http://orcid.org/0000-0002-0455-3484
Figures
Abstract
Seed germination is considered the beginning of the spermatophyte lifecycle, and it is a crucial stage in determining subsequent plant growth and development. Although many previous studies have found that melatonin can promote seed germination, the role of melatonin in cotton germination remains unexamined. The main objective of this study is the characterization of potential promotional effects of melatonin (at doses of 0, 10, 20, 50, 100 and 200 μM) on cotton seed germination. This experiment demonstrated that low concentrations of melatonin can promote germination, while high concentrations failed to promote germination and even inhibited germination. Together, these results indicate that a 20 μM melatonin treatment optimally promotes cotton seed germination. Compared with the control, germination potential (GP), germination rate (GR), and final fresh weight (FW) increased by 16.67%, 12.30%, and 4.81%, respectively. Although low concentrations of melatonin showed some improvement in vigor index (VI), germination index (GI), and mean germination time (MGT), these effects were not statistically significant. Antioxidant enzyme activity during seed germination was most prominent under the 20 μM melatonin treatment. Superoxide dismutase (SOD) and peroxidase (POD) activities were significantly increased by 10.37–59.73% and 17.79–47.68%, respectively, compared to the melatonin-free control. Malondialdehyde (MDA) content was reduced by 16.73–40.33%. Two important plant hormones in seed germination, abscisic acid (ABA) and gibberellins (GAs), were also studied. As melatonin concentration increased, ABA content in seeds decreased first and then increased, and GA3 content showed a diametrically opposite trend, in which the 20 μM melatonin treatment was optimal. The 20 μM melatonin treatment reduced ABA content in seeds by 42.13–51.68%, while the 20 μM melatonin treatment increased GA3 content in seeds to about 1.7–2.5 times that of seeds germinated without melatonin. This study provides new evidence suggesting that low concentrations of melatonin can promote cotton seed germination by increasing the activity of antioxidant enzymes, thereby reducing the accumulation of MDA and regulating plant hormones. This has clear applications for improving the germination rate of cotton seeds using melatonin.
Citation: Xiao S, Liu L, Wang H, Li D, Bai Z, Zhang Y, et al. (2019) Exogenous melatonin accelerates seed germination in cotton (Gossypium hirsutum L.). PLoS ONE 14(6): e0216575. https://doi.org/10.1371/journal.pone.0216575
Editor: Thomas Roach, University of Innsbruck, AUSTRIA
Received: April 16, 2019; Accepted: June 11, 2019; Published: June 25, 2019
Copyright: © 2019 Xiao et al. 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 author and source are credited.
Data Availability: All relevant data are within the manuscript and its Supporting Information files.
Funding: This work was supported by the National Key R&D Program of China (2018YFD0100306, LL), National Natural Science Foundation of China (No. 31871569 to LL; 31171495) and Modern Technology System of Agricultural Industry in Hebei (HBCT2018040201, CL). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The authors have declared that no competing interests exist.
Introduction
Seed germination is the process by which the radicle breaks through the seed coat; it is an early and crucial stage in the spermatophyte life cycle, referring to the physiological process starting from the uptake of water by the dry seed and ending with radicle protrusion [1]. Seed germination is a complex process regulated by many coordinated metabolic, cellular, and, molecular events in the life cycle of higher plants, and it is also a key period for the establishment of crop populations. Germination includes a range of physical and metabolic events [2]. This stage is greatly affected by the external environment, a period of stress sensitivity and also a critical period for determining the survival of plants under adverse conditions. Seed germination can be considered both the starting point of the plant life cycle and the initial life stage of the plant’s perception of the external environment. Seed germination directly affects the growth and final yield of subsequent cotton seedlings. Therefore, seed germination has important economic and ecological significance [3, 4]. Cotton (Gossypium hirsutum L.) is a globally important cash crop, fiber crop, and oil crop, and it plays an important role in China’s economic development [5]. The quality of seed germination is related to the growth of subsequent cotton seedlings and resulting cotton yields.
