Phytoextraction of Trace Metals (Cd, Ni and Pb) by Panicum maximum Grown on Natural Soil

Abstract

This study aims to assess the effective capacity of Panicum maximum to accumulate cadmium (Cd), nickel (Ni) and lead (Pb). P. maximum observed in a greenhouse was subjected to 2 ppm of Cd, 50 ppm of Ni, 100 ppm of Pb contaminated soil and uncontaminated soil, for 120 days. Plant growth and biomass produced concentration of trace metals in soil and plant, bioaccumulation and transfer factors, location of potentially toxic elements in tissues and cells of plant have been determined. Stem length and biomass produced by P. maximum were higher on the uncontaminated soil followed respectively by those of soil-contaminated by Pb, Cd and Ni. Bioaccumulation factors of trace metals were 8.93 (Pb), 8.47 (Ni) and 3.37 (Cd). Ni was more accumulated in shoot biomass (FT > 1), while Pb and Cd were concentrated in root biomass (FT < 1). Pb is accumulated preferentially in endodermis (roots) and epidermis (leaves). As for Ni and Cd, they are concentrated in central cylinder of roots and in conductive bundles of leaves. At cellular level, Ni and Cd are mainly concentrated in intracellular compartments of leaves and roots, while Pb is strongly detected at cell walls.

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Coulibaly, H. , Ouattara, P. , Messou, A. and Coulibaly, L. (2021) Phytoextraction of Trace Metals (Cd, Ni and Pb) by Panicum maximum Grown on Natural Soil. Open Journal of Applied Sciences, 11, 929-945. doi: 10.4236/ojapps.2021.118068.

1. Introduction

Anthropogenic activities are the major source of many pollutants disseminated in the environment. Trace metals are among these priority risk pollutants because they are potentially very toxic and non-degradable elements. They stay in the environment for a long time [1]. These metals present in the soil cause risks to all the biosphere and are taken up through direct ingestion, absorbed by plants which can be hazardous both to the plant and also to the food chain [2] [3] [4]. At the microscopic scale, trace metals have adverse effects on bacterial populations, which are not without consequences on the functioning of the ecosystem [5]. Consequently, several physical and chemical remediation technologies for trace metals, contaminated soils have been developed. However, these technologies are generally expensive, greatly disrupt the biological activity of soils and alter their physical and chemical characteristics [6] [7]. As a result, research is increasingly directed towards biological processes exploiting the properties of living organisms (microorganisms or plants) to carry out the clean-up operation. In fact, despite their potential toxicity, most sites contaminated by trace metals often have a diverse flora that tolerates more or less high levels of metals. The study of these resistant plants, by their capacities of detoxification, immobilization or absorption of trace metals, paved the way for the development of a new tool for soil rehabilitation, phytoremediation [8]. Phytoremediation could provide a sustainable technique for metals-contaminated soils remediation. Indeed, phytoremediation is a less expensive technique, more extensive and ecological [9] [10] [11]. This technology has received more attention [12] and has shown better results in several countries [11] [13]. However, plant species previously experienced are not always present in Cote d’Ivoire. Consequently, their implementation may be confronted with problems of adaptation to local soils, hence the need to explore endogenous species with potential for accumulation. In Côte d’Ivoire, the work of Messou [14] on Akouédo landfill made it possible to assess the accumulation capacities of certain endogenous species, including Panicum maximum. This work has shown that this plant produced both a significant plant biomass and had a high potential for the accumulation of Cd, Pb, Cu, Ni and Zn [14]. However, this study does not make it possible to apprehend the effects of competition or inhibition of trace metals. Moreover, the remediation mechanisms for trace metals were not elucidated. The work of Hogban et al. [15] carried out on synthetic soil also showed that Panicum maximum accumulates Cd, Ni and Pb. However, seen the interactions that could occur in natural soil, it has proven to be a good idea to replicate the work on natural soil. Thus, it involves evaluating the effect of the trace metals studied on the growth of plants and soil microorganisms, determining the potential for extraction of these trace metals by P. maximum and understanding their accumulation mechanisms.

2. Material and Methods

2.1. Experimental Procedure

The experimental was performed in a greenhouse (length = 13 m and width = 11 m) at the experimental site of the biotechnology and environmental engineering research unit of Nangui Abrogoua University, Côte d’Ivoire. It was equipped with a fan powered by a solar plate to regulate the temperature and the flow of air inside. Inside the greenhouse, 32 PVC pots (length = 27 cm, width = 20 cm, height = 45 cm) containing soil contaminated or not, at a height of 40 cm, were arranged.

