GIMENEZ, J.I.; FERREIRA, G.; CAVARIANI, C. Tetrazolium test for assessment of seed viability of atemoia (Annona cherimola Mill. x A. squamosa L.). Journal of Seed Science, Londrina, v.36, n.3, p.357-361, 2014. ). Both species had embryos with 100% viability.

The experimental design was completely randomized, with three replicates per plot, in a 3 x 5 (treatments x evaluation times) factorial arrangement.

Treatments consisted of a) seeds without soaking, b) seeds soaked in distilled water for four days (called “seeds in water”), and c) seeds soaked in plant growth regulators (400 mg L-1 of GA4+7 and N-(phenylmethyl)-aminopurine (benzyladenine - BA), PROMALIN® a commercial product with the mixture of the two substances) solution for four days. The use of GA4+7 + BA and its concentration (400 mg L-1) were set based on previous experiments (FERREIRA et al., 2016 FERREIRA, G.; DE-LA-CRUZ-CHACON, I.; GONZALEZ-ESQUINCA, A. R. Overcoming seed dormancy in Annona macroprophyllata and Annona purpurea using plant growth regulators. Revista Brasileira de Fruticultura, Jaboticabal, v. 38, n. 3, e-234, 2016. ).

The phytoregulator solution was prepared by dissolving 22.2 g of the product per liter, Commercial mixture (PROMALIN®) contains 1.8% of each phytoregulator and the concentration of each substance was 400 mg.L-1. Soaking time (four days – 96 hours) was set as a function of time required by phase I of the water acquisition curve (imbibition); soaking solutions were maintained under constant aeration through aquarium pumps (FERREIRA et al., 2014 FERREIRA, G.; GONZÁLEZ-ESQUINCA, A.R.; DE-LA-CRUZ-CHACÓN, I. Water uptake by Annona diversifolia Saff. and A. purpurea Moc. e Sessé ex Dunal seeds (Annonaceae). Revista Brasileria de Fruticultura, Jaboticabal, v.36, n.1, p.288-295, 2014. Número Especial. ).

Seeds received treatments and then were placed in a roll of germination paper moistened with distilled water (2.5 times its dry weight). Then, seeds were maintained in germination chamber at 50-60% relative humidity, 30 °C (±2 °C), and in the absence of light (FERREIRA et al., 2016) FERREIRA, G.; DE-LA-CRUZ-CHACON, I.; GONZALEZ-ESQUINCA, A. R. Overcoming seed dormancy in Annona macroprophyllata and Annona purpurea using plant growth regulators. Revista Brasileira de Fruticultura, Jaboticabal, v. 38, n. 3, e-234, 2016. until collection at each germination stage (evaluation times) for biochemical analyses, when three replicates of each treatment were used for the performance of each biochemical analysis. The application of plant growth regulators in seeds promotes 71% germination on Annona macroprophyllata seeds and 29% on A. purpurea seeds. On the other hand, seeds without treatments do not germinate. These results were reported in Ferreira et al. 2016.

Evaluation times (zero, two, five, ten, and fifteen days after sowing) were determined as a function of germination stages according to previous experiment (FERREIRA et al., 2016 FERREIRA, G.; DE-LA-CRUZ-CHACON, I.; GONZALEZ-ESQUINCA, A. R. Overcoming seed dormancy in Annona macroprophyllata and Annona purpurea using plant growth regulators. Revista Brasileira de Fruticultura, Jaboticabal, v. 38, n. 3, e-234, 2016. ). Time zero corresponded to the initial metabolic stage of seeds (before treatments). Times two and five days corresponded to intermediate stages, with no primary root protrusion. At ten and fifteen days, germinated seeds (that received GA4+7 + BA) presenting 1 mm and 1 cm primary root were collected, respectively. At the same times (ten and fifteen days) ungerminated seeds were collected (without primary root). Thus, seeds treated with GA4+7 + BA and without treatments with no signal of germination were simultaneously collected.

Total soluble sugars, proteins, and lipids were quantified in endosperm samples of each treatment and at each evaluation time (without embryos). Furthermore, endosperms plus embryos were used for ABA and GA quantification.