Melatonin (N-acetyl-5-methoxytryptamine), a highly conserved and efficient molecule, exists widely in plants and animals [6]. The tryptophan-derived compound is synthesized in the hypothalamus [7] and was first isolated from the pineal gland of cattle in 1958, suggesting it only existed in animals. However, since melatonin was first detected in nine edible plants, including tomatoes (Lycopersicon esculentum) and cucumbers (Cucumis sativus) in 1995 [8], melatonin has been detected in more than 300 plants, including some in monocotyledonous and dicotyledonous families [9–11], and the biosynthetic pathways and physiological functions of melatonin in plants have been extensively studied [12]. Melatonin has been detected in the seeds, roots, fruits, and leaves of plants [13, 14]. In recent years, many studies have shown that melatonin in plants is synthesized from tryptophan and plays an important role in coping with various environmental stresses, regulating plant growth, and development [14–16], including the regulation of seed germination [17]. Moreover, the effect of melatonin on seed germination differs in a concentration-dependent manner such that higher concentrations of melatonin inhibit or do not affect seed germination, while lower concentrations promote seed germination [18–20].
The production of reactive oxygen species (ROS) during seed aerobic metabolism leads to lipid peroxidation, which is an important cause of seed deterioration and inhibition of seed germination. Melatonin is the most potent endogenous compound known to scavenge free radicals, at rates twice and four times as high as those of vitamin E and glutathione, respectively [21, 22]. In normal life activities, plants produce high levels of ROS through enzymatic reactions and leakage of electron transport chains during photosynthesis and respiration. Under normal conditions, cells achieve homoeostasis between ROS production and elimination through antioxidant systems, thus maintaining low ROS levels. As the beginning of plant life, seeds are vulnerable to oxidative damage, but the activity of antioxidant enzymes in seeds is very low, while melatonin has the ability to enhance the activities of scavenging enzymes [23, 24], such as superoxide dismutase (SOD; EC 1.15.1.1) and peroxidase (POD; EC 1.11.1.7), which play crucial roles in decreasing and eliminating ROS. Ultimately, melatonin can protect seeds from environmental damage, thereby ensuring the smooth reproduction of plants [25].
In 2004, Hernández-Ruiz et al. first proposed that melatonin may be a plant growth hormone [18]. It is well known that phytohormones can affect the dormancy and germination of seeds and are important signal molecules for transmitting environmental changes during seed germination. At the same time, they have been extensively studied in dicots and monocots [26]. Abscisic acid (ABA) and gibberellins (GAs) are considered to be the main hormones in seed germination [27]. The dynamic balance of synthesis and catabolism of ABA and GA is the key to complete germination of seeds. GAs, a group of important plant hormones, were first isolated from the pathogenic fungus Gibberella fujikuroi in 1938 by Japanese scholars [28]. GAs regulate the overall growth and development of plants and participate in controlling various plant development processes. At present, more than one hundred kinds of GAs have been found, with only a few, e.g., GA1 and GA3, demonstrating activity. Most related compounds are GA synthesis precursors or products inactivated by metabolism. The active components of plant gibberellins mainly consist of GA1, GA3, GA4, and GA7. GAs can break seed dormancy, promote seed germination, trigger seed germination in suitable environments and time periods, and prepare for subsequent seedling growth [29].
ABA is also an important hormone in the regulation of plant growth and development and accordingly plays a critical role in regulating various physiological processes in plants. It is derived from carotenoid precursors, which can delay seed germination and promote seed dormancy. ABA levels increase when plants are subjected to certain abiotic stresses, such as water deficits, and during seed development.
The positive effect of melatonin on seed germination observed in several plant species motivated this research. The objectives of the study were to investigate (1) whether melatonin can improve germination of cotton seeds, (2) whether melatonin can improve the physiological activity of seeds, and (3) whether melatonin affects the hormones that regulate seed germination. This study aims to provide insight into the roles of melatonin in the germination of cotton seeds.
Materials and methods
Reagents
Melatonin (N-acetyl-5-methoxytryptamine) was obtained from Sigma-Aldrich (St. Louis, MO, USA). All other reagents were obtained from Sinopharm Chemical Reagent Beijing Co., Ltd. (Beijing, China). All chemicals used in all experiments were of analytical grade.
