Structurally Different Exogenic Brassinosteroids Protect Plants under Polymetallic Pollution via Structure-Specific Changes in Metabolism and Balance of Cell-Protective Components
by
,
Ilya E. Zlobin
1,2,
Elena D. Danilova
1,
Ol’ga K. Murgan
1,
Liliya V. Kolomeichuk
1,
Raisa P. Litvinovskaya
3,
Alina L. Sauchuk
3,
Vladimir V. Kuznetsov
1,2,* and 
Marina V. Efimova
1,* 1
Department of Plant Physiology, Biotechnology and Bioinformatics, Biological Institute, National Research Tomsk State University, Lenin Avenue 36, Tomsk 634050, Russia
2
K.A. Timiryazev Institute of Plant Physiology, Russian Academy of Sciences, Botanicheskaya Street 35, Moscow 127276, Russia
3
Institute of Bioorganic Chemistry, National Academy of Sciences of Belarus, Kuprevich Street 5/2, 220084 Minsk, Belarus
*
Authors to whom correspondence should be addressed.
Molecules 2023, 28(5), 2077; https://doi.org/10.3390/molecules28052077
Submission received: 16 January 2023
/
Revised: 8 February 2023
/
Accepted: 20 February 2023
/
Published: 22 February 2023
(This article belongs to the Special Issue Analysis of Phytochemical Components)
Abstract
:Heavy metals and aluminum are among the most significant abiotic factors that reduce the productivity and quality of crops in acidic and contaminated soils. The protective effects of brassinosteroids containing lactone are relatively well-studied under heavy metal stress, but the effects of brassinosteroids containing ketone are almost unstudied. Moreover, there are almost no data in the literature on the protective role of these hormones under polymetallic stress. The aim of our study was to compare the stress-protective effects of lactone-containing (homobrassinolide) and ketone-containing (homocastasterone) brassinosteroids on the barley plant’s resistance to polymetallic stress. Barley plants were grown under hydroponic conditions; brassinosteroids, increased concentrations of heavy metals (Mn, Ni, Cu, Zn, Cd, and Pb), and Al were added to the nutrient medium. It was found that homocastasterone was more effective than homobrassinolide in mitigating the negative effects of stress on plant growth. Both brassinosteroids had no significant effect on the antioxidant system of plants. Both homobrassinolide and homocastron equally reduced the accumulation of toxic metals (except for Cd) in plant biomass. Both hormones improved Mg nutrition of plants treated with metal stress, but the positive effect on the content of photosynthetic pigments was observed only for homocastasterone and not for homobrassinolide. In conclusion, the protective effect of homocastasterone was more prominent compared to homobrassinolide, but the biological mechanisms of this difference remain to be elucidated.
1. Introduction
Heavy metals and aluminum are among the most significant abiotic factors that reduce the productivity and quality of crops around the world [1,2,3,4]. The excessive content of mobile forms of aluminum, manganese, and a number of other heavy metals is an inherent property of acidic soils, covering about 30–40% of all arable land, and is one of the most important stress factors for plants on such soils [5,6,7,8,9]. In addition, hundreds of thousands of sites around the world are contaminated with heavy metals as a result of anthropogenic emissions [1]. To date, acid depositions and the use of nitrogen fertilizers result in the expansion of acidic areas [5], while the input of heavy metals into agricultural soils continues as a result of industrial activities and the usage of fertilizers, pesticides, etc. [4]. Thus, the importance of the negative effects of heavy metals and aluminum on plants will likely increase in the future [9].
The polygenic nature of traits linked with plant resistance to heavy metals and with the regulation of their uptake makes difficult the use of breeding or genetic engineering methods to obtain heavy metal-resistant plants, and therefore, the use of growth regulators to control the uptake and resistance of plants to heavy metals is of considerable interest [3]. Brassinosteroids are a group of plant hormones that can increase plant resistance to a wide range of adverse environmental factors. A significant number of studies show that brassinosteroids are able to improve the growth and functional state of plants under conditions of metal-induced stress [10,11]. Moreover, the specific feature of brassinosteroids is their ability to significantly limit the accumulation of heavy metals by plants [3,12]. At the same time, a number of studies have also revealed a negative effect of brassinosteroids on the resistance of plants to heavy metals [2,13]. On the other hand, a number of studies have also found negative effects of brassinosteroids on plant resistance to heavy metals [2,13]. The effects of brassinosteroids on plant resistance to metal-induced stress can strongly depend on the plant developmental stage, experimental conditions, metal species, types, and active concentrations of brassinosteroids used, etc. [2,7,13]. However, the question of whether the chemical structure of brassinosteroids affects the protective responses of plants to heavy metal stress remains open. The most studied brassinosteroids, namely, brassinolide, 24-epibrassinolide and 28-homobrassinolide, possess a lactone structure of the B cycle of the steroid backbone and represent the final link in the biosynthetic chain having high phytohormonal activity. The biological activities of 6-keto brassinosteroids, such as 24-epicastasterone and 28-homocastasterone, which are biogenetic precursors of lactones, are much less studied. Comparative data on the mechanisms of the stress-protective action of ketone- and lactone-containing steroid compounds are virtually absent [14,15].
In this regard, we aimed to compare the effects and stress-protective mechanisms of lactone-containing (homobrassinolide, HBL) and ketone-containing (homocastasterone, HCS) brassinosteroids (Figure 1) on the resistance of barley plants to the polymetallic stress. Barley is highly resistant to various abiotic stressors, but it is sensitive to acidic soils and increases the availability of ions of heavy metals and aluminum in the soil solution [5].
The following tasks were set:
- -
- To compare the effects of different methods of HBL and HCS application on the morphological parameters of barley plants under polymetallic stress;
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- To study the influence of brassinosteroids on the photosynthetic apparatus and the antioxidant system of plants;
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- To study how hormones influence the accumulation of toxic and essential elements in the roots and shoots of barley plants and the functioning of some systems of detoxification of excessive elements;
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- To reveal the effect of polymetallic stress on the accumulation of endogenous B-lactones and B-ketones.
