Abstract
Metallic nanoparticles that have photocatalytic activity can be synthesized using aqueous plant extracts. The aim of this study was to synthesize iron nanoparticles using Lantana trifolia extracts and to evaluate their ability to degrade Congo red dye. The nanoparticles were characterized using UV–Vis spectrophotometer (UV–Vis), Fourier transform infra-red spectrophotometer, wide angle X-ray diffractometer, dynamic light scattering, transmission electron microscopy (TEM), and thermal gravimetric analyzer to determine the functional groups, thermal properties, crystalline phases and diameter distribution of the particles. Cyclic voltammetry was used to evaluate the redox potential of the extracts while photocatalytic activity of the nanoparticles was evaluated using a UV–Vis spectrophotometer. Functional groups analysis revealed presence of secondary metabolites having OH and C=C groups while a redox potential of + 0.3 V was an indication that the extracts can reduce iron. The presence of sharp peaks at 2θ values of 19.87°, 20.22°, 22.88°, 28.81°, 32.73°, 35.32°, 38.45°, 40.23° and 41.08° correspond to cubic crystal system of iron nanoparticles while particle aggregation was observed on TEM micrographs which also indicated that they were less than 200 nm. In the presence of H2O2, the nanoparticles catalyzed degradation of Congo red dye in a first order reaction that was temperature dependent. In conclusion, secondary metabolites in L. trifolia can reduce metallic ion to iron nanoparticles which can degrade Congo red dye.
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1 Introduction
Metallic nanoparticles have received great attention due to their unique physical, chemical and biological properties that makes them find applications in various fields such as medicine and in environmental remediation as photocatalysts [1]. During the past decade, many biological systems such as plants [2], algae [3], diatoms [4], bacteria [5], yeast [6], fungi [7], and human cells [8] have been used to transform inorganic metal ions into metal nanoparticles via the reductive capacities of the metabolites found in these organisms. For iron nanoparticles, several physical and chemical production methods including mechanical milling [9], sodium borohydride [10, 11], ethylene glycol [12], solvothermal method [13], and carbothermal synthesis [14] have been employed for their preparation [15]. Iron nanoparticles synthesized by these methods rapidly agglomerate to form clusters due to interparticle Van der waals and magnetic forces and may further undergo rapid oxidation [16, 17]. However, secondary metabolites found in plant extracts such as terpenoids, alkaloids, phenolic acids, polyphenols, sugars and proteins can play a significant role in the bioreduction of the Fe3+ ions to iron nanoparticles [15, 18]. This synthesis approach does not require heating and the metabolites act as reducing and capping agents thereby protecting the nanoparticles formed from autooxidation [15, 18,19,20]. These biosynthesized iron nanoparticles have found significant importance in environmental remediation as catalyst for degradation of organic dyes, chlorinated organic pollutants and adsorbent for heavy metal removal. In the presence of H2O2, iron nanoparticles catalyze the production of free radicals which promote the increase in the rate of degradation of organic dyes [21]. Lantana trifolia or lantana as it is commonly referred to, is a highly invasive shrub thought to have been brought into Africa from Europe and it is usually harvested from the wild for its medicinal value, where it is used locally as a source of food, medicine and wood. GC–MS profile of the plans has revealed the presence of secondary metabolites such as nonanoic acid, Ethyl iso-allocholate, 1,7-octadien-3-ol, cis-3-Hexenoic acid, cis-3-hexenoic acid, 2-Nonen-1-ol, 3-cyclopropyl-7-hydroxylmethyl bicycle[4.1.0]heptane, Germacrene D among many other compounds [22]. The aim of this study was to synthesize iron nanoparticles using aqueous extracts from L. trifolia and to evaluate their ability to catalyze the degradation of Congo red dye. The influence of temperature and contact time on the rate of degradation were evaluated using UV–Vis spectroscopy while the functional groups present, and thermal properties of the nanoparticles were investigated using Fourier Transform infrared spectroscopy and thermal gravimetric analysis. Wide angle X-ray diffractometer was used to evaluate the crystalline phases of the nanoparticles while TEM was used to determine their sizes.
2 Materials and methods
2.1 Sample preparation
Dry L. trifolia plant materials were collected from Juja, Kambu County in Kenya washed with distilled water and dried in the oven for 48 h at 70 °C. After cooling, the sample was finely ground (In-house fabricated mechanical grinder) and 100 g of the ground material was then mixed with 1000 ml of distilled water, boiled for 5 min, cooled and the solution filtered through a Whatman filter paper no. 1. The extract was then stored in a refrigerator at 4 °C until further studies [23].