Plant material
The experiment was conducted in the Yellow River basin at Hebei Agricultural University, Baoding (38.85°N, 115.30°E), Hebei Province, China. All cotton seeds used in this study were of the ‘NDM601’ cotton cultivar. ‘NDM601’ is a cotton cultivar that is widely grown in the Yellow River Valley region of China and was developed by Hebei Agricultural University.
Germination tests
Selected cotton seeds were surface sterilized with 1% NaClO for 30 min and rinsed in distilled water five times. Fifty seeds were then placed in Petri dishes (15 × 15 cm) containing double filter paper (Whatman International Ltd., Maidstone, UK) wet with 10 mL of the different treatment solutions and incubated at 25°C in a darkened growth chamber. The following treatments were used: M0 (0 μM melatonin, i.e., distilled water only), M10 (10 μM melatonin), M20 (20 μM melatonin), M50 (50 μM melatonin), M100 (100 μM melatonin), and M200 (200 μM melatonin). Germination tests were performed with six replicates.
Seedlings were harvested at 7 days after sowing (DAS) for the determination of seedling fresh and dry weights and of seed germination rates. Germination assay samples were harvested at days 2, 4, and 6, and were stored at -80°C until the analyses of malondialdehyde (MDA) contents, antioxidant enzymes activities, and hormones were conducted.
Seed germination assessment
Seeds were considered to be germinated when the total radicle and hypocotyl length exceeded half the length of the seeds. Germination of seeds was recorded daily.
The numbers of germinated seeds on the day 3 and 7 after initiation were germination potential (GP) and germination rate (GR), respectively [30,31]. Germination index (GI) was calculated using the method developed by Wang et al. [32], i.e., GI = ∑ (Gi / Ti), where Gi is the number of germinated seeds per day corresponding to Ti, and Ti is the day of the germination test. Vigor index (VI) was calculated as VI = GI × fresh weight (FW) of germinated seeds on day 7. Mean germination time (MGT) was calculated according to the method by Ellis and Roberts [33], i.e., MGT = ∑ (NiTi) / ∑ Ni, where N is the number of seeds germinated at time i, and Ti is day of the germination test.
Measurement of SOD, POD, and MDA activities
Superoxide dismutase (SOD, EC1.15.1.1) activity was estimated based on the method by Giannopolitis and Ries [34] using the photochemical nitro blue tetrazolium chloride (NBT) method. Peroxidase (POD; EC 1.11.1.7) activity was measured at 25°C according to the method by Scebba et al. [35]. Malondialdehyde (MDA) content was determined following the method by Hodges et al. [36].
Quantification of ABA and GA3 phytohormones
GA3 and ABA concentrations were determined using an indirect ELISA technique [37]; the antibodies used in this assay were all monoclonal antibodies provided by China Agricultural University.
Statistical analysis
Analysis of variance was performed using IBM SPSS Statistics 22.0 (IBM Corp., Armonk, NY, USA). All data are reported as mean ± standard deviation (SD) values. We performed six independent replicates for each treatment. The statistical significance was considered for P-values less than 0.05 in a one-way ANOVA.
Results
Germination rate, fresh weight, mean germination time, and germination index
We conducted an extensive set of germination assays using cotton seeds to determine how different concentrations of melatonin (0–200 μM) affect seed germination. The seeds started to germinate on the second day of incubation at 25°C. Fig 1 shows the daily germination percent of each treatment within 7 days of germination and illustrates the germination speed of each treatment. As Table 1 shows, GR increased first and then decreased as melatonin concentration increased. Among the treatments with different melatonin concentrations, the 20 μM melatonin treatment displayed the maximal effect on germination promotion, but showed no significant differences with other treatments. Compared with the control group (M0), the GR of the M10, M20, and M50 treatment groups increased by 10.8%, 12.3%, and 1.5%, respectively, but did significantly differ from the control. When the melatonin concentration increased to 100 μM, the GR began to decrease. The GR and GP of the M100 treatment were significantly lower than those of the M0 group, by 12.6% and 21.7%, respectively. As the concentration of melatonin was further increased, the GR and GP significantly decreased. The GR and GP of the M200 treatment decreased by 32.2% and 36.5%, respectively. This indicates that low melatonin concentrations (i.e., treatments M10–M50) promoted the GR and GP of cotton seeds, but after a critical concentration, melatonin had a serious inhibitory effect on GR and GP. As the melatonin concentration increased, the inhibition of seed germination was enhanced further.