2. Results
2.1. Plant Growth and Morphology
The nutrient medium used to grow plants was characterized by a low pH content, low ionic strength, and a concentration of phosphate ions, thus mimicking the composition of the soil solution (Table 1) [16,17]. As a result, even quite moderate excessive concentrations of heavy metals and aluminum resulted in a substantial reduction in plant growth (Figure 2, Supplementary Materials Table S1). The root growth was the most sensitive parameter, decreasing by 38%; the leaf area decreased by 21%; and the stem length decreased by 15%, all of which resulted in a 26% decrease in the fresh weight of plants. HCS had a pronounced protective effect on plant growth (Figure 2, Table S1) at high HCS concentrations (10 nM) regardless of exposure time. Compared with BS-untreated stress-exposed plants, plants treated with a high concentration (10 nM, regardless of exposure time) of HCS had increased leaf area and total weight, and the length of the stem and root increased under exposure to both low (0.1 nM) and high (10 nM) HCS, regardless of exposure time. The protective effect of HBL was less prominent. Under prolonged (10 days) treatment, both low (0.1 nM) and high (10 nM) HBL concentrations increased total leaf area, whereas stem length was increased only by exposure to high HBL concentrations. The difference in protective effects of HBL and HCS at the same concentration and exposure time could be due to their different bioavailability caused by chemical structure. Therefore, for further analysis, we chose to compare the effects of treatment with HBL and HCS for 10 days at a 10 nM concentration.
2.2. Plant Photosynthetic Apparatus
Primary photosynthetic processes were found to be highly resistant to polymetallic stress, with no significant suppression of any parameters studied. The action of brassinosteroids did not influence the photosystem II functioning (Figure 3, Table S2). However, the polymetallic stress clearly impacted the pigment apparatus of barley plants, decreasing the contents of chl a and chl b, correspondingly, by 70 and 68% and the carotenoid content by 58% from control (Figure 3, Table S3). HBL treatment had almost no influence on the pigment contents, whereas HCS treatment increased the contents of chl a, chl b and carotenoids, correspondingly, to 52%, 46%, and 64% from the control level.
2.3. Oxidative Stress and Antioxidant Enzymes
Under the action of polymetallic stress, the content of TBARS increased substantially by 2.37 times in barley roots, whereas no significant effects were observed in the shoots (Figure 4, Table S4). Brassinosteroids exerted differently directed changes in the TBARS content. HBL decreased the TBARS content in the roots of stressed plants, whereas the shoots’ TBARS content was increased. Treatment with HCS increased the TBARS content in barley roots.
Both polymetallic stress and treatment with brassinosteroids influenced the SOD activity neither in the roots nor in the shoots of barley plants (Figure 4, Table S4). POD activity increased in the roots of stressed plants by 2.36 times, and were unchanged in the shoots (Figure 4, Table S4). HCS treatment did not influence the POD activity, whereas HBL induced a more than two-fold increase in the POD activity in the barley roots and shoots compared to the levels in stressed plants.
2.4. Accumulation of Mineral Elements
As expected, the conditions of polymetallic stress induced the substantial increase in the contents of all excessive elements in barley roots and shoots. For Ni, Zn, Cu, and Pb, the accumulation was substantially more prominent in the roots than in the shoots (Figure 5 and Figure 6, Tables S5 and S6). The extent of metal accumulation was close in the roots and shoots for Mn (by 16.08 and 9.44 times, respectively) and for Cd (by 170 and 256 times, respectively) (Figure 5 and Figure 6, Tables S5 and S6). Paradoxically, aluminum was found in substantial concentrations in the organs of control plants; therefore, the measurement of aluminum was likely unreliable. Translocation factors, which are the ratio between shoot and root element contents, decreased in metal-stressed plants for all excessive metals except for Cd, for which the translocation factor increased 1.57 times.
Both brassinosteroids induced the significant decrease in the root contents of all excessive metals except for Cd, for which the effects of hormones were non-significant. The extent of the decrease was similar for both brassinosteroids. In shoots, both HBL and HCS induced the significant decrease in Cd and Zn accumulation, whereas HCS was only effective in decreasing the Mn and Ni accumulation (Figure 5 and Figure 6, Table S6). For Pb accumulation in the shoot, no effect of HCS was observed, whereas HBL induced the increase in the Pb accumulation in the shoot. Both brassinosteroids did not influence the translocation factors of metals substantially compared to the action of polymetallic stress only.
Compared to the excessive elements, changes in the contents of the remaining elements under polymetallic stress were less prominent. Polymetallic stress induced an increase in the root contents and a decrease in the shoot contents of Na, P, and K, and both brassinosteroids increased Na accumulation in both the roots and shoots. For Mg, polymetallic stress induced the uniform decrease in both the roots and shoots, and brassinosteroids increased the Mg content in both organs.
2.5. Expression of Genes of Metal Detoxification
The action of polymetallic stress induced relatively little changes in the expression of all genes studied. The only gene for which more than two-fold changes were observed was ALMT, which increased 4.73 times in the roots and decreased by 55% in the shoots of stressed plants (Figure 7A,B, Table S7). HBL did not exerted significant effects on gene expression in roots, while it increased the expression of all genes in the shoots compared to the levels in stressed plants (Figure 7A,B, Table S7). HCS decreased the expression of the studied genes in both the roots and shoots.
2.6. Accumulation of Endogenous Brassinosteroids
Polymetallic stress did not induce the significant changes in the contents of B-lactones, neither in the roots nor in the shoots of barley plants. The contents of B-ketones remained unchanged in roots, whereas in shoots, a significant 1,9-fold increase was observed compared to control plants (Figure 8, Table S8).
3. Discussion
Brassinosteroids are well-known to exert protective effects on plants threated by heavy metal stress; however, among numerous members of this class, 24-epibrassinolide is by far the most studied protector that forms heavy metal stress, whereas stress-protective effects of other brassinosteroids, including ketone-containing ones, are rarely studied [18]. We observed that HCS exerted a substantial protective effect on the elongation of the roots and shoots of barley plants regardless of the concentrations and exposure time, and at high concentrations (10 nM), it also increased the leaf area and total plant weight. The protective effect of HBL was substantially lower than that of HCS and was generally observed only under a long exposure time (10 days).