2.2 Synthesis of iron nanoparticles
To synthesize iron nanoparticles, the aqueous plant extract was mixed with 0.1 M FeCl3·6H2O solution prepared in double distilled water in different ratio and concentration. For the reduction of Fe3+ ions, different volume of the aqueous plant extracts was then added slowly to the ferric chloride solution and vortexed (Vortex Genie 2, scientific industries, USA) for 3 min at room temperature. The formation of iron nanoparticles was indicated by a change in colour of the solution from light yellow to black [24]. The black precipitate was obtained through centrifugation at 1000 rpm (Hettich zentrifugen, Andreas Hettich group Tuttlingen, Germany) washed several times with MilliQ water and dried at 60 °C in the oven until further analysis [18].
2.3 Cyclic voltammetry
In our study, voltammetric measurements were carried out using a Metroohm Autolab made up of a potentiostat–galvanostat equipped with NOVA 2.0 software [25,26,27,28]. The experiment was performed in a single-compartment Pyrex cell using a conventional three-electrode configuration. Two-millimeter glassy carbon disk working electrode (GCE) polished before each measurement, a platinum wire counter electrode, and an Ag/AgCl saturated KCl reference electrode were used. Twenty milliliters of supporting solution were dispensed into an electrochemical cell followed by addition of appropriate volume of plant extracts. Cyclic voltammograms measurements were performed at positive potentials, at a scan rate of 100 mVs−1 at room temperature in the presence of KCl (0.1 M) as a supporting electrolyte [25].
2.4 Characterization of iron nanoparticles
UV–Vis absorption analysis was carried out using a Shimadzu UV–Vis 1800 spectrophotometer (Shimadzu, Japan) in the range of 200–800 nm [1]. The functional groups present in the nanoparticles were determined using a Bruker Tensor II FT-IR spectrophotometer model (Bruker, Ettlingen, Germany). The KBr pellets of the samples were prepared by grinding 10 mg of the samples with 250 mg KBr (FT-IR grade) [29, 30]. The thermal properties of FeNPs was evaluated using a Mettler Tolledo Thermal Gravimetric DSC/TGA 3 + system (Mettler-Toledo GmbH, Switzerland). 10 mg of the sample was heated from 25 to 500 °C at 10 min−1 cooled to 25 °C. The crystalline phase was identified using STOE STADIP P X-ray Powder Diffraction System (STOE & Cie GmbH, Darmstadt, Germany). The X-ray generator was equipped with a copper tube operating at 40 kV and 40 mA and irradiating the sample with a monochromatic CuKα radiation with a wavelength of 0.1545 nm [31]. The particle size distribution, zeta potential and poly-dispersibility index of the FeNPs solution were measured using a Bechman Coulter DelsaMax pro Dynamic light scattering analyzer (Indianapolis, United States). TEM analysis was performed on a Tecnai G2 Spirit (Thermo Fischer scientific, Oregon USA) operated at 120 kV equipped with veleta 2048 × 2048 wide angle and Eagle 4096 × 4096 bottom mount detectors. The dried iron nanoparticles were suspended in ultrapure water (18 MΩ cm Barnstead Genpure UV-TOC, Thermo Fischer scientific, Germany) and vortexed (Vortex Genie 2, scientific industries, USA) to obtain a solution of suspended nanoparticles. The solution was then drop casted in Carbon films 300 mesh (Electron microscopy science, CF300-CU) and dried to evaporate the solvent before TEM analysis.
2.5 Photodegradation studies
The ability of the synthesized nanoparticles to degrade Congo red dye under different reaction conditions was evaluated using UV–Vis spectrophotometer [32]. In 2.5 ml of Congo red dye (50 ppm) 0.5 ml H2O2 (30% v/v) was added to the reaction in a quartz cuvette followed by addition of 10 mg of iron nanoparticles. Absorbance readings were taken at 2 min intervals until equilibrium was attained and the degradation efficiency was determined using the following equation:
where A0 is the dye absorbance before decolorization and At is the dye absorbance after decolorization. The effect of temperature on degradation was investigated at different temperatures between 25 and 40 °C under constant pH while the effect of time was studied for 120 min respectively [32].
3 Results and discussions
3.1 Synthesis of iron nanoparticles
Synthesis of iron nanoparticles involved variation of metal ion in solution and the volume ratio of the extract to the metal ions and the results are depicted in Fig. 1.
