Brazil has great floristic diversity, especially in Bromeliaceae, with 1,712 species catalogued (Gouda et al., 2022). Among the states with the highest concentration of species, Bahia (358), Espírito Santo (334), Rio de Janeiro (333) and Minas Gerais (331) stand out, with species occurring mainly in the Atlantic Forest (940) and Cerrado (255) (Reflora, 2023). The production of bromeliads on a commercial scale is a viable and well-explored activity in Brazil, with highlighted use in landscaping projects and for decoration of indoor environments, due to the easy maintenance, hardiness and acclimatisation of these plants to different environments (Anacleto and Negrelle, 2013). The species present different colours and leaf shapes, which increases their added value. In this sense, bromeliads of the genus
Due to the increased use of bromeliads in Brazilian landscaping, large numbers of plants end up being removed from nature, which is one of the factors contributing to the increase in endangered species (Pereira et al., 2010). Among the
Interest in the propagation of native species has intensified due to the growing concern with environmental problems. However, the knowledge available for the management and analysis of the seeds of most species is still limited, making it difficult to characterise their physical and physiological attributes. It is crucial to understand the behaviour of growth and development factors in native species as this allows the creation of cultivation protocols. These protocols, in turn, make it possible to introduce new species of economic and ornamental value to the market, in addition to contributing to the recovery of already degraded areas (Ribeiro et al., 2012; Borges et al., 2018).
For the germination process to occur uniformly and with the highest possible percentage, some procedures can be adopted in the seeds, such as the application of plant growth regulators, for example, gibberellic acid (GA3). Gibberellins promote germination through several metabolic state changes in the seed that allow the embryo to re-establish its activity (Hossel et al., 2018).
One way of stimulating germination provided by GA3 is through the induction of the production of hydrolytic enzymes (such as amylases) in the endosperm, which break down starch and other reserve substances, thus generating soluble organic compounds that provide energy for the germinating embryo (Hossel et al., 2018). There are reports of improvement in germination and overcoming dormancy of seeds of several species with the use of GA3 (Hossel et al., 2018). Despite this, one of the obstacles to the application of plant growth regulators is that they are easily degraded when exposed to environmental factors, such as light and temperature, resulting in the loss of their activity. In this context, the use of nanotechnology aims to provide nanoscale materials capable of improving stability and activity, in addition to reducing possible environmental impacts (Ashraf et al., 2021). Thus, nanoencapsulation provides advantages such as longer action time, increased biological activity, and reduced concentration required for the desired effect. Another important point is that the material that makes up the particles produces non-toxic metabolites and is easily degraded, hence the option to use natural biodegradable polymers, such as alginate and chitosan (Francisco and García-Estepa, 2018; Pascoli et al., 2018).
Studies associating nanoparticles (NPs) containing plant regulators such as GA3 are still in infancy and mainly aimed at large crops such as beans (
The experiment was conducted at the Seed Laboratory of the State University of Londrina (UEL). Ripe fruits of
The fruits were allocated in Kraft® (Londrina-PR) paper bags, identified and transported to the laboratory. In a shaded place, they were dried in the open air for 3 days to facilitate the extraction of the seeds, which were stored in Kraft® paper bags, in the refrigerator at 7.5 ± 1.0°C and at a relative humidity (RH) of 26 ± 7%, for 270 days. For the characterisation of the lot, the water content and viability of the seeds were determined by the tetrazolium test, both following the specifications of the Rules for Seed Analysis (BRASIL, 2009). This characterisation occurred after the harvest (10 days) and before the installation of the experiment (after 270 days).
For the determination of water content, 0.2 g of seeds of each species were placed in an oven at 105 ± 3°C for 24 hr. For carrying out the tetrazolium test, four repetitions of 25 seeds each were used. For each species, the seeds were placed in cryovials with a capacity of 2 mL and subsequently completed with distilled water. After 24 hr at 25°C in a germination chamber, the water was removed, and a 1% tetrazolium salt solution was added. The seeds then remained in a germination chamber in the absence of light for 24 hr at 30°C. After this period, the percentage of viable seeds was evaluated with the aid of a magnifying glass. To calculate the percentage of viable seeds, empty seeds were not considered, that is, those without an embryo.