The most well-known protective effect of brassinosteroid is their stimulation of a plant’s antioxidative system, and this effect is considered to be the most important component of the protective effects of brassinosteroids under heavy metal stress [3,10,18,19,20]. The stimulating effect of brassinosteroids on the antioxidative system of plants and the resulting decrease in oxidative stress under heavy metal treatment were found in several studies [10,20,21]. However, we did not observe the consistent positive effect of brassinosteroids on the antioxidative system of barley plants (Figure 4, Table S4). SOD activity was unchanged under polymetallic stress and action of brassinosteroids, whereas POD activity increased under HBL but not under HCS action. The TBARS content was decreased in the roots but increased in the shoots of HBL-treated plants, whereas HCS action increased the root TBARS content. The functioning of the photosystem II, which is well-known for its sensitivity to oxidative damage [22], was not impaired by polymetallic stress and not influenced by hormones (Figure 3, Table S2). At the same time, we should keep in mind that HCS had a greater protective effect on the carotenoid content under polymetallic stress than HBL. As is known, carotenoids are considered effective quenchers of singlet oxygen (1O2) and triplet Chls through a physical mechanism that involves the transfer of excitation energy leading to thermal deactivation. Additionally, leaf carotenoids can quench 1O2 by a chemical mechanism involving their oxidation [23].
To sum up, the positive effects of brassinosteroids were not due to the stimulation of the antioxidative system.
The other possible protective effect of brassinosteroids is their influence on the accumulation of toxic elements (Figure 5 and Figure 6, Tables S5 and S6). It was previously shown that the application of 24-epibrassinolide to B. juncea L. cv PBR 91 seedlings eliminated the negative effects of heavy metals, such as Zn, Mn, Co, and Ni, improved growth, and reduced the accumulation and absorption of metals [24]. Indeed, brassinosteroids decreased the root accumulation of all excessive metals except for Cd. In shoots, both hormones decreased Cd and Zn accumulation, and HCS additionally decreased Mn and Ni accumulation. In other experiments, the application of HBL regulated Mn uptake and growth of B. juncea L. [25] and was involved in GSH metabolism and redox status against Zn toxicity in R. sativus seedlings [26]. According to the data obtained, the protective effect of both hormones was not due to the restriction of metal transported to the aboveground part, since the hormones did not substantially influence translocation factors. The effect of both HBL and HCS on the accumulation of excessive metals was quite similar; therefore, it is unlikely that the more pronounced protective effect of HCS on plant growth was due to its better ability to decrease the accumulation of toxic metals compared to HBL. One of the ways that the accumulation of toxic elements can be decreased is via the activation of systems involved in the transport and detoxification of these elements, but we did not observe the prominent stimulating effect of brassinosteroids on the expression of selected genes involved in metal tolerance (Figure 7A,B, Table S7). On the contrary, HCS decreased the expression of all the genes studied. Therefore, the brassinosteroid-induced decrease in metal accumulation in barley plants was not due to the regulation of the expression of the studied genes.
Considering non-excessive essential elements, the most prominent positive effect exerted by brassinosteroids was the alleviation of the stress-induced decrease in Mg contents, which was complete in the roots, but only partial in the shoots (Figure 5, Tables S5 and S6). It is well-known that a Mg deficit leads to a decrease in chlorophyll biosynthesis and therefore to chlorosis [27]. However, it is unlikely that the improved Mg nutrition underlay the HCS-induced increase in the chlorophyll content, since both HCS and HBL induced similar increases in the shoot Mg content, whereas the increase in the chlorophyll content was prominent for HCS but not for HBL (Figure 3, Table S3).
In conclusion, the protective effect of HCS under the conditions of polymetallic stress was substantially more prominent compared to HBL. The difference between these compounds was neither due to differences in their effects on the antioxidative system nor due to different effects on the accumulation of excessive and essential elements in roots and shoots.
The difference in activity of these two steroid phytohormones could be explained by a specific set of regulating factors for each, which, when acting together, are responsible for the resulting effect. Being dependent on the chemical structure, some molecular characteristics are influenced, and this is expressed in obvious changes in biosynthetic processes, membrane permeability, enzyme activity, and ion transport. At least some of these clearly observed phenomena could be connected with a different affinity of the hormones for the BS-receptor. Another important result pointing to a possible reason for the higher activity of B-ketosteroid hormone compared to B-lactone is our finding a significant activation of BS-ketones biosynthesis under stress, which may be an indication of their protective role under these conditions.
Our results indicate that homocastasterone was more effective than homobrassinolide in mitigating the negative effects of polymetallic stress on plant growth. Both brassinosteroids had no significant effect on the antioxidant system of plants. Both homobrassinolide and homocastron equally reduced the accumulation of toxic metals (except for Cd) in plant biomass. Both hormones improved the Mg nutrition of plants that were treated with metal stress, but the positive effect on the content of photosynthetic pigments, including carotenoids, was observed only for homocastasterone and not for homobrassinolide. However, solving the question of what the molecular mechanisms are the influence of the chemical structure of different groups of brassinosteroids on the plant’s tolerance to polymetallic stress requires further investigation.
4. Materials and Methods
The studies were performed on barley plants (Hordeum vulgare L.) cv. Biom. Plants were grown in climatic chamber in mixture of soil and perlite for 5 days at a temperature of 19 ± 2 °C, a relative humidity of 50–60%, and a PAR quantum flux density of 200–250 μmol × m2 × s–1 with a 16 h photoperiod. Then, for 5 days, the plants were adapted to a liquid nutrient medium according to Blamey et al. [16], with pH 4.5. This nutrient medium is characterized by low pH level, low phosphate content, and low ionic strength, and most fully corresponds to the real soil composition of acidified and polluted areas, on which the availability of metals for plants is increased. After the 5 days adaptation period, the experimental period began. Two independent experiments were performed.
In the first experiment, growth parameters of barley plants were analyzed. The experiment lasted for 10 days. The following experimental variants were used:
- Control variant with the standard nutrient medium.