ABA and GA quantification-The method for ABA and GA extraction and quantification was adapted by Kelen et al. (2004) KELEN, M.; DEMIRALAY, E.Ç.; SEN, S.; ALSANCAK, G.Ö. Separation of abscisic acid, indole-3-acetic acid, gibberellic acid in 99 R (Vitis berlandieri x Vitis rupestris) and rose oil (Rosa damascene Mill.) by reversed phase liquid chromatography. Turkish Journal of Chemistry, Ankara, v. 28, p.603-610, 2004. . Three replicates of five dry seeds (~ 5.5 g) were soaked in 70% methanol and maintained at 4 °C for 12h. The material was submitted to vacuum filtration and rotaevaporation at 45 °C to remove methanol. The aqueous phase was adjusted to pH 8.5 with 0.1 M phosphate buffer and partitioned three times with ethyl acetate (AcOEt). The ethyl acetate phase was removed and the pH of the aqueous phase was adjusted to 2.5 with 1N HCl. The material was again partitioned with EtOAc, the organic portion was filtered over anhydrous sodium sulfate, and AcOEt was evaporated.

ABA and GA were analyzed according to Kellen et al. (2004) KELEN, M.; DEMIRALAY, E.Ç.; SEN, S.; ALSANCAK, G.Ö. Separation of abscisic acid, indole-3-acetic acid, gibberellic acid in 99 R (Vitis berlandieri x Vitis rupestris) and rose oil (Rosa damascene Mill.) by reversed phase liquid chromatography. Turkish Journal of Chemistry, Ankara, v. 28, p.603-610, 2004. , and Bandurska et al. (2017) BANDURSKA, H.; NIEDZIELA, J PIETROWSKA-BOREK, M.; NUC, K.; CHADZINIKOLAU T.; RADZIKOWSKA, D.. Regulation of proline biosynthesis and resistance to drought stress in two barley (Hordeum vulgare L.) genotypes of different origin. Plant Physiology and Biochemistry, Amsterdam, v.118, p.427-437, 2017. , by High-Performance Liquid Chromatography (HPLC, PerkinElmer NCI 900 Series) in reverse phase (Spheri-5 RP-18, 100 mm x 4.6 mm; 5 μm particle diameter). The mobile phase consisted of acetonitrile: water (26:74). The isocratic flow rate was 1 mL min-1, and column temperature was maintained at 30 °C. UV detection was performed at 210 nm. The standard calibration curve of each plant growth regulator was made from stock solutions containing 250, 225, 150, 100, 50, 25, 12, 6; and 3 μM ABA and 275, 250, 200, 150, 100, 50, and 25 μM GA3. Linear regression curves were made for GA (y= 6403x-182769, R2 = 0.98) and ABA (y= 20742x+287104, R2 = 0.99) contents. The Perkin Elmer Turbochrom software was used for data analysis and integration of chromatographic peaks.

Samples were dissolved in ethanol to obtain concentration of 2 mg L-1. Then, 20 μL of such solutions were injected into the HPLC system for analysis. The identification of hormones was confirmed by comparing peaks obtained using HPLC and the UV spectrum of pure standards. GAs were expressed as their total content.

Total soluble sugar quantification-Total soluble sugars were extracted according to Garcia et al. (2006) GARCIA, I.S.; SOUZA, A.; BARBEDO, C.J.; DIETRICH, S.M.C.; FIGUEIREDO-RIBEIRO, R.C.L. Changes in soluble carbohydrates during storage of Caesalpinia echinata LAM. (Brazilwood) seeds, an endangered leguminous tree from the Brazilian Atlantic Forest. Brazilian Journal of Biology, São Carlos, v. 66, p.739-745, 2006. and quantified through the phenolsulfuric acid method (DUBOIS et al., 1956 DUBOIS, M.; GILLES, K.A.; HAMILTON, J.K.; REBERS, P.A.T.; SMITH, F. Colorimetric method for determination of sugars and related substances. Analytical Biochemistry, Harlow, v.28, p.350-356, 1956. ). Extraction was performed using three replicates of dry seeds (~ 1.2 g per replicate) from each treatment. Samples were ground in 10 mL of 80% ethanol and then maintained in water bath at 90 °C for 5 min to inactivate enzymes. After, they were centrifuged at 1000g at 4 °C for 5 min and the residue was extracted twice more with 80% ethanol at 80 °C for 5 min and once more with water at 60 °C for 5 min. For each sample, extracts were combined and submitted to vacuum concentration at 35 °C.