Gibberellic acid (GA3—90%), sodium alginate (ALG), chitosan (CS) and tripolyphosphate (TPP) were obtained from Sigma-Aldrich® (São Paulo-SP). The NPs were provided by Professor Dr. Leonardo Fernandes Fraceto from Universidade Estadual Paulista (UNESP/ Sorocaba) following the methodology of Pereira et al. (2017).
For the preparation of free GA3 solutions, the product was weighed and diluted in alcohol (70%), and then distilled water was added to obtain an initial concentration of 50 mg · L−1. Next, this solution was diluted in distilled water to obtain the desired doses (0.25, 0.5, 0.75, 1.0, 2.5 and 5.0 mg · L−1).
The nanoformulations were prepared at an initial concentration of 50 mg · L−1. Alginate/chitosan (ALG/ CS) NPs were prepared by the ionotropic pre-gelation method. Initially, with the aid of a peristaltic pump (Miniplus 3, Gilson® (São Paulo-SP)), 3.75 mL of calcium chloride (CaCl2) solution (18 mM) was added to 59 mL of ALG solution (0.063%, pH 4.9) under strong magnetic stirring (500 rpm). During this step, cross-linking of CaCl2 on ALG occurs through ionic interactions, forming a structure called an ‘egg box’.
Subsequently, GA3 was added under stirring until complete dissolution to reach the desired concentration (50 mg · L−1). The ALG/CaCl2/GA3 solution was kept under agitation, and 12.5 mL of an aqueous solution of chitosan (0.07% pH 4.6), prepared in an aqueous solution containing 5.7% of acetic acid, was added over 90 min, forming a polyelectrolyte complex between polymers. The same process occurred without the presence of the GA3 regulator to obtain the ALG/CS NPs without the growth regulator.
Chitosan/tripolyphosphate (CS/TPP) NPs were prepared by the gelling method, with modifications. First, 10 mL of a CS solution (0.2%, pH 4.5), prepared in an aqueous solution of 0.6% acetic acid, was kept under vigorous agitation (500 rpm), and GA3 was added until the final concentration of 50 mg · L−1. After dissolution of GA3, 6 mL of TPP solution (0.1%, pH 4.5 at 4°C) was added. CS/TPP NPs were also prepared without the presence of the regulator.
The formulations were characterised by size, zeta potential, encapsulation efficiency (quantified by high-performance liquid chromatography—HPLC), the polydispersity index (PDI) and pH. The ALG/CS NPs with and without GA3 showed an average size of 450 ± 10 nm, PDI of 0.3, zeta potential of −29 ± 0.5 mV, pH of 4.9% and 100% encapsulation efficiency. CS/TPP NPs with and without GA3 showed an average size of 195 ± 1 nm, PDI of 0.3, zeta potential of +27 ± 3 mV, pH of 4.7 and 90% encapsulation efficiency. Both NPs remained stable for 60 days at room temperature (Pereira et al., 2017).
In all experiments, the seeds were sterilised in a 1% sodium hypochlorite solution (1 min), followed by immersion in 70% alcohol (1 min) and subsequently washed with distilled water. They were then soaked in their respective treatments in Erlenmeyer flasks (50 mL), containing 5 mL of the formulation, and shaken for 5 min at room temperature. In the control treatment (0 mg · L−1), the seeds were pre-soaked in distilled water.
In the work with free GA3, seeds of
For each species, tests were carried out for the first and final germination count since there is no recommendation in the Rules for Seed Analysis for the studied species. The 4th day was considered for the first count and the 10th day for the end of the test. The percentage of germination (GERM) and abnormal seedlings (AS), first germination count (FGC), germination speed index (GSI), mean germination time (MGT), seedling length (SL) and seedling dry mass (SDM) were considered. For SL and SDM, the seedling as a whole was considered, that is, with aerial part and root.