- Polymetallic stress by the addition of excessive metal ions to the medium. The effective concentrations of heavy metals (Mn2+, Cd2+, Cu2+, Ni2+, Zn2+, and Pb2+) and aluminum (Al3+) were selected on the basis of the typical concentrations of these ions in soil solutions of industrially polluted acidic soils [1,17] and on the basis of the results of our previous experiments [28,29], see Table 1.
- Pretreatment with 0.1 nM HBL for 1 day by addition to the nutrient medium with the following 10-day polymetallic stress.
- Pretreatment with 10 nM HBL for 1 day with the following 10-day polymetallic stress.
- Pretreatment with 0.1 nM HCS for 1 day with the following 10-day polymetallic stress.
- Pretreatment with 10 nM HCS for 1 day with the following 10-day polymetallic stress.
- Simultaneous treatment with 0.1 nM HBL added to the nutrient medium and with polymetallic stress.
- Simultaneous treatment with 10 nM HBL and with polymetallic stress.
- Simultaneous treatment with 0.1 nM HCS and with polymetallic stress.
- Simultaneous treatment with 10 nM HCS and with polymetallic stress.
Based on the results of first experiment, the second experiment was performed. Only four experimental variants were used:
- Control variant with the standard nutrient medium.
- Polymetallic stress by the addition of excessive metal ions to the medium.
- Simultaneous treatment with 10 nM HBL was added to the nutrient medium and polymetallic stress.
- Simultaneous treatment with 10 nM HCS was added to the nutrient medium and polymetallic stress.
The biological material from the second experiment was used for the analysis of plant photosynthetic processes for biochemical and molecular analyses. Photosynthetic activity was determined on intact leaves. For biochemical analyses, root and shoot samples were fixed in liquid nitrogen and freeze-dried under vacuum using a VirTis 6211 sublimation chamber (LabX, Midland, ON, Canada). For RNA isolation, root and shoot samples were fixed in liquid nitrogen at −70 °C.
4.1. Physiological and Biochemical Analyses
4.1.1. Determination of Growth Parameters
Root and shoot length, total leaf surface area, and fresh plant biomass were determined. Total leaf surface area was calculated using the Anikeev and Kutuzov formula [30]. Fresh biomass was determined using analytical balance (Sartorius, Goettingen, Germany).
4.1.2. Determination of the Lipid Peroxidation Level
The extent of lipid peroxidation was evaluated by the formation of a colored complex between thiobarbituric acid and thiobarbituric acid-reactive substances (TBARS) upon heating [31]. TBARS content was determined spectrophotometrically using a Genesys 10S UV–Vis Genes spectrophotometer (ThermoScientific, Waltham, MA, USA) at wavelengths of 532 and 600 nm.
4.1.3. Determination of the Photosynthetic Pigments Content
To determine the content of photosynthetic pigments, a sample of leaves (15 mg) was ground in 96% ethanol, and the homogenate was centrifuged for 10 min at 8000 rpm using a MiniSpin centrifuge (Eppendorf, Hamburg, Germany). The optical density of the alcoholic extract (final volume of the solution was 1.5 mL) was measured using a Genesys 10S UV–Vis spectrophotometer (ThermoScientific, Waltham, MA, USA) at 470.0, 648.6, 664.2, and 720.0 nm. The pigment concentration in the alcoholic extract was calculated according to Lichtenthaler [32].
4.1.4. Determination of Photosynthetic Activity
The photochemical activity of plants was measured on a PAM fluorimeter (Mini-PAM II, Heinz-Walz, Effeltrich, Germany). Before measurement, the samples were adapted to darkness for 20 min. Then, the light was switched for 10 min (I = 190 μmol photons m−2 s−1 PAR). The intensity of the saturating light was 6000 μmol photons m−2 s−1. Saturating pulses were generated every 30 s. Maximal (Fv/Fm) and effective (Y(II)) quantum yields of PSII photochemistry, coefficients of photochemical quenching based on the “lake” model (qL) and the “puddle” model (qP), electron transport rate (ETR), and quantum yields of nonregulated (Y(NO)) and regulated (Y(NPQ)) energy dissipation were calculated using Junior-PAM software WinControl-3.
4.1.5. Determination of the Activity of Antioxidant Enzymes
Total superoxide dismutase (SOD, EC 1.15.1.1) and peroxidase (POD, EC 1.11.1.7) activities were determined in crude extracts of leaf tissues. Leaf samples were ground in liquid nitrogen with insoluble polyvinyl pyrrolidone, extracted in 0.066 M potassium phosphate buffer (pH 7.4) containing 0.5 mM dithiothreitol, and 0.1 mM phenylmethylsulfonyl fluoride in dimethyl sulfoxide, and then centrifuged for 20 min at 8000 rpm and 4 °C using a 5430R centrifuge (Eppendorf, Germany). The1 total SOD activity was determined according to Beauchamp and Fridovich [33]. The reaction medium (2 mL) contained 10 μL of supernatant, 1.75 mL of 50 mM Tris-HCl buffer (pH 7.8), 0.2 mL of 0.1 M DL-methionine, 0.063 mL of 1.7 mM Nitro Blue tetrazolium (Fermentas, Waltham, Massachusetts, USA), 0.047 mL of 1% Triton X-100, and 0.060 mL of 0.004% riboflavin. The reaction proceeded under LED lamps (I = 232 μmol photons/m−2 s−1) for 30 min. Absorption was measured at 560 nm using a Genesys 10S UV–Vis spectrophotometer (Thermo Scientific, Waltham, MA, USA). Peroxidase activity was determined as previously described [34]. The reaction mixture contained 50 μL of supernatant, 1.95 mL of 0.066 M potassium phosphate buffer (pH 7.4), 200 μL of 7 mM guaiacol, and 250 μL of 0.01 M H2O2. Absorption was measured at 470 nm using a Genesys 10S UV–Vis spectrophotometer (ThermoScientific, Waltham, MA, USA). The protein content in the samples was determined according to Esen [35].