In the case of biological synthesis of nanoparticles, the aqueous metal ions are reduced and as a result a color change is the first qualitative indication that nanoparticles have been formed (Fig. 1) [33, 34]. Variation of the ratio of the extract to the iron solution revealed that the nanoparticles were synthesized when the volume of the extracts to that of the metal ion was high (Fig. 1). Changes in metal ion concentration revealed that at lower and higher concentrations, the solutions did not become turbid as no particles were formed at lower concentration while at higher concentration, the reducing capability of the extracts was greatly reduced (Figure S1) [35]. Moreover, disappearance of the shoulder centered at 350 nm in the plant extract was only observed when the concentration of iron used was 0.1 M. The metal ion concentration is an important factor that needs to be considered and this may be adjusted by dilution [21, 36]. The presence of chemically complex biomolecules, e.g., enzymes, amino acids, proteins, vitamins, and polysaccharides, and organic acids act as reducing and capping agents during synthesis [33].
3.2 Measurement of redox potential of the extracts
The redox potential of the extracts was measured against standard ascorbic acid and the results are depicted in Fig. 2.
The extracts showed peak anodic currents at + 0.3 V and + 0.7 V an indication that they have strong free reducing capabilities as they are oxidized at relatively low potential [37]. The peak potential correlates with the type of reductant; low oxidation potentials are associated with a greater facility or strength of a given molecule to donate electrons [38, 39]. The reduction potential of the plant extracts (+ 0.7) was as a result of presence of polyphenols which make them able to reduce Fe3+ (+ 0.77) to Fe2+ [21, 40]. However, the extract did not completely reduce the Fe3+ to zero-valent iron as they are strongly stabilized due to the presence of polyphenols ligands and they rapidly oxidize in the presence of oxygen to give Fe2+ polyphenol complexes in a phenomenon known as autoxidation (Fig. 5) [41]. Moreover, the reduction potential of Fe2+ to Fe0 is highly negative which implies that the plant extracts in the present study do not have the appropriate potential to reduce Fe3+ to Fe0.
3.3 Determination of functional groups present
The functional groups present in the phytomediated iron nanoparticles are depicted in Fig. 3.
From Fig. 3, the peak at 3650.53 and 3400 cm−1 can be attributed to OH stretching vibrations, while the peaks at 2925, 1623.7, 1415.3 and 1024.6 cm−1 were attributed to CH2, C=C, CH, C–O–C stretching vibrations of secondary metabolites such as terpenes and terpenoids present in L. trifolia extracts which acted as capping and stabilizing agents during synthesis. The appearance of a small peak at 678 cm−1 is due to the presence of iron-carbonyl complexes (Fe–C=O) which confirmed the presence of secondary metabolite coating in the nanoparticles [42]. The results indicate that the plant polyphenols are part of the components in the iron nanoparticles and besides clinging on the surface of the particles they act as capping agents. Similar results were observed when iron nanoparticles were synthesized with extracts from Eucalyptus tereticornis, Melaleuca nesophila, Rosemarinus officinalis and green tree extracts [41, 43].
3.4 X-ray diffractogram of iron nanoparticles
Single crystal X-ray diffractogram of iron nanoparticles synthesized are depicted in the Fig. 4.
From Fig. 4 and Table 1, the synthesized nanoparticle comprised of iron nanoparticles with a cubic crystal system. A search in the crystal data base revealed that the 2θ values at 19.87°, 20.22°, 22.88°, 28.81°, 32.73°, 35.32°, 38.45°, 40.23° and 41.08° correspond to cubic crystal system of iron nanoparticles as reported by [44, 45]. The broad amorphous background was due to the secondary metabolites coating surrounding the iron nanoparticles which explains their role as capping agents [46]. At low FeNPs concentrations, the iron peaks are masked in XRPD due to a large amorphous background which impart the non-crystalline phases to the nanoparticles [36]. Similar observations have been made in a study in which identification of silver nanoparticles encapsulated with a silica shell with powder XRD was difficult due to the presence of an amorphous background [47, 48]. Hence the dried powder of Fe–P NPs, which was prepared using L. trifolia extracts were organic and amorphous in nature [41].
3.5 TGA and DTGA of iron nanoparticles
The thermal property of iron nanoparticles was evaluated using thermal gravimetric analyzer (TGA) and DTGA and the thermograms are depicted in Fig. 5.
From Fig. 5, an initial weight loss observed at 100 °C was attributed to loss of residual water adsorbed on the surface of the particles. The second degradation step centered at 250 °C in DTGA can be linked to the decomposition of the organic layer around the particles. This decomposition makes the main peak in the DTGA curve which has been reported to be present as phyto mediated synthesis of nanoparticles affords them an organic capping layer [33, 49].