The seeds were placed to germinate on blotting paper moistened with distilled water in the amount of 2.5 times the mass of the non-hydrated paper and placed in crystal polystyrene boxes (Gerbox® (DicaLab – Londrina-PR)) with dimensions 11 cm × 11 cm × 3 cm. The Gerbox® boxes were kept in a growth chamber (B.O.D. type) at 25°C for a photoperiod of 16 hr and under an illuminance of 120 μmol · s−1 · m−2 from fluorescent lamps (BRASIL, 2009).
The GERM was determined considering the normal seedlings, and the AS were also evaluated (BRASIL, 2009), being considered normal those that showed the potential to continue their development and give rise to normal plants when developed under favourable conditions. The FGC was performed at the time of primary root protrusion, which occurred on the 4th day (Nakagawa, 1999). The result was expressed as a percentage.
Concomitantly to the germination test, the count of germinated seeds was performed to establish the GSI obtained through the formula described by Maguire (1962). GSI = G1/N1 + G2/N2 + … + Gn/Nn, in which G1, G2 and Gn are the number of normal seedlings, computed in the first, second and last counts, respectively, and N1, N2 and Nn are the number of sowing days at the first, second and last counts, respectively. The MGT was obtained through the methodology described by Labouriau (1983) and performed simultaneously with the germination test, the number of germinated seeds being counted daily. This index is calculated by the MT equation = (G1T1 + G1T1 + … + GnTn)/(G1 + G2 + … + Gn), where MT is the mean time, in days, required to reach maximum germination; G1, G2 and Gn are the number of germinated seeds at times T1, T2 and Tn, respectively.
At the end of 10 days, the GERM and AS were determined, and the result was expressed as percentage, in addition to the SL (mm) through the measurement of normal seedlings and obtained with the aid of a calliper. The SDM (mg) was determined on an analytical scale (precision ±0.0001 g), after keeping the seedlings in paper bags and ovens with forced air circulation at 65°C until they reached constant mass.
Aiming to identify the phases of the germination process, the seeds were weighed at intervals of 1 hr (in the first 8 hr) and then every 2 hr until 100 hr had passed from the beginning of the weighing. The seeds were placed on blotting paper moistened with distilled water, in a volume 2.5 times the dry weight of the paper and placed in Gerbox® boxes. In the treatment with GA3, the seeds were soaked for 5 min at doses of 0.75 mg · L−1 for the species
The experimental design was completely randomised in both stages. The first stage consisted of seven treatments containing different doses (0, 0.25, 0.5, 0.75, 1.0, 2.5 and 5.0 mg · L−1), and the second stage was composed of five treatments (free GA3, NP ALG/CS/GA3, NP ALG/CS, NP CS/TPP/GA3 and NP CS/TPP) with seven doses in each one (0, 0.25, 0.5, 0.75, 1.0, 2.5 and 5.0 mg · L−1). For the germination test of the two stages and imbibition curve, at each dose, four repetitions of 50 seeds were used. For measurements of length and dry mass, 16 seedlings were randomly selected per replication, and the result was expressed as the average of the four seedlings.
The assumptions of normality of errors and homogeneity of variances were tested using Shapiro– Wilk and Bartlett (
For the characterisation of the seed lot, the values of viability and water content of the seeds are shown in Table 1. The four species studied presented high viability immediately after harvesting, ranging from 78% to 88%, and germination from 71% to 84%. After storage for 270 days in a dry and cold place, there was a reduction in viability to values between 68% and 73% and germination to 36% to 45%. In addition, the water content remained low after storage, ranging from 8.4% to 9.5% after harvest to 7.7% to 8.9% after storage. However, it is noteworthy that a reduction in viability and a significant decrease in germination over time were observed, indicating a possible induction of dormancy caused by the storage period. In addition, pathogens/fungi were not identified in the seeds during the conservation period and in the germination test.