2.2. Soil

Topsoil used was collected from an uncultivated plot of NanguiAbrogoua University. The soil was air dried, thoroughly mixed and sieved to 2 mm. The soil was artificially contaminated with metallic salt. Depending on the desired contamination, the soils were saturated with an amount of metallic salt determined by Equation (1) [5] [16]:

m metallicsalt = C × m soil × M metallicsalt M heavymetals (1)

mmetallic salt = mass of heavy metals (mg);

Mmetallic salt = Molar mass of heavy metals (g/mol);

Mheavy metal = Molar mass of heavy metals (g/mol);

msoil = Mass of soil in the pot (kg);

C = Theoretical concentration of heavy metals (mg/kg).

2.3. Plant Selection

Panicum maximum was selected according to its availability, its rapid growth and its potential tolerance of heavy metals (Pb, Cd, Ni) [14]. In addition, P. maximum produces significant shoot and root biomass and has been described as phytoaccumulator [14] [17].

2.4. Experimental Design

The experiment was performed with plants grown on uncontaminated (control) and contaminated soil. Contaminated soil was treated with nickel (Ni), lead (Pb), cadmium (Cd). Each treatment was replicated eight times. Trace metals concentrations in soil at the start of experience were 2 ppm for Cd, 50 ppm for Ni and 100 ppm for Pb. Moreover, seedlings of P. maximum were used to establish nurseries on the experimental site. Plants with the same morphological development were selected and cultured.

2.5. Data Collection

Growth monitoring was carried out by weekly measurement of the height of the studied plant stems using a tape measure. Plants of two (2) replicates per trace metals contaminated were harvested monthly and the plant biomasses produced were determined by weighing on a 10−3 precision Sartorius EB150FEG-I scale.

Trace metals concentrations were analyzed on composite samples taken monthly from horizons (0 - 10, 10 - 20, 20 - 30 and 30 - 40 cm) of soils. The samples were kept in hermetically sealed jars until analysis.

To assess trace metals accumulation, two (2) plant replicas were taken heavy metals contaminated soil every month (30 days). Harvested plants were separated into shoot and root parts. Each plant sample was washed with distilled water and high purity water. After air-drying, each plant sample was dried at 80˚C to a constant weight. The dried samples were crushed using a stainless-steel plant tissue grinder (LD-Y500A).

2.6. Samples Analysis

Trace metals concentrations of soil were carried out according to the standard ISO 11466, [18]. The soil sample (0.5 g) was digested with a mixture of HCl and HNO3 (7.5 ml of HCl and 2.5 ml of HNO3). The content was filtered at 0.45 µm and diluted up to 50 ml with distilled water. Trace metals concentrations were determined by plasma-coupled induction atomic emission spectrometry (ICP-AES).

The mineralization of plant samples was made according to the standard NF X31-151 [19]. Subsample (20 g) of crushed plant material was oven-dried at 500˚C for 2 hours and 0.5 g of that burned sample was digested with 10 ml of aqua regia (7.5 ml of HCl and 2.5 mL of HNO3). Then, the sample was put in an oven at 180˚C for 30 min for ending digested process. The filtrate obtained after cooling was used for trace metals analysis by plasma coupled induction atomic emission spectrometry (ICP-AES).

2.7. Phytoextraction Efficiency

Two factors were calculated to evaluate plant phytoextraction efficiency. The bioaccumulation factor (BF) was calculated to determine the degree of metal accumulation in the plants grown (Equation (2)) [20]. However the transfer factor (TF) defined as the ratio between the metal concentration in plant shoots and its concentration in roots (Equation (3)) [21] [22]. It indicated the capability of plants to take up trace metals from their roots and to translocate them to their shoots.

BF = Metal concentration in roots + Metal concentration in shoots Metal concentration in soil (2)

TF = Metal concentration in shoots Metal concentration in roots (3)

- TF > 1: accumulation of trace metals in the shoot biomass of plants;

- TF < 1: accumulation of trace metals in the root biomass of plants.