Protein quantification-For protein extraction (SUDA; GIORGINI 2000 SUDA, C.N.K.; GIORGINI, J.F. Seed composition and mobilization during germination and initial seedling development of Euphorbia heterophylla. Revista Brasileira de Fisiología Vegetal, Londrina, v.12, p.226-245, 2000. ), three replicates of dry seeds (~ 1.2 g) from each treatment were considered. Proteins were extracted from endosperm consecutively according to their solubility - albumins (with distilled water), globulins (with 5% sodium chloride), prolamins (60% ethanol), and glutelins (with 0.4% sodium hydroxide) every 24h. Extracts were centrifuged at 15,000g for 30 min and supernatants were collected and used for protein quantification according to Bradford (1976) BRADFORD, M.M. A rapid and sensitive method for the quantification of microgram quantities of protein utilizing the principle of protein-dye binding. Analytical Biochemistry, Harlow, v.72, p.248-254. 1976 .

Lipid quantification-Lipids were extracted according to Ambalkar et al. (2011) AMBALKAR, V.U.; SAPKAL, V.S.; TALIB, M.; KHANDELWAL, S.A. Soxhlet extraction of Neem seed (Azadirachta indica A. Juss) using hexane as a solvent. International Journal Chemical and Analytical Science, Amsterdam, v. 2, p.10-11, 2011. from three replicates of three seeds (~ 4.0 g per replicate) from each treatment. Endosperms were ground in mortar and then lipids were extracted with hexane under continuous flow for three periods of 8h. During each extraction period, the supernatant was collected, filtered, concentrated and stored.

Statistical analysis-Data regarding ABA, GA , total soluble sugar, protein, and lipid contents are indicated in dry basis and were submitted to analysis of variance, with posterior construction of polynomial regression models corresponding to the period between beginning of soaking and visible germination (PIMENTEL-GOMES, 2009 PIMENTEL-GOMES, F. Curso de estatística experimental. 15. ed. Piracicaba: ESALQ, 2009. 75p. ).

Correlation analysis among ABA, GA, sugars, proteins and lipid contents was performed. For analysis purposes, r values between 0.8 - 1.0 were considered strong correlations. Statistical analysis was performed using the SAS and PAST software (SAS institution, Cary, NC; Hammer et al, 2001 HAMMER, Ø.; HARPER, D.A.T.; RYAN, P.D. PAST: Paleontological statistics software package for education and data analysis. Palaeontologia Electronica, College Station, v.4, n.1, p.1-9, 2001. ).

Results and discussion

In ungerminated seeds (without soaking and soaked in water), reductions in ABA content were not observed over time, while small changes were observed in GA content. Nevertheless, seeds soaked in GA4+7 + BA showed reduction in ABA content and increased GA levels from the beginning of soaking until the beginning of primary root protrusion (1 mm) after 10 days (Figure 1 A-D).

Figure 1
Abscisic acid (ABA) and giberellin (GA) contents in Annona macroprophyllata (A and C) and A. purpurea (B and D) seeds without soaking (?), soaked in water (?) and soaked in GA4+7 +BA (?) evaluated at 0, 2, 5, 10, and 15 days after treatments. Equations represent treatments with plant regulators. The values represent the average of replicates, and standard deviations are indicated.

It must be emphasized that Annona macroprophyllata seeds showed higher GA content compared to A. purpurea from seed dispersal and particularly after treatment with plant growth regulators. The application of GA4+7 + BA led to increase in GA content over time, while ABA content decreased. After 2 days of soaking in plant growth regulators, reduction in ABA content was constant in both species, although A. purpurea seeds showed the highest ABA levels even after treatment with plant growth regulators (Fig. 1B).

In both species, seeds treated with GA4+7 + BA showed constant degradation of albumins (Fig. 2 AB), differing from ungerminated seeds (without soaking and soaked in water). The degradation level was different in each species. Seeds without soaking in water, A. macroprophyllata seeds (time 0), showed 9668.3 μg g-1 albumin content, decreasing to 2347.3 μg g-1 at 15 days after the beginning of soaking in plant growth regulators.