Viability by tetrazolium test (%), germination (%) and water content (%) of
Species | Viability | Germination | Water content | |||
---|---|---|---|---|---|---|
10 days | 270 days | 10 days | 270 days | 10 days | 270 days | |
79 | 68 | 71 | 38 | 9.2 | 8.5 | |
81 | 71 | 75 | 36 | 9.5 | 8.9 | |
88 | 69 | 84 | 45 | 8.7 | 8.1 | |
78 | 73 | 75 | 37 | 8.4 | 7.7 |
Table 2 presents the
FGC | GERM | AS | GSI | MGT | SL | SDM | |
---|---|---|---|---|---|---|---|
0.8012 | 0.8558 | 0.9081t | 0.8954 | 0.7463 | 0.8915 | <0.001 | |
CV (%) | 41.14 | 16.33 | 50.42 | 7.35 | 4.86 | 5.49 | 10.10 |
0.0037 | <0.001 | 0.9844t | <0.001 | 0.0211 | 0.0011 | <0.001 | |
CV (%) | 26.34 | 11.45 | 40.2 | 13.00 | 5.40 | 8.65 | 11.08 |
0.0102 | 0.3135 | 0.8692t | 0.9646 | 0.0166 | 0.0403 | <0.001 | |
CV (%) | 23.44 | 14.95 | 37.86 | 17.23 | 7.81 | 16.02 | 14.80 |
<0.001 | <0.001 | - | <0.001 | <0.001 | <0.001 | <0.001 | |
CV (%) | 15.80 | 6.00 | - | 5.18 | 3.16 | 2.89 | 5.78 |
Data transformed to √x.
AS, abnormal seedlings; CV, coefficient of variation; FGC, first germination count; GA3, gibberellic acid; GERM, germination; GSI, germination speed index; MGI, mean germination time; SDM, seedling dry mass; SL, seedling length.
For FGC, GERM and SDM, the highest values found were at a dose of 5.0 mg · L−1 (21%, 62% and 3.1 g, respectively). In comparison, in the control treatment, the values for the same variables were 10%, 36% and 1.8 g, respectively. MGT was lower at a dose of 5.0 mg · L−1, that is, at this dose, the seeds took 3.00 days for germination.
There was an increase in the GSI with the increased dose of GA3; however, this index stabilised at higher doses, ranging from 9.53 to 11.08 between doses of 1.0 mg · L−1 and 5.0 mg · L−1. A similar response was obtained for SL, so that at doses between 1.0 mg · L−1 and 5.0 mg · L−1, seedlings of 7.65 mm and 7.97 mm were obtained. The responses of
For FGC, there was an increase in germination up to a dose of 0.8 mg · L−1 with 15% germinated seeds. Above this dose, there was a reduction in germination and stabilisation from a dose of 1.0 mg · L−1, ranging from 9% to 11%. For MGT, doses of 0.75 mg · L−1 and 1.0 mg · L−1 provided a shorter time for seed germination, with 3.20 days and 3.38 days, respectively.
In SL, there was an increase of up to a dose of 1.2 mg · L−1, reaching 7.49 mm, with subsequent reduction in length. For SDM, the estimated dose of 0.7 mg · L−1 showed greater mass, with 5.7 mg, and showed a mass reduction for doses above this value. For these variables, in relation to the maximum point obtained, there was an increase of 46% in SL and 56% in SDM compared to the control.
For FGC and GERM, the maximum point obtained was at a dose of 5.0 mg · L−1, with 23% and 64%, respectively. By comparison, the control presented 10% FGC and 35% GERM. In the GSI variable, the highest value was also observed for a dose of 5.0 mg · L−1 (with 10.88), as well as the lowest value of MGT (2.98). The same was also observed for the growth variables, with a greater response in SL (8.28 mm) and SDM (3.98 mg) at a dose of 5.0 mg · L−1.
Regarding the imbibition curves, all the species studied showed three-phase water absorption behaviour, with a rapid increase in initial mass, subsequent stabilisation and then a new increase. According to Figure 5, for
For
The imbibition curves for
For
After verifying the positive effect of free GA3 on germination and vegetative growth, mainly in relation to
Through analysis of variance, it was possible to observe a significant difference for the various variables according to the treatment. The only exception was BP, which had a variation of 2–3% in all treatments. It was also possible to observe that treatments with only NPs (NP ALG/CS and NP CS/TPP) had no effect on GERM, FGC, MGT, SL and SDM (Table 3).