4.2. Analysis of Elemental Composition of Shoots and Roots
The shoot and root samples were digested in glass tubes with solutions of concentrated HNO3 and HClO4 (2:1 v/v) for 24 h at room temperature and then incubated in a dry block thermostat at 150 °C for 1.5 h and then at 180 °C for 2 h. To desorb metal ions form the apoplast, roots were rinsed in 2 mM CaCl2 before digestion. Analysis of the contents of several elements (Na, Mg, Al, P, K, Ca, Mn, Ni, Cu, Cd, Pb, and Zn) in roots and leaves of barley plants was performed by inductively coupled plasma mass spectrometry (ICP-MS), Agilent 7900, Santa Clara, CA, USA.
4.2.1. Determination of the Endogenous Content of Brassinosteroids
4.2.2. RNA Isolation and cDNA Synthesis
Leaf samples were grinded in liquid nitrogen, and RNA was extracted using TRIzol reagent (Invitrogen, Waltham, MA, USA), according to manufacturer’s instructions (http://www.invitrogen.com, accessed on 14 January 2023). Sample contamination with genomic DNA was prevented using DNase I, RNase-free (Thermo Fisher Scientific, USA). Complementary DNA was synthetized with MMLV-RevertAid reverse transcriptase (Thermo Fisher Scientific, USA), using oligo-dT21primer (Evrogen, Moscow, Russia).
4.2.3. Identification of Candidate PCR Reference and Target Genes and Primer Design
Levels of gene transcript content were determined by real-time PCR on LightCycler®96 System (Roche, Basel, Switzerland), using SYBR Green I (Eurogen, Moscow, Russia). The reaction mixture contained qPCRmix HS SYBR (Eurogen, Russia), cDNA, PCR primers, and ddH2O. Each sample was treated in 3 technical replicates, and ddH2O was used as a negative control. Gene-specific primers were selected using Primer-BLAST (https://www.ncbi.nlm.nih.gov/tools/primer-blast/, accessed on 14 January 2023) and Vector NTI 11. The description of genes of interest, primer sequences, amplicone length, and melting temperature are present in Table 2. The following amplification program was used: 95 °C for 5 min, then 40 cycles of 95 °C for 15 s, Tm °C for 30 s, and 72 °C for 15 s. The effectiveness of each primer pair was determined using standard curve, using the serial 10-fold dilution of mixture of cDNA samples. The transcript levels of the genes of interest were normalized to the expression of the Actin gene and HvGAPDH gene. Transcript amount was calculated according to manufacturer’s instruction using MS Excel.
4.3. Statistical Analysis
Each experiment was repeated in at least three biological replicates. The number of plants per biological replicate ranged from 55 to 60. The figures and tables present the mean values and their standard errors (SE). The means were compared with control values at corresponding time points using Student’s t-test. Asterisks (*) indicate significant differences from the control variant, and a letters indicate significant differences from the polymetallic stress-treated variant (p < 0.05).
Supplementary Materials
The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/molecules28052077/s1, Table S1: The effects of heavy metal stress and treatment with brassinosteroids on the growth parameters of barley plants; Table S2: The effects of heavy metal stress and treatment with brassinosteroids on the primary photosynthetic processes in barley plants; Table S3: The effects of heavy metal stress and treatment with brassinosteroids on concentrations of photosynthetic pigments (mg/g fresh weight) in barley plants; Table S4: The effects of heavy metal stress and treatment with brassinosteroids on the content of TBARS and activity of antioxidant enzymes–SOD and POD in barley plants; Table S5: The effects of heavy metal stress and treatment with brassinosteroids on the elemental content (μg/g dry weight) and translocation factors in roots of barley plants; Table S6: The effects of heavy metal stress and treatment with brassinosteroids on the elemental content (μg/g dry weight) and translocation factors in shoots of barley plants; Table S7: The effects of heavy metal stress and treatment with brassinosteroids on the expression of genes involved in metal detoxification in barley plants; Table S8: effects of heavy metal stress on brassinosteroids content (ng/g dry weight) in roots and shoots of barley plants.
Author Contributions
Conceptualization, V.V.K. and M.V.E.; methodology, I.E.Z.; software, O.K.M.; validation, L.V.K., formal ELISA and data curation, R.P.L. and A.L.S.; writing—original draft preparation, E.D.D. and M.V.E.; writing—review and editing, I.E.Z. and M.V.E.; visualization, O.K.M.; supervision, M.V.E.; project administration, M.V.E. and V.V.K.; funding acquisition, V.V.K. All authors have read and agreed to the published version of the manuscript.
Funding
Analysis of elemental composition and expression of genes of metal detoxification were supported by the Tomsk State University Development program (Priority-2030; project no. 2.1.2.22). Physiological analyses were supported by the Russian Science Foundation (project no. 23-44-10019). Analysis of primary photosynthetic processes was supported by the Ministry of Science and Higher Education of the Russian Federation (project No. 122042700044-6). Determination of the endogenous content of brassinosteroids was performed with the financial support by the Belarusian Republican Foundation for Fundamental Research (project no. X23RSF-087).
Institutional Review Board Statement
Not applicable.
Informed Consent Statement
This article does not contain any research involving humans and animals as research objects.
Data Availability Statement
The data supporting the findings of this study are available within the article its Supplementary Materials.
Conflicts of Interest
The authors declare no conflict of interest.
Sample Availability
Samples of the brassinosteroid compounds were synthesized in the Laboratory of Steroid Chemistry of the Institute of Bioorganic Chemistry.