3.6 Size distribution, zeta potential and poly-dispersibility index
The size distribution, zeta potential and polydispersibility index were determined by dynamic light scattering (DLS) and the results are depicted in Fig. 6.
The results show that the average size of particle synthesized using L. trifolia extracts was in the range between 150 and 700 nm in diameter. DLS measures the hydrodynamic diameter, which is the diameter of the particle plus ions or molecules that are attached to the surface and moves with the FeNPs in solution. The zeta potential and polydispersibility index of a given solution are important parameters that can be used to predict the stability and molecular mass distributions of nano emulsions. The value of zeta potential is related to the short- and long-term stability of emulsions where by émulsions with a high zeta potential (negative or positive) are electrically stabilized while emulsions with low zeta potentials tend to coagulate or flocculate, possibly leading to poor physical stability [50]. In this study, the PDI of synthesized nanoparticle was found to be 0.5607 ± 0.045 and Zeta potential was found to be − 0.10 ± 0.08 indicating that the particles tended to flocculate.
3.7 TEM analysis of iron nanoparticles
TEM micrographs of iron nanoparticles are depicted in Fig. 7.
From TEM micrographs, it was observed that the particles were aggregated possibly due to drying after synthesis, but an organic coating could be observed around them. Presence of this organic coating affords the amorphous nature of the nanoparticles which resulted to a large amorphous background in the diffractograms. Presence of aggregates posed a challenge in size determination of green synthesized nanoparticles as absence of single particles meant that use of image processing software wasn’t possible though those that were measured lied between 200 and 500 nm. Biosynthesized FeNPs were aggregated like grapes which was attributed to different components and concentrations of polyphenols in L. trifolia plant extracts, that played a key role in dictating the final structures and size of the nanoparticles [41].
3.8 Photocatalytic activity
The effect of reaction time, temperature and amount of iron nanoparticles on Congo red degradation were evaluated and the results are depicted in Fig. 8 and figures S2–S4.
From Fig. 9 Table 2, degradation of Congo red dye using iron nanoparticles synthesized in this study was found to be dependent on the contact time between the nanoparticles and the temperature of the reaction media (Figure S3). With an increase in the temperature and time of the reaction, there was a subsequent increase in the rate of the reaction (Table 2) and percent degradation. At higher reaction temperatures, the nanoparticles were able to degrade Congo red dye by 91 ± 0.03% as compared to lower reaction temperature 72 ± 0.05%. The reaction temperature also influenced the degradation rate as at higher temperatures the rate of the first order reactions was high (Table 2). The disappearance of the peak at 496 nm suggested that the nanoparticles effectively degraded CR dye [32]. This observation is consistent with previous findings in which the degradation of malachite green using Bacillus cereus KM201428 was investigated [32]. The results obtained in this study at 30 °C were used to determine the order of CR degradation and the rate constants for the degradation of Congo red are depicted in Table 2. The results show that degradation of CR dye using iron nanoparticles synthesised using L. trifolia extracts follow first order reaction kinetics since the correlation coefficient was highest for this model [32]. From the Van’t Hoff plot of In K versus 1/T the degradation of Congo red was found to be an endothermic reaction since as the temperature increased the equilibrium constant for the reaction at the specified temperature also increased [51]. In the presence of H2O2, iron oxide nanoparticles are able to genereate OH· and O· radicals which are able to catalyze the degradation of organic dyes in solution.
4 Conclusion
Lantana trifolia extracts possess secondary metabolites that have a good redox potential that are able to reduce ferric chloride solution to corresponding iron nanoparticles which are further capped. Analysis of the synthesized nanoparticles revealed present of iron crystal structure that have been reported in literature and they comprised of an amorphous structure which was observed in diffractograms. Aggregation of the nanoparticles after drying led to an overall increase in the size of the nanoparticles as revealed by TEM analysis which also aided in the observation of capping as a result of presence of secondary metabolites. Degradation of Congo red dye followed a first order reaction rate which was greatly influenced by the temperature of the reaction media.
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Acknowledgements
The authors take this opportunity to acknowledge the National research fund, AFRICA-ai-JAPAN Project JFY 2018/2019, Jomo Kenyatta University of Agriculture, and Technology for their financial support and the Federal Swiss Government Scholarship for a 1-year research scholarship to the University of Fribourg under Prof. Katharina M. Fromm.
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Madivoli, E.S., Kareru, P.G., Gachanja, A.N. et al. Phytofabrication of iron nanoparticles and their catalytic activity. SN Appl. Sci. 1, 879 (2019). https://doi.org/10.1007/s42452-019-0951-0
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DOI: https://doi.org/10.1007/s42452-019-0951-0