FGC | GERM | AS | GSI | MGT | SL | SDM | |
---|---|---|---|---|---|---|---|
NP ALG/CS-GA3 | |||||||
<0.001 | <0.001 | - | <0.001 | <0.001 | <0.001 | <0.001 | |
CV (%) | 14.56 | 5.41 | - | 3.41 | 3.65 | 2.35 | 7.09 |
Mean | - | - | 3.14 | - | - | - | - |
NP CS/TPP-GA3 | |||||||
<0.001 | <0.001 | - | <0.001 | <0.001 | <0.001 | <0.001 | |
CV (%) | 14.97 | 7.24 | - | 4.23 | 3.27 | 1.97 | 6.44 |
Mean | - | - | 2.29 | - | - | - | - |
NP ALG/CS | |||||||
0.414 | 0.064 | - | <0.001 | 0.024 | 0.053 | 0.474 | |
CV (%) | 22.68 | 10.74 | - | 6.08 | 3.20 | 4.70 | 11.18 |
Mean | 11.0 | 42.0 | 2.71 | 7.45 | - | 7.06 | 7.09 |
NP CS/TPP | |||||||
0.669 | 0.057 | - | <0.001 | 0.006 | 0.003 | 0.406 | |
CV (%) | 22.09 | 11.18 | - | 3.49 | 2.56 | 2.72 | 8.28 |
Mean | 11.0 | 38.0 | 3.14 | 7.06 | - | - | 2.24 |
ALG, sodium alginate; ALG/CS, alginate/chitosan; AS, abnormal seedlings; CS, chitosan; CV, coefficient of variation; FGC, first germination count; GA3, gibberellic acid; GERM, germination; GSI, germination speed index; MGT, mean germination time; NP, nanoparticle; SDM, seedling dry mass; SL, seedling length; TPP, sodium tripolyphosphate.
For FGC, the maximum point obtained for free GA3 was at a dose of 5 mg · L−1 with 23%, while in the treatments with nanoencapsulated GA3, it was 19% and 18%, in the estimated doses of 1.4 mg · L−1 and 0.3 mg · L−1 for NP ALG/CS-GA3 and CS/TPP-GA3, respectively. In GERM, the highest response was obtained for free GA3 with 64% at a dose of 5 mg · L−1, and when encapsulated, the maximum response was 60% for NP ALG/CS-GA3 at an estimated dose of 2.1 mg · L−1 and 55% for NP CS/TPP-GA3 at an estimated dose of 1.7 mg · L−1. The control treatment presented 35% GERM and 10% FGC (Figure 7).
In the GSI and MGT variables, the highest values were also observed for free GA3 at a dose of 5 mg · L−1, with 10.88 and 2.98, respectively. For treatments with nanoencapsulated GA3, the estimated dose of 0.5 mg · L−1 presented the highest values of GSI and MGT, respectively, of 10.19 and 3.16 for NP ALG/CS-GA3 and of 9.05 and 3.28 for NP CS/TPP-GA3. The control treatment presented GSI and MGT, respectively, of 7.05 days and 4.16 days. For MGT, it was also possible to observe a response from empty NPs (NP ALG/CS and CS/TPP), with a maximum response at a dose equivalent to 2.9 mg · L−1 for NP ALG/ CS with 3.8 days, and 2.7 mg · L−1 for NP CS/TPP with 3.8 days (Figure 8).
For SL, when seeds were treated with free GA3, the dose of 5.0 mg · L−1 showed the best response, obtaining average seedlings of 8.28 mm. The same was observed for SDM, with 3.98 mg for the same dose. For NP ALG/ CS-GA3, the estimated optimum dose was 0.3 mg · L−1 with 8.04 mm of SL and 3.68 mg of SDM. For NP CS/ TPP-GA3, the estimated dose of 0.2 mg L−1 had the best response for SL with 7.78 mm, and the estimated dose of 0.4 mg · L−1 presented higher SDM with 3.45 mg. It was also possible to observe an empty response for NP CS/TPP for SL, with 7.26 mm at the equivalent dose of 2.0 mg · L−1. The control treatment presented a mean SL of 6.61 mm and an SDM of 2.15 mg (Figure 9).