Treatments were performed with different melatonin concentrations.
By focusing solely on the GP of the seeds, it is clear that the M20 treatment seeds germinated well. Under the M20 treatment, the GP of the seeds was 16.7% higher than that of the M0 group and reached a significant level. During seed germination days 4–7, the GR of the M20 treatment group continued to increase but not significantly. Therefore, this data indicates that the promotion of seed germination by melatonin is likely to occur at the early stage of seed germination. Fig 2A shows the germination condition after 24 h of germination, and only three treatments (M0, M20, M200) with obvious contrasts are presented in the figure. Fig 2B shows the germination observed on the same day of the determination of GP. It can be clearly seen that M10–M200 melatonin treatments promoted the germination length of the seeds, while M100–M200 melatonin treatments did not promote or inhibit seed germination.
The GP refers to the germination speed and uniformity of seeds germinated, indicating the general vigor of the seed. Seeds with high GP values are highly active, and the resulting seedlings tend to grow uniformly and vigorously. Accordingly, VI is often used to evaluate seed quality. At day 7 of germination, VI and GI were significantly decreased (P < 0.05) while MGT was reduced in the M100 and M200 treatments. On day 7 of seed germination, we obtained the fresh weight of the seeds. The M10–M200 treatments increased the FW of the seeds, with the M20 seeds reaching a significantly higher weight. The FW of cotton seed in the M20 treatment increased by 4.81% in comparison with M0 (Fig 3).
Activity of antioxidant enzymes
In our experiment, SOD and POD activities were determined for each treated seed on days 2, 4, and 6 of germination. Fig 4A shows that the trend in SOD activity was basically uniform across each period, that is, as the concentration of melatonin increased, the content first rose and then decreased. Among the effects of the treatments, that of the M20 treatment was most prominent, but showed no significant difference from the control. On day 2, the activities of SOD under the M10 and M20 treatments were increased by 28.8% and 39.2%, respectively, and the difference was significant, compared to the activity of the M0 treatment. However, as the melatonin concentration was further increased, SOD activity decreased; when the concentration increased to that of the M200 treatment, SOD activity was reduced by 4.0% compared with the M0 treatment. By day 4 of seed germination, SOD activity did not change, but the activity of each treatment decreased, while that of the M20 treatment was still the highest and significantly different compared to the activity of the M0 treatment. The SOD activity on day 6 was the highest in the three periods measured, while the SOD activity of each treatment tended to be consistent and did not differ, with seeds under the M20 treatment still exhibiting optimal efficacy.
The trend in POD is consistent with that in SOD. By day 2 of seed germination, the POD activities of the M10 and M20 treatment groups continuously increased, by 5.1% and 17.8%, respectively, relative to the M0 treatment, but not significantly. As the melatonin concentration was continually increased, POD activity actually decreased. When the concentration was increased to that of the M200 treatment, POD activity significantly decreased by 16.8% compared with that of the M0 treatment. By day 6, the POD activity of the M20 treatment was still highest, and there was no significant difference compared with that of the M0 and M10 treatments. When the melatonin concentration was increased to that of the M50, M100, and M200 treatments, POD activity continued to decrease and reached a significant difference compared with that of the M20 treatment. The POD activity of the M200 treatment group was even less than half of that of the M20 group. Thus, the effect of the M20 treatment on POD was optimal.