Figure 2
Albumin, globulin, prolamin and glutelin contents in Annona macroprophyllata (A. C , E and G) and A. purpurea (B, D , F and H) seeds without soaking (?), soaked in water (?) and soaked in GA4+7 +BA (?) evaluated at 0, 2, 5, 10, and 15 days after soaking. Equations represent treatments with plant regulators. The values represent the average of replicates, and standard deviations are indicated.

In A. purpurea, initial level was 19632.4 μg g-1 and reduced to 6368.5 μg g-1 at the end of the evaluation period.

Distinct patterns between species were observed regarding albumin and globulin degradation in seeds treated with GA4+7 + BA. In A. macroprophyllata, slow albumin degradation was detected at the beginning of evaluations (0 and 2 days), while sharp globulin degradation occurred from the beginning of soaking (Fig. 2C). In A. purpurea seeds, albumin and globulin (Fig. 2 B-D) degradation started later (10 days), but it was similar to that observed in A. macroprophyllata (4461 and 3929 ug g-1, respectively).

Prolamins and glutelins were also degraded in both species over time due to the application of GA4+7 + BA. Nevertheless, such proteins showed 100-fold lower contents and their degradation was only significant at 15 days (Fig. 2 E-H).

Regarding total soluble sugar degradation, dormant A. macroprophyllata and A. purpurea seeds showed small decrease in sugar content regardless of soaking in water, thus requiring exogenous application of GA4+7 + BA to stimulate higher degradation (Fig. 3 A-B). Total soluble sugar degradation is higher as more energy is required for embryo development, thus resulting in lower total soluble sugar content, which was observed at 1 cm primary root.

Figure 3
Total soluble sugar content in A) Annona macroprophyllata and B) A. purpurea seeds without soaking (?), soaked in water (?) and soaked in GA4+7 +BA (?) evaluated at 0, 2, 5, 10, and 15 days after the treatments. Equations represent treatments with plant regulators. The values represent the average of replicates, and standard deviations are indicated.

Comparing species when treated with GA4+7 + BA, A. purpurea seeds showed lower initial sugar content and faster degradation since the beginning of soaking (Fig. 3B). However, both species showed similar sugar levels in primary root protrusion.

Lipid reserves were degraded in seeds from all treatments and with the application of GA4+7 + BA (Fig. 4),degradation was faster compared to the others treatments.

Figure 4
Lipid content in A) Annona macroprophyllata and B) A. purpurea seeds without soaking (?), soaked in water (?) and soaked in GA4+7 +BA (?) evaluated at 0, 2, 5, 10, and 15 days after the treatments. Equations represent treatments with plant regulators. The values represent the average of replicates, and standard deviations are indicated.

In A. macroprphyllata seeds (Fig. 4A), such reduction was more evident at 15 days, while A. purpurea seeds showed greater energy consumption after 10 days for the maintenance of seedling development (Fig. 4B).

Thus, application of GA4+7 + BA led to faster reserve degradation, mainly of proteins and total sugars, followed by lipids, which confirms the action of such plant growth regulators on reserve degradation.

Correlation analysis between presence of plant regulators and reserve amounts (Tabela 1) indicates that, in general, the higher the presence of ABA (r = 0.72-0.99), the higher the content of reserve macromolecules. These relationships were more evident in a larger number of reserve molecule types in Annona purpurea than in A. macroprophyllata.

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Table 1
Correlation analysis between presence of phytoregulators and reserves of Annona macroprophyllata and Annona purpurea.

On the other hand, inverse linear relationships between gibberellins and reserves are statistically weak, which indicates the activity of these plant regulators to trigger mobilization, that is, there is an exact balance point between ABA decrease and increase of gibberellins, leading to germination and reserve degradation.

In the present study, ABA content was higher than GA in freshly dispersed A. macrophyllata and A. purpurea seeds, thus explaining the absence of germination.