2.8. Localization of Cd, Ni and Pb in Tissues and Cells of P. maximum

This study determined the distribution of trace metals in plant roots and leaves, precisely at the tissue and the cell level. It was performed using a scanning electron microscope equipped with an X-ray detector connected to an EDS micro-analyzer platform (SEM-EDS). For the analyses, the plant materials (leaves and roots) were collected at the end of the experiment from the Cd, Ni and Pb contaminated soil. Those samples were fixed for 24 hours in 2.5% glutaraldehyde (pH 7.2). Then, they were rinsed two or more times with distilled water. A 2 mm cross-section of the samples (leaf or root) was followed by dehydration in successive baths of 30 min of ethanol (from 70% - 100%). The samples were subsequently dried in the open air and fixed on pads placed on a plate carried in the metallizer to spray them with gold. The plate was finally mounted on the stage of scanning electron microscope equipped with an X-ray detector connected to an EDS micro-analyzer platform to perform trace metals observations in the tissue and the cell.

2.9. Statistical Analysis

Statistical analysis of the data was performed with R software version 3.3.2. The normality of the data distribution of the variances was verified with the Shapiro test. To examine differences between growth and biomass produced by the plant in the culture pots, transfer factor and bioaccumulation factors, data were analyzed using the parametric test (t-test, ANOVA test) and the non-parametric test (Mann Whitney). Statistical significance was defined at the level of p < 0.05.

3. Results

3.1. Plant Growth

The growth of P. maximum, assessed from the average length of the stems during the treatment trial, is shown in Figure 1. Regular growth of the plant is observed the pots of culture. The order of the average lengths of stem at the end of the experiment is as follows: 176 cm (STe) > 167 cm (SPb) > 135 cm (SCd) > 83 cm (SNi). Statistical analysis shows plant lengths of stem on Ni-contaminated soil is much smaller than those of the others (Mann-Whitney test: p < 0.05). On the other hand, growth of plant on uncontaminated soil (control soil) and that contaminated with Pb do not differ significantly (Mann-Whitney test: p > 0.05).

3.2. Biomass Produced

Figure 2 shows the variation of shoot and root biomass of P. maximum during the experiment. It noted that shoot and root biomasses increase over time.

Figure 1. Growth profile of P. maximum stems during the experiment; STe = Control soil soil; SNi = Soil contaminated by nickel; SCd = Soil contaminated bycadmium; SPb = Soil contaminated by lead.

Figure 2. Plant biomass of P. maximum produced as a function of the duration of the treatment, STe = Control soil; SNi = Soil contaminated by nickel; SCd = Soil contaminated by cadmium; SPb = Soil contaminated by lead.

However, shoot biomass of P. maximum remains higher than the root biomass. From day 30 to day 120, shoot biomasses recorded vary from 198 ± 1.8 - 409.5 ± 5 g (STe), de 176 ± 32 - 390.3 ± 4.3 g (SPb), de 156 ± 8.9 - 337 ± 8.9 g (SCd) et de 104 ± 4.5 - 156.2 ± 3 g (SNi). On the other hand, root biomasses evolve from 80 ± 1.5 - 306.4 ± 5 g, de 76.4 ± 0.92 - 279.2 ± 2.5 g, de 72.6 ± 0.4 - 244.8 ± 1.5 g et de 53.8 ± 1.6 - 103.5 ± 2 g, respectively in the uncontaminated soil (control soil) and those contaminated with Pb, Cd and Ni. Comparing biomasses (shoot and root) produced by P. maximum, we notice that biomass from Ni contaminated soil is much lower than others (t test: p < 0.05) (Figure 3).

3.3. Trace Metals Accumulation Potential ofP. maximum

Pb and Cd accumulation in the shoot and root biomasses of P. maximum (Table 1) indicated that the higher concentrations were recorded in the root. In contrast, Ni concentrations were higher in shoot biomass. However, concentrations of each trace metals obtained in shoot and root biomasses increase during treatment. Pb concentrations ranged from 23.93 - 234.7 ppm in shoot biomass and from 36.62 - 384.75 ppm in root biomass. For Cd, it ranged from 0.15 - 2.54 ppm in shoot biomass and from 0.16 - 3.23 ppm in root biomass. Ni concentrations in shoot and root biomass ranged from 33 - 216.75 ppm and from 22.5 - 99.75 ppm, respectively.

Figure 3. View of the plants at the end of the experiment.

Table 1. Concentration of trace metals in biomass of P. maximum.

Table 2 shows the Bioaccumulation Factor (BF) and Transfer Factor (TF) of trace metals for P. maximum. BF values ranged from 0.64 - 8.93 (Pb), 0.16 - 3.37 (Cd) and 1.2 - 8.47 (Ni). These BF values were not significantly different (ANOVA test: p > 0.05). Concerning TF values, they ranged from 0.41 - 0.91 (Pb), from 0.72 - 0.83 (Cd) and from 1.47 - 3.38 (Ni). The transfer factor for Ni was the highest and was greater than 1. Moreover, TF for Ni were significantly different of TF for Pb and Cd (ANOVA test: p < 0.05).