Effects of melatonin on malondialdehyde content
Fig 5 shows that the degree of membrane lipid peroxidation of cotton seeds generally increased with time. On days 2, 4, and 6 of seed germination, the MDA content of the M20 treatment was the lowest, but not significantly lower than that of the other treatments. Notably, on days 2 and 4, high concentrations of melatonin caused a significant increase in MDA content. Especially on day 2, the MDA content of the M200 treatment reached 2.6 times that of the M0 treatment. At the end of the germination experiment, the MDA content of each treatment tended to be consistent, with significant differences only between the M20 and M50 treatments. Thus, the melatonin concentration of the M20 treatment minimally damaged cell membranes across the whole seed germination trial, while high concentrations of melatonin appeared to cause great damage.
Effects of melatonin on contents of phytohormones
The phytohormones ABA and GA3 are well-known regulators of seed germination. We measured the levels of these phytohormones in seeds subjected to germination trials under different concentrations of melatonin on days 2, 4, and 6 of germination.
Throughout the process of seed germination, GA3 content did not continually increase, and it peaked on day 4 of germination (Fig 6A). However, by observing the results of germination at each stage separately, we can see that the trends in GA3 content were relatively uniform across the different concentrations of melatonin, showing an initial increase followed by a decrease. On day 2 of germination, the M20 and M50 treatments showed a significant increase in GA3 content, while other concentrations were associated with different degrees of increase and decrease in GA3 content, but without reaching any significant differences. Until day 4 of germination, the GA3 content of seeds under the M10 and M20 treatments increased by 79.37% and 151.46% respectively, compared with M0. However, there were no significant differences in GA3 content for the other concentration treatments. At the end of the seed germination assay, GA3 content decreased as a whole, and the trend among the different concentrations was fairly uniform. GA3 content under the M10 and M20 treatments were still highest, while the M100 and M200 treatments exhibited significant decreases in GA3 content.
As Fig 6B shows, the ABA content of seeds gradually increased with days of germination. On day 2, the M20 treatment showed a significant decrease in ABA content, with M100 having the highest ABA content, reaching a significant level. On day 4 of seed germination, seeds under the M20 treatment still performed best. The ABA content levels under the two treatments were 33.19% and 36.32% lower, respectively, than that under the M0 treatment. There was no significant difference in ABA content between the M100 and M20 treatments, but when the concentration increased to M200, the ABA content increased sharply, and it was not different from that under the M0 treatment. On day 6 of germination, the ABA content was the highest, with only M20 and M50 treatments exhibiting a significant inhibition of ABA content. The M10, M100 and M200 treatments exhibited different degrees of increase or decrease in ABA content, but this did not reach a significant difference compared to M0.
Discussion
Current research indicates that exogenous melatonin has a variety of effects on plants and can be used to regulate plant growth and development. For example, melatonin can promote the growth of lateral roots [38] and slow the senescence of plant stems and leaves [39]. In addition, melatonin also improves the resistance of plants to drought [40], salt damage [41], high temperatures [42], cold damage [43], and other adverse conditions, and it can protect cell structural substances and biological macromolecules, such as proteins, from oxidation damage [44, 45]. Melatonin can promote the growth of plants and affect the morphological development of plants. Hernánde et al. [18] found that treatment of etiolated lupins (Lupinus albus) with melatonin promoted hypocotyl growth. Wen et al.[46] investigated the effects of melatonin on adventitious root formation of de-rooted tomato seedlings and observed the occurrence of adventitious roots in the treated seedlings. The induction of adventitious roots in tomato was related to the melatonin concentration of the treatment. The concentration of 50 μM exogenous melatonin was optimal for promoting adventitious root emergence in tomato seedlings.
Our experiments assessed GR, GP, GI, VI, MGT, and FW in order to accurately evaluate the germination vigor and quality of cotton seeds. GP is used to assess germination speed and uniformity. The higher the value, the stronger the germination potential is, which is one of the key indicators of seed quality. After the cotton seeds in the experiment were treated with different concentrations of melatonin, the GP of melatonin-treated seeds at concentrations of 10–50 μM was improved compared with the control group, with the 20 μM melatonin treatment performing significantly better. In contrast, treatment with 100–200 μM melatonin significantly inhibited GP. Our study revealed that high melatonin concentrations (i.e., 100–200 μM) significantly inhibited the GR of cotton seeds (Table 1).