ABA accumulation in dormant seeds occurs in the final maturation stages, inducing dormancy (GUBLER et al., 2005 GUBLER, F.; MILLAR, A.A.; JACOBSEN, J.V. Dormancy release, ABA and pre-harvest sprouting. Current Opinion in Plant Biology, Saint Louis, v. 8, p.183-187, 2005. ; BENTSIN and KOORNNEEF, 2008 BENTSINK L, KOORNNEEF M. Seed dormancy and germination. The Arabidopsis Book, Rockville, v.6, p.1-18, 2008. ) and ensuring the survival of species under adverse conditions. Such a strategy would allow both species to withstand dry and hot months until the beginning of the rainy season, as also suggested by González-Esquinca et al. (2015) GONZÁLEZ-ESQUINCA, A.R.; DE-LA-CRUZ-CHACÓN, I.; DOMÍNGUEZ-GUTÚ, L.M. Dormancy and germination of Annona macroprophyllata (Annonaceae): the importance of the micropylar plug and seed position in the fruits. Botanical Sciences, Ciudad de México, v. 93, n.3, p.1-7, 2015. .

Thus, there is probable temporary inability of seeds of both species to increase endogenous GA due to ABA content with the objective of guaranteeing dormancy (YAMAGUCHI, 2008 YAMAGUCHI, S. Gibberellin metabolism and its regulation. Annual Review of Plant Biology, Palo Alto, v.59, p.225-251, 2008. ; BEWLEY et al., 2013 BEWLEY, J.D.; BRADFORD, K.J.; HILHORST, H.W.M.; NONOGAKI, H. Seeds: physiology of development, germination and dormancy. 3rd ed. London: Springer, 2013. 392p. ; KANG et al., 2015 KANG, J.; YIM, S.; CHOI, H.; KIM, A.; LEE, K.P.; LOPEZ-MOLINA, L. MARTINOIA, E.; LEE, Y. Abscisic Acid transporters cooperate to control seed germination. Nature Communications, Londres, v.6, p.1-10, 2015. ). Such fact was demonstrated when GA content did not increase after reactivation of seed metabolism during soaking in water. The hormonal balance needs to be changed for dormancy overcoming, either in response to environmental changes or by exogenous application of germination promoters, which was performed and observed with the application of GA4+7 + B in the present study.

In the present study, GA3 was effectively used as a reference to express the content of total gibberellins.

GA3 is a phytoregulator involved in seed germination (CHEN et al., 2010 CHEN, S.Y.; CHIEN, C.T.; BASKIN, J.M.; BASKIN, C.C. Storage behavior and changes in concentrations of abscisic acid and gibberellins during dormancy break and germination in seeds of Phellodendron amurense var. wilsonii (Rutaceae). Tree Physiology, Oxford, v.30, n.2, p.275-284, 2010. ), especially in Annona diversifolia (CAMPBELL; POPENOE, 1968 CAMPBELL, C.W. ; POPENOE, J. Effect of gibberellic acid on seed dormancy of Annona diversifolia Saff. Tropical Region American Society for Horticultural Science, Mount Vermon, v.11, p.33-36, 1968. ). Although there are more active forms of gibberellins (OGAWA et al., 2003 OGAWA, M.; HANADA, A.; YAMAUCHI, Y.; KUWAHARA, A.; KAMIYA, Y.; YAMAGUCHI, S. Gibberellin biosynthesis and metabolism: A convergent route for plants, fungi and bacteria. Plant Cell, Rockville, v.15, p.1591–1604, 2003. ), the increase in GA3 indicates (even when not directly related to biosynthesis) an increase in total gibberellins.