Abbreviations
| BS | brassinosteroid |
| ETR | electron transport rate |
| Fv/Fm | maximal quantum yields of PSII |
| HBL | 28-homobrassinolide |
| HCS | 28-homocastasterone |
| POD | peroxidase |
| qL | coefficients of photochemical quenching based on the “lake” model |
| qP | coefficients of photochemical quenching based on the “puddle” model |
| SOD | superoxide dismutase |
| TBARS | complex between thiobarbituric acid and thiobarbituric acid-reactive substances |
| TF | translocation factor |
| Y(NO) | quantum yields of nonregulated energy dissipation |
| Y(NPQ) | quantum yields of and regulated energy dissipation |
| Y(II) | effective quantum yields of PSII |
References
- Kopittke, P.M.; Blamey, F.P.C.; Asher, C.J.; Menzies, N.W. Trace metal phytotoxicity in solution culture: A review. J. Exp. Bot. 2010, 61, 945–954. [Google Scholar] [CrossRef] [PubMed] [Green Version]
- Villiers, F.; Jourdain, A.; Bastien, O.; Leonhardt, N.; Fujioka, S.; Tichtincky, G.; Parcy, F.; Bourguignon, J.; Hugouvieux, V. Evidence for functional interaction between brassinosteroids and cadmium response in Arabidopsis thaliana. J. Exp. Bot. 2012, 63, 1185–1200. [Google Scholar] [CrossRef] [PubMed] [Green Version]
- Singh, S.; Parihar, P.; Singh, R.; Singh, V.P.; Prasad, S.M. Heavy metal tolerance in plants: Role of transcriptomics, proteomics, metabolomics, and ionomics. Front. Plant Sci. 2016, 6, 1143. [Google Scholar] [CrossRef] [Green Version]
- Srivastava, V.; Sarkar, A.; Singh, S.; Singh, P.; de Araujo, A.S.F.; Singh, R.P. Agroecological responses of heavy metal pollution with special emphasis on soil health and plant performances. Front. Plant Sci. 2017, 5, 64. [Google Scholar] [CrossRef] [Green Version]
- Bian, M.; Zhou, M.; Sun, D.; Li, C. Molecular approaches unravel the mechanism of acid soil tolerance in plants. Crop J. 2013, 1, 91–104. [Google Scholar] [CrossRef] [Green Version]
- Kopittke, P.M.; Blamey, F.P.C. Theoretical and experimental assessment of nutrient solution composition in short-term studies of aluminum rhizotoxicity. Plant Soil 2016, 406, 311–326. [Google Scholar] [CrossRef]
- Gomes, M.M.A. Physiological effects related to brassinosteroid application in plants. In Brassinosteroids: A Class of Plant Hormone; Springer: Dordrecht, The Netherlands, 2011; pp. 193–242. [Google Scholar] [CrossRef]
- Horst, W.J.; Wang, Y.; Eticha, D. The role of the root apoplast in aluminium-induced inhibition of root elongation and in aluminium resistance of plants: A review. Ann. Bot. 2010, 106, 185–197. [Google Scholar] [CrossRef]
- Singh, S.; Tripathi, D.K.; Singh, S.; Sharma, S.; Dubey, N.K.; Chauhan, D.K.; Vaculik, M. Toxicity of aluminium on various levels of plant cells and organism: A review. Environ. Exp. Bot. 2017, 137, 177–193. [Google Scholar] [CrossRef]
- Shahzad, B.; Tanveer, M.; Che, Z.; Rehman, A.; Cheema, S.A.; Sharma, A.; Song, H.; Rehman, S.U.; Dong, Z. Role of 24-epibrassinolide (EBL) in mediating heavy metal and pesticide induced oxidative stress in plants: A review. Ecotoxicol. Environ. Saf. 2018, 147, 935–944. [Google Scholar] [CrossRef]
- Rao, X.; Dixon, R.A. Brassinosteroid mediated cell wall remodeling in grasses under abiotic stress. Front. Plant Sci. 2017, 8, 8061143. [Google Scholar] [CrossRef] [Green Version]
- Vriet, C.; Russinova, E.; Reuzeau, C. Boosting crop yields with plant steroids. Plant Cell 2012, 24, 842–857. [Google Scholar] [CrossRef] [Green Version]
- Wu, C.; Li, F.; Xu, H.; Zeng, W.; Yu, R.; Wu, X.; Li, S.; Liu, Y.; Li, J. The potential role of brassinosteroids (BRs) in alleviating antimony (Sb) stress in Arabidopsis thaliana. Plant Physiol. Biochem. 2019, 141, 51–59. [Google Scholar] [CrossRef]
- Kolomeichuk, L.V.; Danilova, E.D.; Khripach, V.A.; Zhabinskyi, V.N.; Kuznetsov, V.V.; Efimova, M.V. Ability of lactone- and ketone-containing brassinosteroids to induce priming in rapeseed plants to salt stress. Russ. J. Plant Physiol. 2021, 68, 499–509. [Google Scholar] [CrossRef]
- Kovtun, I.S.; Kukharenko, N.E.; Kuznetsov, V.V.; Khripach, V.A.; Efimova, M.V. Effect of lactone- and ketone-containing brassinosteroids on photosynthetic activity of barley leaves during aging. Russ. J. Plant Physiol. 2021, 68, 440–450. [Google Scholar] [CrossRef]
- Blamey, F.P.C.; Hernandez-Soriano, M.C.; Cheng, M.; Tang, C.; Paterson, D.J.; Lombi, E.; Wang, W.H.; Scheckel, K.G.; Kopittke, P.M. Synchrotron-based techniques shed light on mechanisms of plant sensitivity and tolerance to high manganese in the root environment. Plant Physiol. 2015, 169, 2006–2020. [Google Scholar] [CrossRef] [PubMed] [Green Version]
- Li, Z.; Wang, P.; Menzies, N.W.; Kopittke, P.M. Defining appropriate methods for studying toxicities of trace metals in nutrient solutions. Ecotoxicol. Environ. Saf. 2018, 147, 872–880. [Google Scholar] [CrossRef]
- Kour, J.; Kohli, S.K.; Khanna, K.; Bakshi, P.; Sharma, P.; Singh, A.D.; Ibrahim, M.; Devi, K.; Sharma, N.; Ohri, P.; et al. Brassinosteroid Signaling, Crosstalk and, Physiological Functions in Plants Under Heavy Metal Stress. Front. Plant Sci. 2021, 12, 608061. [Google Scholar] [CrossRef]