GI indicates the germination speed, and the larger the value, the faster the germination speed [47]. The germination test found that treatments with 10–50 μM melatonin promoted the increase of GI. Similarly, M20 still performed best. M100 and M200 significantly reduced GI and reached a highly significant level (Fig 3A). However, VI is a better indicator of the subsequent growth of seedlings than is GR. The 10–50 μM melatonin treatments increased the VI compared with the M0 treatment, but not significantly, and the 100–200 μM treatments significantly inhibited the VI (Fig 3B). These results indicate that high concentrations of melatonin are likely to have irreversible effects on cotton seeds and even affect the growth of seedlings at later stages. Our test also uses MGT as an indicator to measure seed germination. The lower the MGT value, the faster a population of seeds has germinated [48]. The 10–50 μM melatonin treatments had little effect on MGT, and M100 and M200 can significantly increase MGT (Fig 3D). This indicator further validates the above conclusions. Our findings are broadly consistent with those of Simlat et al. [49], who reported that the lowest melatonin concentrations examined (5 and 20 μM) exerted a significantly positive effect on Stevia seed germination compared with the 100 and 500 μM treatments. Previous studies have found that melatonin application significantly increased osmopriming effects, such that 50 μM melatonin achieved maximal results [43]. Similar positive effects of melatonin treatment have been reported for red cabbage seeds [50]. However, another study indicated that melatonin had no effect on the germination of cucumber seeds regardless of germination conditions [51].
The germination of seeds begins with their swelling and water absorption. Accordingly, moisture conditions, a precondition for seed germination, have a significant effect on seed germination. Seeds can only germinate after absorbing a certain amount of water, which is important for the growth of the resulting seedlings. The seeds of different types of plants have different water absorption and germination requirements. FW can directly reflect the water absorption of the seed and the accumulation of biomass. Bajwa et al. [52] reported that the application of low concentrations (10–40 μM) of melatonin increased the FW of Arabidopsis compared with high-concentration (200–400 μM) applications. Our results showed that melatonin (10–200 μM) can increase the FW of the seeds, with the 20 μM melatonin treatment having the strongest effect and also reaching a significant level (Fig 3C). This result indicates that 20 μM melatonin promotes the water absorption or water absorption rate during seed germination and thus promotes the accumulation of biomass inside seeds, and the inhibitory effect of high concentrations of melatonin on FW was not observed in our study, probably because the highest melatonin concentration examined was insufficient to elicit this response.
As a byproduct of aerobic metabolism [53, 54], reactive oxygen species (ROS) exist in the form of non-free radicals, including hydrogen peroxide (H2O2), and free radical forms, such as O2•−. The antioxidant system formed during plant evolution contributes to the balance of active oxygen metabolism. The antioxidant defense system includes the enzymatic system and non-enzymatic system. SOD and POD are essential antioxidant enzymes that can effectively eliminate superfluous ROS, such as H2O2, hydroxyl, and superoxide anions, from plant cells [55, 56]. SOD can catalyze the disproportionation of two superoxide anion radicals to form O2 and H2O2, while H2O2 is further decomposed by other antioxidant enzymes such as catalase.
Melatonin and its metabolites are endogenous free radical scavengers, broad-spectrum antioxidants, and H2O2 scavengers. Melatonin can scavenge reactive oxygen species by donating electrons and can also affect some oxidative and antioxidant enzymes in cells and tissues through its receptors, for example, by enhancing SOD and POD levels, which act to scavenge free radicals. Among antioxidants, SOD is a particularly active substance in the living body, where it eliminates harmful substances generated by plant metabolism. It is important to determine whether melatonin can also reduce the inhibition of seed germination by ROS [57, 58]. Our study found that different concentrations of melatonin have effects that include low concentration promotion and high concentration inhibition of SOD and POD activity during seed germination, and the peak activity of both occurred under the 20 μM treatment (Fig 4). This finding suggests that low concentrations of melatonin increase the activity of antioxidant enzymes, including SOD and POD, and exogenous applications of melatonin appear to play a role in the first line of defense against oxidative stress. However, there are studies that offer the opposite conclusion; Shi et al. [59] and Shi et al. [60] found no significant effects of melatonin on antioxidant enzyme activity under controlled conditions. Other researchers have found that melatonin not only directly eliminates ROS, but also upregulates the activity of various antioxidant enzymes [61]. This was in accord with observations in the current study.