It has recently been proposed that GA3 can be converted into GA1 (CHEN et al., 2008 CHEN, S.Y.; KUO, S.R.; CHIEN, C.T. Roles of gibberellins and abscisic acid in dormancy and germination of red bayberry (Myrica rubra) seeds. Tree Physiology, Oxford, v.28, n.9, p.1431-1439, 2008. ), which in fungi is a more recurrent fact (SALAZAR CEREZO et al., 2018 SALAZAR-CEREZO, S.; MARTINEZ-MONTIEL, N.; GARCIA-SANCHEZ, J.; PEREZ-Y-TERRON, R.;MARTÍNEZ-CONTRERAS, R. D. Gibberellin biosynthesis and metabolism: A convergent route for plants, fungi and bacteria. Microbiological Research, Jena, v.208, p.85-98, 2018. ). For this reason, the presence of total gibberellins and not only GA3 has been reported. In addition, reduction in ABA content is not sufficient for dormancy overcoming, since changes in sensitivity to ABA and increased levels of promoters are needed, because seeds unable to produce GAs do not germinate (YAMAGUCHI, 2008 YAMAGUCHI, S. Gibberellin metabolism and its regulation. Annual Review of Plant Biology, Palo Alto, v.59, p.225-251, 2008. ; NONOGAKY et al., 2010 NONOGAKI, H.; BASSEL, G.W.; BEWLEY, J.D. Germination-still a mystery. Plant Science, Limerick, v.179, p.574-581, 2010. ; KANG et al., 2015 KANG, J.; YIM, S.; CHOI, H.; KIM, A.; LEE, K.P.; LOPEZ-MOLINA, L. MARTINOIA, E.; LEE, Y. Abscisic Acid transporters cooperate to control seed germination. Nature Communications, Londres, v.6, p.1-10, 2015. ). An increase in GA content leads to the synthesis of degradative enzymes for embryo development (KUCERA et al., 2005 KUCERA, B.; COHN, M.A.; LEUBNER-METZGER, G. Plant hormone interactions during seed dormancy release and germination. Seed Science Research, Wallingford, v.15, p.281-307, 2005. ), and lipids and carbohydrates are used as energy source (PRITCHARD et al., 2002 PRITCHARD, S.L.; CHARLTON, W.L.; BAKER, A.; GRAHAM, I.A. Germination and storage reserve mobilization are regulated independently in Arabidopsis. The Plant Journal, Oxford, v. 31, n.5, p.639-647, 2002. ; SUBEDI; BHATTARAI 2003 SUBEDI CK, BHATTARAI T. Effect of gibberellic acid on reserve food mobilization of maize (Zea mays L. var. Arun-2) endosperm during germination. Himalayan Journal of Sciences, Haridwar, v.1, p.99-102, 2003. ), while proteins and amino acids are used in the formation of new tissues (RAMAKRISHNA, 2007 RAMAKRISHNA, V. Mobilization of albumins and globulins during germination of Indian bean (Dolichos lablab L. var. lignosus) seeds. Acta Botanica Croatica, Zagreb, v. 66, p. 135-142, 2007. ). In both species, reserve degradation began during imbibition phase in seeds treated with GA4+7 + BA. Among reserves, lipids were found in higher contents, followed by proteins and soluble sugars.

Galastri (2008) GALASTRI, N.A. Morfoanatomia e ontogênese de frutos e sementes de Annona dioica A.St.-Hil., Duguetia furfuracea (A.St.-Hil.) Saff. e Xylopia emarginata Mart. (Annonaceae). 2008. Dissertação (Mestrado) – Instituto de Biociências, Universidade Estadual Paulista, Botucatu, 2008. detected higher protein and lipid contents in seeds of other Annonaceae species (Duguetia furfuracea and Xylopia emarginata) and detected higher starch content in Annona dioica seeds. Reduction in total sugar content was detected from the beginning of soaking in plant growth regulators in both species, until the protusion of the primary roots (end of germination). Similary, Gimenez et al. (2014) GIMENEZ, J.I.; FERREIRA, G.; CAVARIANI, C. Tetrazolium test for assessment of seed viability of atemoia (Annona cherimola Mill. x A. squamosa L.). Journal of Seed Science, Londrina, v.36, n.3, p.357-361, 2014. observed fast reduction from total soluble sugars in Annona emarginata seeds during imbibition (Phase I of the germination process), changed from 43 mg g-1 in the beginning (seeds with 20% of water) to 29 mg g-1 at the end of this phase, when seeds showed 35% of water. This rapid reduction in soluble sugar content may be related to its easy degradation for respiration activation and ATP generation for the biosynthesis of proteins and other molecules required for cell division and elongation or other physiological processes such as ATPase-mediated solute transport (BEWLEY et al., 2013 BEWLEY, J.D.; BRADFORD, K.J.; HILHORST, H.W.M.; NONOGAKI, H. Seeds: physiology of development, germination and dormancy. 3rd ed. London: Springer, 2013. 392p. ). Soluble sugars represent less than 10% of the total lipid reserves of A. macroprophyllata and A. purpurea seeds. So, while these seeds have about 470mg g-1 and 450 mg g-1 of lipids, they have 37 mg g-1 and 33 mg g-1 of sugars, respectively. The use of GA4+7 + BA lead a rapid lipid degradation maybe to guarantee energy to the germination process.