- Pal, M.; Janda, T.; Szalai, G. Interactions between plant hormones and thiol-related heavy metal chelators. Plant Growth Regul. 2018, 85, 173–185. [Google Scholar] [CrossRef] [Green Version]
- Rajewska, I.; Talarek, M.; Bajguz, A. Brassinosteroids and response of plants to heavy metals action. Front. Plant Sci. 2016, 7, 629. [Google Scholar] [CrossRef] [Green Version]
- Kaur, N.; Pati, P.K. Harnessing the potential of brassinosteroids in abiotic stress tolerance in plants. In Brassinosteroids: Plant Growth and Development; Springer: Singapore, 2019; pp. 407–423. [Google Scholar] [CrossRef]
- Campbell, D.A.; Tyystjärvi, E. Parameterization of photosystem II photoinactivation and repair. Biochim. Biophys. Acta (BBA)-Bioenerg. 2012, 1817, 258–265. [Google Scholar] [CrossRef] [Green Version]
- Ramel, F.; Birtic, S.; Cuine, S.; Triantaphylides, C.; Ravanat, J.L.; Havaux, M. Chemical quenching of singlet oxygen by carotenoids in plants. Plant Physiol. 2012, 158, 1267–1278. [Google Scholar] [CrossRef] [PubMed] [Green Version]
- Sharma, P.; Bhardwaj, R. Effect of 24-epibrassinolide on seed germination, seedling growth and heavy metal uptake in Brassica junceae L. Gen. Appl. Plant Physiol. 2007, 33, 59–73. [Google Scholar] [CrossRef]
- Bhardwaj, R.; Sharma, P.; Arora, H.K.; Arora, N. 28-Homobrassinolide regulated Mn-uptake and growth of Brassica juncea L. Can. J. Pure Appl. Sci. 2008, 2, 149–154. [Google Scholar]
- Ramakrishna, B.; Rao, S.S.R. Preliminary studies on the involvement of glutathione metabolism and redox status against zinc toxicity in radish seedlings by 28-homobrassinolide. Environ. Exp. Bot. 2013, 96, 52–58. [Google Scholar] [CrossRef]
- Marschner, H. (Ed.) Marschner’s Mineral Nutrition of Higher Plants; Academic Press: Cambridge, MA, USA, 2012; 651p. [Google Scholar] [CrossRef]
- Danilova, E.D.; Kuznetsov, V.V.; Efimova, M.V.; Zlobin, I.E. Exogenic melatonin reduces the toxic effect of polymetallic stress on barley plants. Dokl. Biochem. Biophys. 2021, 499, 228–232. [Google Scholar] [CrossRef]
- Danilova, E.D.; Litvinovskaya, R.P.; Zlobin, I.E.; Kolomeichuk, L.V.; Murgan, O.K.; Sauchuk, A.L.; Khripach, V.A.; Kuznetsov, V.V.; Efimova, M.V. Polymetallic stress changes the endogenous status of brassinosteroids and reduces the effectiveness of photochemical reactions photosystem II in barley plants. Dokl. Biochem. Biophys. 2022, 504, 123–127. [Google Scholar] [CrossRef]
- Anikiev, V.V.; Kutuzov, F.F. Novyj sposob opredelenija ploshhadi listovoj poverhnosti u zlakov [A new method for leaf area estimation in cereals]. Russ. J. Plant Physiol. 1961, 8, 375–377. [Google Scholar]
- Buege, J.A.; Aust, S.D. Microsomal lipid peroxidation. Meth. Enzymol. 1978, 52, 302–310. [Google Scholar] [CrossRef]
- Lichtenthaler, H.K. Chlorophylls and carotenoids: Pigments of photosynthetic biomembranes. Meth. Enzymol. 1987, 148, 350–382. [Google Scholar] [CrossRef]
- Beauchamp, C.; Fridovich, I. Superoxide dismutase improved assays and an assay applicable to acrylamide gels. Anal. Biochem. 1971, 44, 276–287. [Google Scholar] [CrossRef]
- Efimova, M.V.; Khripach, V.A.; Boyko, E.V.; Malofii, M.K.; Kolomeichuk, L.V.; Murgan, O.K.; Vidershpun, A.N.; Mukhamatdinova, E.A.; Kuznetsov, V.V. The priming of potato plants induced by brassinosteroids reduces oxidative stress and increases salt tolerance. Dokl. Biol. Sci. 2018, 478, 33–36. [Google Scholar] [CrossRef]
- Esen, A. A simple method for quantitative, semiquantitative, and qualitative assay of protein. Anal. Biochem. 1978, 89, 264–273. [Google Scholar] [CrossRef]
- Pradko, A.G.; Litvinovskaya, R.P.; Sauchuk, A.L.; Drach, S.V.; Baranovsky, A.V.; Zhabinskii, V.N.; Mirantsova, T.V.; Khripach, V.A. A new ELISA for quantification of brassinosteroids in plants. Steroids 2015, 97, 78–86. [Google Scholar] [CrossRef]
- Efimova, M.V.; Litvinovskaya, R.P.; Medvedeva, Y.V.; Murgan, O.K.; Sauchuk, A.L.; Kuznetsov, V.V.; Khripach, V.A. The endogenous brassinosteroid content and balance in potato microclones is determined by organ specificity and the variety ripening term. Dokl. Biol. Sci. 2019, 485, 33–36. [Google Scholar] [CrossRef]
- Wang, X.K.; Gong, X.; Cao, F.; Wang, Y.; Zhang, G.; Wu, F. HvPAA1 encodes a P-Type ATPase, a novel gene for cadmium accumulation and tolerance in barley (Hordeum vulgare L.). Int. J. Mol. Sci. 2019, 20, 1732. [Google Scholar] [CrossRef] [Green Version]
- Tiong, J.; McDonald, G.; Genc, Y.; Shirley, N.; Langridge, P.; Huang, C.Y. Increased expression of six ZIP family genes by zinc (Zn) deficiency is associated with enhanced uptake and root-to-shoot translocation of Zn in barley (Hordeum vulgare). New Phytol. 2015, 207, 1097–1109. [Google Scholar] [CrossRef]
Figure 1.
Chemical structure of brassinosteroids.
Figure 2.
The effects of heavy metal stress and treatment with brassinosteroids on the growth parameters of barley plants. The value in the control plants was taken as 1.0, and the relative decrease is indicated in blue. Here and below: For description of experimental variants, see Materials and methods. Pairwise comparisons of the means were performed using Student’s t-test. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 2.