Plant damage is closely related to membrane lipid peroxidation induced by reactive oxygen species accumulation. The accumulation of ROS and free radicals in organisms often leads to membrane lipid peroxidation and causes metabolic disorders. The integrity of cell structure is the basis of seed vigor, so once the cell membrane system is destroyed, leakage increases throughout the progression of germination. MDA is a product of lipid peroxidation, so it represents the level of lipid peroxidation and the degree of membrane damage in cells. The MDA content under the 20 μM melatonin treatment was the lowest, but not significantly, while the high-concentration (100–200 μM) treatments significantly increased the MDA content (Fig 5). This indicates that low concentrations of melatonin can alleviate peroxidative stress during seed germination but that it can still have a negative effect at high concentrations.
Seed germination, as the beginning of the agricultural cycle from the perspective of the plant, is the first stage of crop growth. Hormones inside the seed control the germination of seeds [62]. For example, ethylene and gibberellin weaken the seed coat and break seed dormancy to promote seed germination [63]. Numerous studies have shown that melatonin has synergistic and antagonistic relationships with various other plant hormones, for example, promoting plant root and young leaf growth at low concentrations, which is similar in action to IAA [64].
There are few studies on the effects of melatonin treatment on gibberellin content. Under salt stress, melatonin treatment of cucumber seedlings can upregulate the expression of GA biosynthesis genes and increase the content of active GAs such as GA3 and GA4, thus promoting subsequent germination processes under salt stress [65, 66]. The present study shows that although changes in GA3 content may slightly differ among the days of seed germination, both 10 μM and 20 μM melatonin treatments, especially the latter, can significantly increase the GA content of seeds. Compared with the control treatment, melatonin had no effect on GA3 content and even inhibited it at concentrations of 50–200 μM. At present, there are few studies on the effects of melatonin treatment on gibberellin content (Fig 6A). However, melatonin treatment has been reported to increase the content of active GAs such as GA3 and GA4 in cucumber seedlings, thus promoting the germination process under salt stress inhibition [65, 67].
ABA is the most important plant hormone regulating seed dormancy and germination [63]. It induces and maintains seed dormancy, inhibits seed germination and regulates seedling growth and development. Melatonin treatment can induce decreases in ABA level during seed germination under salt stress by inducing upregulation of ABA catabolic genes and downregulation of ABA biosynthesis genes [65]. In heat-induced senescence of the perennial ryegrass (Lolium perenne L.) leaves, exogenous melatonin treatment reduced ABA content and delayed its aging process [68]. In our study, we found that low concentrations of melatonin inhibited ABA content, while 100–200 μM melatonin treatments promoted ABA content in seeds, but not significantly (Fig 6B).
Conclusions
The present study demonstrates the positive effects of melatonin on seed germination in cotton. Low concentrations of melatonin (10–50 μM) had a positive effect on cotton seed germination compared with high concentrations (100–200 μM), of which 20 μM melatonin was the optimal treatment. This concentration also resulted in low levels of MDA concentration as well as high SOD and POD activity. Additionally, melatonin may promote seed germination by regulating the endogenous synthesis of phytohormones, as the hormone content of seeds treated with low concentrations of melatonin, which promoted seed germination, also showed a corresponding pattern, in which the 20 μM melatonin treatment achieved the best germination and significantly increased GA3 content and reduced ABA content. Correspondingly, high concentrations of melatonin generally showed no effect or even inhibited germination somewhat.
Acknowledgments
The authors are grateful to the anonymous reviewers for their valuable comments and suggestions. We would like to thank Yan-dan Bai, Xiang-ming Huang for their assistance with the experiment.
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