With respect to proteins, although degradation has been considered a growth-related process in seedlings (Ramakrishna e Rao 2005a RAMAKRISHNA, V.; RAO, P.R. Axial control of protein reserve mobilization during germination of Indian bean (Dolichos lablab L.) seeds. Acta Biologica Szegediensis, Szeged, v.49, p.23-27, 2005a. , b RAMAKRISHNA, V.; RAO, P.R. Purification of acidic protease from the cotyledons of germinating Indian bean (Dolichos lablab L. var. lignosus) seeds. African Journal of Biotechnology, Nairobi, v.4, p.703-707, 2005b. ), A. macroprophyllata and A. purpurea seeds showed degradation from the first two days of soaking in treatment with GA4+7 + BA. This faster protein degradation due to the aplication of plant growth regulators indicate a possible production of materials like amino acids, to produce new tisses, speeding up germination process, unlike other treatments. Moreover, albumin and globulin fractions were degraded in different ways, globulins were continuously degraded from the beginning of soaking, while albumins reached their maximum degradation at later germination stages, as also observed by Ramakrishna (2007) RAMAKRISHNA, V. Mobilization of albumins and globulins during germination of Indian bean (Dolichos lablab L. var. lignosus) seeds. Acta Botanica Croatica, Zagreb, v. 66, p. 135-142, 2007. during the germination of Dolichos lablab vr. lignosus seeds. Schlereth et al. (2000) SCHLERETH, A.; BECKER, C.; HORSTMANN, C.; TIEDEMANN, J.; MUNTZ, K. Comparison of globulin mobilization and cysteine proteinases in embryonic axes and cotyledons during germination and seedling growth of vetch (Vicia sativa L.). Journal Experimental Botany, Oxford, v.51, p.423-1433, 2000. observed degradation of the majority of globulins from the embryonic axis of Vicia sativa seeds, showing radicle protrusion after 24h of soaking, while degradation from cotyledons had not yet been detected. Early glutelin degradation during soaking was also observed by Suda and Giorgini (2000) SUDA, C.N.K.; GIORGINI, J.F. Seed composition and mobilization during germination and initial seedling development of Euphorbia heterophylla. Revista Brasileira de Fisiología Vegetal, Londrina, v.12, p.226-245, 2000. in Euphorbia heterophylla seeds.

The authors also found low prolamin contents in seeds of different Annonaceae species.

The two species evaluated in the present study were different regarding ABA content needed for maintaining dormancy and inducing germination. A. macroprophyllata required 0.10 μg g-1 ABA, while A. purpurea required 0.60 μg g-1 for maintaining dormancy. After application of plant growth regulators, reduction in ABA content was detected, reaching 0.02 μg g-1 (A. macroprophyllata ) and 0.20 μg g-1 (A. purpurea ) in germinated seeds, showing 1 mm primary root. Higher ABA content in A. purpurea seeds may be responsible for improved resistance for overcoming seed dormancy (29% germination). In this context, lower initial ABA content may have facilitated dormancy overcoming in A. macroprophyllata seeds (71% germination). It is noteworthy that in A. purpurea seeds with broken dormancy, ABA content was higher than in A. macroprophyllata seeds. However, in both species, the final GA content in germinated seeds was very similar.