3.4. Localization of Cd, Ni and Pb in the Tissues and Cells of Panicummaximum

Figures 4-6 show SEM/EDS of root and leaf of Panicum maximum accumulated trace metals (Ni, Pb and Cd). In tissues, Pb was accumulated preferentially on endodermis (roots) and epidermis (leaves). As for Ni and Cd, they were concentrated in the central cylinder of roots and in the conductive bundles of leaves. Moreover, by carrying out the investigations at cellular level, it was noted that Ni and Cd were mainly concentrated in the intracellular compartments of leaves and roots of P. maximum, while Pb was strongly detected on the cell walls

3.5. Density of Microorganisms in Soils

Figure 7 shows the density of microorganisms (total mesophilic flora and

Figure 4. SEM/EDS of root ((a) and (b)) and leaf ((c) and (d)) of Panicum maximum accumulated Ni.

Figure 5. SEM/EDS of root ((a) and (b)) and leaf ((c) and (d)) of Panicum maximum accumulated Pb.

Figure 6. SEM/EDS of root ((a) and (b)) and leaf ((c) and (d)) of Panicum maximum accumulated Cd.

Figure 7. Density of microorganisms in soils; (a) total mesophilic flora and (b) P. aeruginosa; STe = control soil; SNi = soil contaminated by nickel; SCd = soil contaminated by cadmium; SPb = soil contaminated by lead.

Table 2. Bioaccumulation Factor (BF) and Transfer Factor (TF) of trace metals.

Pseudomonas aeruginosa) in the pots contaminated by Pb, Ni and Ni and in control pot. It is observed that the density of microorganisms increases with duration of the treatment of the soils in the culture pots. In addition, densities recorded in the control remain the highest compared to those in contaminated pots. Densities of the total mesophilic flora ranged from 0.82 × 105 - 7.72 × 105 UFC/g, from 0.48 × 105 - 6.87 × 105 UFC/g, from 0.24 × 105 - 3.33 × 105 UFC/g and 0.62 × 105 - 5.10 × 105 UFC/g respectively in control soil and Cd, Ni and Pb contaminated soil, from day 30 to day 120. These densities do not differ significantly (Kruskal-wallis test: p > 0.05). Concerning P. aeruginosa, its varies from 17.12 - 72.37 UFC/g in control, from 6 - 21.37 UFC/g in soil contaminated by Ni, from 8.62 - 38.62 UFC/g in soil contaminated by Cd and from 11.25 - 31.87 UFC/g in soil contaminated by Pb. Statistical analysis indicates that there is no significant difference between the densities of P. aeruginosa in the different soils culture (ANOVA test; p > 0.05).