In addition to the storage conditions for seeds of the species under study being recommended for seeds with orthodox behaviour (cold and dry), the ideal period for storing and maintaining seed viability is directly related to the water content in which the seeds are conserved. In this sense, the water content, despite being at an adequate level for the studied species (7%–9%), is not applicable to all with the same effectiveness since each one has a tolerable limit regarding desiccation (Rajanaidu and Ainul, 2013).
Even under ideal storage conditions, there was a loss of viability of these seeds since with aging, damage to the membranes occurs and the enzymes lose their catalytic activity (Oliveira et al., 2011). In addition, according to the observed results, the seeds may have entered a state of dormancy after storage. This can also be explained by the tetrazolium test, where despite the low germination after storage, the seeds presented high viability (71–84%). A favourable point of the tetrazolium test is that its results do not suffer interference from conditions that usually interfere in germination analysis, such as the incidence of microorganisms; in addition, this test also serves to clarify factors not explained by the germination test, in this case, relating to dormancy (Carvalho et al., 2013).
Another associated factor is that most
In the case of the seeds under study, this primary dormancy was not observed, so it can thus be classified as secondary dormancy. All the processes involved in this type of dormancy are not yet well elucidated in the literature, and it is recognised that seeds with secondary dormancy germinate normally, but when exposed to unfavourable environmental factors, they are induced to a state of dormancy (Silva et al., 2018). Among the possibilities of dormancy, the physiological possibility occurs through the interaction between inhibitors and germination promoters and is generally overcome through the addition of plant growth regulators, such as GA3, which was observed in this study (Rego et al., 2018).
This GA-induced degradation of seed reserves occurs through the production of hydrolases, which are responsible for weakening the tissue surrounding the embryo (Bocatto and Forti, 2019). Hydrolases, such as amylases, react with the reserves stored in the embryo, breaking down starch and other substances, allowing the resumption of growth of the embryonic axis. With this, simple sugars, amino acids and nucleic acids are formed that stimulate cell elongation, causing the radicle to break the seed coat, accelerating and standardising germination (Paixão et al., 2021).
It was observed in
The regulation of endogenous levels of GAs in seeds, as well as in the plant, occurs through several processes. Internally, the so-called active GAs undergo the process of conjugation, that is, sugars such as glucose unite with the GAs, making them glycosylated and thus reversibly inactive. GAs can also be irreversibly inactivated by enzymes. These mechanisms control and contribute to the balance in the levels of GAs; in addition, studies demonstrate several inhibitors that act in the process of biosynthesis of GAs (Kashiwaqui et al., 2019).
Regarding the improvement in plant growth variables, that is, length (SL) and mass (SDM), all species were stimulated by GA3. Gibberellins promote these responses through several factors, such as the orientation of microtubules towards the axis of cell growth; thus, cells increase only towards the axis of growth (Chaudhary et al., 2019; Purba et al., 2021).
GAs stimulate cell division, especially meristematic cells, and affect cell wall plasticity, favouring growth. Furthermore, GAs have the potential to stimulate active plant growth, such as stem and leaf elongation. GAs also interact with other hormones, such as cytokinins and auxins, enhancing these effects (Gupta and Chakrabarty, 2013; Chaudhary et al., 2019; Purba et al., 2021).
Research shows that the use of GA3 has an effect at different stages of plant development. Treatment with 100 μM of GA3 promoted greater height and a greater number of flower buds in jewelweed (
The pre-germination treatment of beton seeds (
The imbibition curve data indicate a triphasic pattern of water absorption by the seeds. It is known that the speed of occurrence of this process depends on the characteristics of the seeds of each species, such as the chemical composition and permeability of the seed coat (Albuquerque et al., 2009). Phase I results in rapid absorption of water and is characterised by the beginning of the modification of the reserves present in the seeds to guarantee energy and essential nutrients for the growth of the embryo (Araújo et al., 2018).
In phase II, water absorption decreases and stabilisation occurs, being a phase also known as stationary. Another characteristic of this phase is the reactivation and initiation of cellular metabolic processes, with the expansion of the embryo and increased activity of enzymes used for embryo development. Finally, in phase III, there is again an increase in water absorption by the seed due to seedling growth and cell reorganisation. The striking characteristic of this phase is that germination becomes visible, that is, the radicle protrudes (Araújo et al., 2018).