While non-dormant seeds showed high metabolism and subsequent germination, dormant seeds showed metabolism with no sufficient changes for inducing germination. Such low metabolic activity is due to the need for dormancy overcoming for later germination, which is due to the high ABA content inhibiting the synthesis of GA and enzymes involved in reserve degradation (PEREZ-FLORES et al., 2003 PÉREZ-FLORES, L.; CARRARI, F.; OSUNA-FERNÁNDEZ, R.; RODRÍGUEZ, M.V.; ENCISO, S.; STANELLONI,R.; SÁNCHEZ, R.A.; BOTTINI, R.; IUSEM, N.D.; BENECH-ARNOLD, R.L. Expression analysis of a GA 20-oxidase in embryos from two sorghum lines with contrasting dormancy: possible participation of this gene in the hormonal control of germination. Journal of Experimental Botany, Oxford, v.54, p.2071-2079, 2003. ; ALI-RACHED et al., 2004 ALI-RACHEDI, S.; BOUINOT, D; WAGNER, M.; BONNET, M.; SOTTA, B.; GRAPPIN, P.; JULLIEN, M. Changes in endogenous abscisic acid levels during dormancy release and maintence of mature seeds: studies with the Cape Verde Islands ecotype, the dormant model of Arabidopsis thaliana. Planta, Berlin, v.219, p.479-488, 2004. ; GUBLER et al., 2005 GUBLER, F.; MILLAR, A.A.; JACOBSEN, J.V. Dormancy release, ABA and pre-harvest sprouting. Current Opinion in Plant Biology, Saint Louis, v. 8, p.183-187, 2005. ). Thus, dormant seeds can support low level of metabolic activity during imbibition (Phase I) and Phase II, but they did not reach Phase III with visible germination (BEWLEY et al., 2013 BEWLEY, J.D.; BRADFORD, K.J.; HILHORST, H.W.M.; NONOGAKI, H. Seeds: physiology of development, germination and dormancy. 3rd ed. London: Springer, 2013. 392p. ).

Conclusion

This study allows conclude that Annona macroprophyllata and A. purpurea seeds are dispersed with ABA content preventing GA synthesis, thus demonstrating their inability to produce GAs after dispersal, ensuring dormancy during the dry period. Dormancy overcoming occurs by changing the relationship between endogenous ABA and GA - in the present study by the application of GA - leading to reduction in ABA content, which results in increased GA synthesis and reserve degradation, thus resulting in complete germination with primary root protrusion.

Acknowledgments

This study was financed in part by the Coordenação de Aperfeiçoamento de Pessoal de Nível Superior – Brasil (CAPES) – Finance Code 001”, with posdoctorade scholarship to first autor.

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SOCOLOWSKI, F.; CICERO, S.M. Use of growth regulators to overcome seed dormancy in Xylopia aromatica (Annonaceae). Seed Science and Technology, Zurich, v.39, p.21-28, 2011.
STENZEL, N.M.C.; MURATA, I.M.; NEVES, C.S.V.J. Superação da dormência em sementes de atemóia e fruta-do-conde. Revista Brasileira de Fruticultura, Jaboticabal, v.25, n.2, p.305-308, 2003.
SUBEDI CK, BHATTARAI T. Effect of gibberellic acid on reserve food mobilization of maize (Zea mays L. var. Arun-2) endosperm during germination. Himalayan Journal of Sciences, Haridwar, v.1, p.99-102, 2003.
SUDA, C.N.K.; GIORGINI, J.F. Seed composition and mobilization during germination and initial seedling development of Euphorbia heterophylla. Revista Brasileira de Fisiología Vegetal, Londrina, v.12, p.226-245, 2000.
YAMAGUCHI, S. Gibberellin metabolism and its regulation. Annual Review of Plant Biology, Palo Alto, v.59, p.225-251, 2008.

Publication Dates

Publication in this collection
09 Nov 2020
Date of issue
2020

History

Received
11 June 2020
Accepted
07 Oct 2020

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	Annona macroprophyllata		Annona purpurea
	ABA	GA	ABA	GA
albumin	0.7260 (0.1649)	-0.3905 (0.5158)	0.9369 (0.0189)	-0.4491 (0.4481)
globulin	0.8752 (0.0419)	-0.2881 (0.6383)	0.7537 (0.1412)	-0.0479 (0.9391)
prolamin	0.6931 (0.1944)	-0.0689 (0.9122)	0.4910 (0.4009)	-0.3728 (0.5366)
glutelin	0.5175 (0.3719)	0.08959 (0.8861)	0.9017 (0.0365)	-0.5246 (0.3641)
total soluble sugars	0.6159 (0.2686)	-0.3163 (0.6041)	0.9969 (0.0002)	-0.6972 (0.1907)
lipids	0.9683 (0.0067)	-0.4995 (0.3915)	0.9296 (0.0222)	-0.7686 (0.1287)

Brasil