4. Discussion

The present study aims to evaluate the capacity of Panicum maximum to accumulate trace metals (Cd, Ni and Pb) on natural soil. Plant growth appeared regular in both the contaminated and uncontaminated (control) soil, due to the considerable proportion of organic matter in the natural soil. However, a slowdown in plant growth has been observed in contaminated soil, possibly due to metal pollutants. Olatunji et al. [23] also observed such plant growth on soils contaminated by Ni, Pb and Cd. However, the analysis of the evolution of the plants revealed that the smallest sizes were recorded in soil contaminated by Ni, probably related to the concentration in the biomass of P. maximum. Indeed this concentration of Ni is, according to Gerendás et al. [24], beyond the critical threshold (10 ppm) of this trace metals in plant biomass. This result could be explained by the fact that Ni is an essential metal element for the plant, unlike Cd and Pb, which are not essential. However, at high concentrations Ni affects plant growth [24]. This justifies much higher P. maximum sizes in Pb and Cd contaminated soil. However, bioaccumulation factors of Pb were higher, followed respectively by those of Ni and Cd, indicating a high tolerance of Pb by P. maximum compared to others trace metals. This result is in agreement with those of several studies including Olatunji et al. [23], Olowoyo et al. [25] and Onojake and Enukoha [26] According to these authors, this sequence of accumulation of the trace metals studied is linked to the physiology of the plant, which tolerates more Pb, compared to others metals. However, of all the trace metals, only the transfer factor of Ni is greater than 1, indicating a preferential accumulation of this metal in shoot biomass. These results are in agreement with those obtained in the treatment of synthetic soil [15] as well as those of the work of Messou [14. Several studies claim that once in the roots, Ni is preferentially translocated into the aerial parts of the plant [27] [28] [29]. Indeed, in the roots, according to Haydon and Cobbett [30] Montargès-Pelletier [31] and Araujo et al. [32] Ni binds to molecular organic ligands (citrate and malate) and amino acids (histidine, glutamine) to limit its precipitation. This complexation would be at the origin of the suppression of the sequestration of Ni in the root vacuoles and promote its transport to shoot of plants [33]. Regarding the soil microorganisms in the different growing soil, the results indicate that the density of total mesophilic flora and that of Pseudomonas aeruginosa increase during soil treatment. In fact, since these bacterial flora are aerobic organisms [34], the watering carried out during the trial would create ecological conditions favorable to a greater proliferation of these organisms. The flow of water through the growing soils would cause oxygen there, which is essential for the proliferation of bacteria during treatment [35] [36]. Furthermore, the increase in shoot biomass of the plant during the treatment would have promoted a similar growth of the root biomass, providing bacteria with more anchoring sites in the growing medium. This trend is similar to that observed in the work of Hogban et al. [15] on synthetic soils. However, the densities of total mesophilic flora and P. aeruginosa remain higher in natural soils compared to synthetic soils. The organic matter would be responsible for this situation. Indeed, because of the higher organic matter content, the soil would have favored a higher development of microorganisms in the culture pots [37]. SEM/EDS microanalysis performed in the root tissues of P. maximum shows that Pb preferentially accumulates in the cell walls of the endoderm. Patra et al. [38] and Seregin et al. [39] made these same observations. According to these authors, this property of Pb is also one of the reasons for its lower toxicity for the plant. In the leaves of P. maximum, Pb binds to the epidermis walls. This phenomenon is used as a strategy to prevent Pb from entering chloroplast cells were it can disrupt the CO2 binding system during photosynthesis [40]. As for Ni and Cd, they are detected in quantity in the cells of the central cylinder of the roots. In contrast, in the leaves, these trace metals are concentrated in the conductive bundles. According to Chen et al. [41], Mendoza Cózatl et al. [42] and Gong et al. [43], Cd binds to ligands containing sulfhydril groups such as phytochelatins, glutathione and cysteines, mainly found in the xylem of the roots and the phloem of the leaves. Regarding to Ni, Chen et al. [41] indicate a high percentage (over 80%) in the central cylinder of the roots. Thus, the great mobility of Ni in this tissue would have favored its translocation in shoots of the plant [44]. However, the significant accumulation of Ni in the conductive bundles of leaves affect the osmotic pressure of the cells of this tissue, especially the phloem responsible for transporting sugars throughout the plant [45].

5. Conclusion

The present study aims to determine the capacity of P. maximum to accumulate trace metals (Pb, Cd, Ni) on natural soil. It appears that stem length and plant biomass produced by P. maximum was higher on the uncontaminated soil followed respectively by those of the soil contaminated by Pb, Cd and Ni. Bioaccumulation factors of trace metals were 8.93 (Pb), 8.47 (Ni) and 3.37 (Cd). Ni was more accumulated in shoot biomass (FT > 1), while Pb and Cd were concentrated in root biomass (FT < 1). Pb is accumulated preferentially in endodermis (roots) and epidermis (leaves). The densities of total mesophilic flora and Pseudomonas aeruginosa increased in all the pots. In tissues, lead is accumulated preferentially on endodermis (roots) and epidermis (leaves). As for Ni and Cd, they are concentrated in the central cylinder of roots and in the conductive bundles of leaves. Moreover, by carrying out the investigations at cellular level, it is noted that Ni and Cd are mainly concentrated in the intracellular compartments of leaves and roots of P. maximum, while Pb is strongly detected on the cell walls. If the results of the present study have shown the capacity of P. maximum to remediate soils contaminated with Ni, Pb and Cd. Studies should be conducted with increasing concentrations of Ni, Pb and Cd to determine the maximum concentrations for which P. maximum can still keep its capacity for soil remediation.

Acknowledgements

We sincerely thank the members of the research team in Biotechnology and Environmental Engineering of Nangui Abrogoua University (Abidjan, Côte d’Ivoire) for their help during the field sampling, their critical examinations and their useful suggestions, all of which have greatly improved this manuscript

Conflicts of Interest

The authors declare no conflicts of interest regarding the publication of this paper.

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