The effects of heavy metal stress and treatment with brassinosteroids on the growth parameters of barley plants. The value in the control plants was taken as 1.0, and the relative decrease is indicated in blue. Here and below: For description of experimental variants, see Materials and methods. Pairwise comparisons of the means were performed using Student’s t-test. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 3.
The effects of heavy metal stress and treatment with brassinosteroids on the primary photosynthetic processes and concentrations of photosynthetic pigments (mg/g fresh weight) in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, and the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 3.
The effects of heavy metal stress and treatment with brassinosteroids on the primary photosynthetic processes and concentrations of photosynthetic pigments (mg/g fresh weight) in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, and the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 4.
The effects of heavy metal stress and treatment with brassinosteroids on the content of TBARS (ng/g fresh weight) and activity of antioxidant enzymes, SOD (U/g protein) and POD (U/g protein in min), in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 4.
The effects of heavy metal stress and treatment with brassinosteroids on the content of TBARS (ng/g fresh weight) and activity of antioxidant enzymes, SOD (U/g protein) and POD (U/g protein in min), in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 5.
The effects of heavy metal stress and treatment with brassinosteroids on the elemental content (μg/g dry weight) and translocation factors in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. TF—translocation factor. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 5.
The effects of heavy metal stress and treatment with brassinosteroids on the elemental content (μg/g dry weight) and translocation factors in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. TF—translocation factor. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 6.
The effects of heavy metal stress and treatment with brassinosteroids on the content of cadmium and nickel ions (μg/g dry weight) and translocation factors in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. TF—translocation factor. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 6.
The effects of heavy metal stress and treatment with brassinosteroids on the content of cadmium and nickel ions (μg/g dry weight) and translocation factors in barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. TF—translocation factor. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 7.
The effects of heavy metal stress and treatment with brassinosteroids on the expression of genes involved in metal detoxification in roots (A) and shoots (B) of barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 7.
The effects of heavy metal stress and treatment with brassinosteroids on the expression of genes involved in metal detoxification in roots (A) and shoots (B) of barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant, and the a letter indicates significant differences from the polymetallic stress-treated variant (p < 0.05).
Figure 8.
The effects of heavy metal stress on brassinosteroids content (ng/g dry weight) in roots and shoots of barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant (p < 0.05).
Figure 8.
The effects of heavy metal stress on brassinosteroids content (ng/g dry weight) in roots and shoots of barley plants. The value in the control plants was taken as 1.0, the relative decrease is indicated in blue, the relative increase is indicated in red. Asterisks (*) indicate significant differences from the control variant (p < 0.05).
Table 1.
Concentrations of metals.
| Metal | Concentration, µM |
|---|---|
| Al3+ | 20 |
| Mn2+ | 50 |
| Cd2+ | 2.8 |
| Cu2+ | 2 |
| Ni2+ | 16 |
| Zn2+ | 40 |
| Pb2+ | 30 |
Table 2.
List of genes, gene-specific primers, and PCR conditions.
| Gene ID | Gene | F (5′→3′) | R (5′→3′) | Tm, °C | Amplicon Size, bp | References |
|---|---|---|---|---|---|---|
| LOC123430406 | Actin, the gene encoding the protein actin | TGGCTGACGGTGAGGACA | CGAGGGCGACCAACTATG | 61 | 121 | [38] |
| LOC123413551 | HvGAPDH, the gene encoding glyceraldehyde-3-phosphate dehydrogenase 1 | GTGAGGCTGGTGCTGATTACG | TGGTGCAGCTAGCATTTGAGAC | 61 | 198 | [39] |
| LOC123406919 | HvPAA1, encodes a specific ATPase for Cu2+/Ag2+ transfer | ATGTGCTTGGTCTTGCCA | TCCCTCGCTGTGAGAAGCTA | 53 | 194 | [38] |
| LOC123407761 | HMA1, encodes a specific ATPase for Zn2+/Cu2+/Cd2+/Pb2+ transfer | CCATGTGCATTGGCAGTAGC | AATACATGCCCGCCTTTCAA | 59 | 92 (512) | |
| LOC123401671 | HMA4, encodes a specific ATPase forZn2+/Cu2+/Cd2+/Pb2+ transfer | GACAGTGGTGGCAGGATTGAAGG | TGGTTCTTGCATCGGTCTCCTCG | 64 | 104 | |
| LOC123414343 | HvMTP1, encodes a metal resistance protein | CGCAGGATGTGGATGCTGAT | CTCCAGCACCAAAGGCAACA | 61 | 223 | [39] |
| LOC123430267 | ALMT, encodes the protein aluminum-activated malate transporter | CGGAGCTCTTTGTCGTCAGT | CATTTCCCCACACGCCATTC | 60 | 133 |
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Zlobin, I.E.; Danilova, E.D.; Murgan, O.K.; Kolomeichuk, L.V.; Litvinovskaya, R.P.; Sauchuk, A.L.; Kuznetsov, V.V.; Efimova, M.V. Structurally Different Exogenic Brassinosteroids Protect Plants under Polymetallic Pollution via Structure-Specific Changes in Metabolism and Balance of Cell-Protective Components. Molecules 2023, 28, 2077. https://doi.org/10.3390/molecules28052077
AMA Style
Zlobin IE, Danilova ED, Murgan OK, Kolomeichuk LV, Litvinovskaya RP, Sauchuk AL, Kuznetsov VV, Efimova MV. Structurally Different Exogenic Brassinosteroids Protect Plants under Polymetallic Pollution via Structure-Specific Changes in Metabolism and Balance of Cell-Protective Components. Molecules. 2023; 28(5):2077. https://doi.org/10.3390/molecules28052077
Chicago/Turabian StyleZlobin, Ilya E., Elena D. Danilova, Ol’ga K. Murgan, Liliya V. Kolomeichuk, Raisa P. Litvinovskaya, Alina L. Sauchuk, Vladimir V. Kuznetsov, and Marina V. Efimova. 2023. "Structurally Different Exogenic Brassinosteroids Protect Plants under Polymetallic Pollution via Structure-Specific Changes in Metabolism and Balance of Cell-Protective Components" Molecules 28, no. 5: 2077. https://doi.org/10.3390/molecules28052077