Morphological studies carried out by Duarte et al. (2009) in
According to the imbibition curve, none of the species of
It is also noted that GA3 acted on the embryo of the most responsive species (
The purpose of application through NPs is to provide slow and sustained release of the active substance, in addition to protecting it against degradation (Pereira et al., 2017). One of the advantages of using biodegradable polymeric systems is that they can be used in the metabolism of living organisms. Furthermore, in this study, none of the NP systems used showed phytotoxic effects during the germination phases, corroborating the results found in the literature (Pereira et al., 2019).
It was observed that the responses for freely applied and nanoencapsulated GA3 had different maximum response points, demonstrating that the form of application provided different biological effects. The greatest effects on variables using NPs were observed at lower doses (0.75mg · L−1 and 1.0 mg · L−1), while the greatest effects of GA3 in the free form occurred at the highest doses (2.5 mg · L−1 and 5.0 mg · L−1). This can be explained by the fact that free GA3 had direct contact with the seeds, being released faster than nanoencapsulated GA3, which provided a slower release. In addition, some NPs remain adhered to the surface of the seed, maintaining the supply of GA3 even after the soaking process. Furthermore, NPs, mainly CS/ALG due to their negative charge, are more likely to enter the seeds, making it impossible for them to become adsorbed by the cell wall (Pereira et al., 2019).
The CS present in NPs is easily absorbed, prolonging the contact time and facilitating the absorption of bioactive molecules, in this case GA3. The good acceptability and absorption of NPs are also reported due to the association with the surface of the plant, or seed, in this case, due to the presence of carboxyl, hydroxyl, amide and phosphate groups that provide potential sites for binding with CS, which with its cationic properties, manages to adsorb on the surface, prolonging the contact of the nanoparticle with the plant (Li et al., 2019).
In the study in question, there was no better response with the use of nanoencapsulated GA3, with emphasis on the dose reduction when supplied this way, probably due to better delivery of GA3 to the plants. The fact that there was no difference in the two forms of release can be explained by the fact that the study experiment was carried out in a fully controlled environment (temperature and humidity), thus not affecting the degradation and bioavailability of GA3.
In studies using different nanocarrier systems containing GA3 through alginate/chitosan (ALG/CS) and CS/TPP, it was demonstrated that the treatment of seeds with ALG/CS-GA3 was more effective and provided an increase in root development, leaf area and photosynthetic pigments (chlorophylls and carotenoids) of bean plants (
The same result was also found in the present study, in which NPs containing ALG/CS showed a better response than CS/TPP, which was also observed by Pereira et al. (2019), in which tomato seeds (
The two NP systems have different GA3 release mechanisms, causing different responses. Among the NP characteristics, the zeta potentials of the studied formulations differ, being negative for ALG/CS and positive for CS/TPP. Studies show that the zeta potential participates in the plant–NP interaction. NPs with positive zeta potential, such as CS/TPP, have a strong interaction with the negative groups of the plant cell wall, with low cell internalisation and a tendency to accumulate on the cell surface. On the other hand, NPs with negative zeta potential, such as those of ALG/CS, manage to be rapidly distributed and internalised in cells (Zhu et al., 2012).
The effect of NPs containing only ALG/CS or CS/TPP was observed for some variables. Of the compounds used in the formulation of NPs, the ability of CS to increase the response in plants depending on the species and concentration has already demonstrated in several studies, being mainly associated with plant defence responses to different biotic and abiotic stresses (Malerba and Cerana, 2016; Odat et al., 2021).
Chitosan was able to improve seed germination and initial growth of wheat seedlings (
The present study shows the importance of physiological knowledge of seeds after maturation and during storage and that seeds of
For
When nanoencapsulated, GA3 resulted in greater responses at lower doses, proving the controlled release of the regulator, with greater responses for NPs containing ALG/CS. The dose of 5.0 mg · L−1 of free GA3 and between 0.75 mg · L−1 and 1.0 mg · L−1 for nanoencapsulated containing ALG/CS-GA3 are recommended for germination of