Abstract
Oak bark, which is commonly used in the wood industry, has by-products often repurposed as fuel. Its extracts are rich in compounds with anticancer, antibacterial, antifungal, and anti-inflammatory properties. This study synthesized platinum nanoparticles (PtNPs) using aqueous extracts from Quercus dalechampii (QD), Q. frainetto (QF), and Q. petraea (QP). Key factors during nanoparticle formation included reaction time, metal ion concentration, pH, extract-to-metal ion ratio, and temperature. The PtNPs were characterized by dynamic light scattering, Fourier transform infrared spectroscopy, and transmission electron microscopy. The average diameters were 58.5 ± 7.6 nm for QD-PtNPs, 41.6 ± 5.4 nm for QF-PtNPs, and 41 ± 5.3 nm for QP-PtNPs. Antioxidant and antimicrobial activities were also analyzed. The QP-PtNPs had the highest DPPH (2,2-Diphenyl-1-picrylhydrazyl), FRAP (Ferric Reducing Antioxidant Power), and CUPRAC (Cupric Reducing Antioxidant Capacity) free radical scavenging activities, while QD-PtNPs excelled in ABTS (2,2′-azinobis-(3-ethylbenzothiazoline-6-sulfonic acid)) scavenging. All PtNPs showed strong antimicrobial properties, particularly against Enterococcus faecalis, Escherichia coli, Candida krusei, and Candida auris. These findings suggest that Quercus-mediated PtNPs have significant potential for developing treatments against bacterial and fungal infections, with promising applications in medicine.
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Green Synthesis of Platinum Nanoparticles Using Aqueous Bark Extract of Quercus sp. for Potential Antioxidant and Antimicrobial Applications
Năstaca-Alina Coman,a Lavinia Berta,b,* Alexandra Nicolae-Maranciuc,c,d Alexandru Nicolescu,e Mihai Babotă,e,f Adrian Man,g Dan Chicea,c Lenard Farczadi,h László Jakab-Farkas,i and Corneliu Tanase f,j
Oak bark, which is commonly used in the wood industry, has by-products often repurposed as fuel. Its extracts are rich in compounds with anticancer, antibacterial, antifungal, and anti-inflammatory properties. This study synthesized platinum nanoparticles (PtNPs) using aqueous extracts from Quercus dalechampii (QD), Q. frainetto (QF), and Q. petraea (QP). Key factors during nanoparticle formation included reaction time, metal ion concentration, pH, extract-to-metal ion ratio, and temperature. The PtNPs were characterized by dynamic light scattering, Fourier transform infrared spectroscopy, and transmission electron microscopy. The average diameters were 58.5 ± 7.6 nm for QD-PtNPs, 41.6 ± 5.4 nm for QF-PtNPs, and 41 ± 5.3 nm for QP-PtNPs. Antioxidant and antimicrobial activities were also analyzed. The QP-PtNPs had the highest DPPH (2,2-Diphenyl-1-picrylhydrazyl), FRAP (Ferric Reducing Antioxidant Power), and CUPRAC (Cupric Reducing Antioxidant Capacity) free radical scavenging activities, while QD-PtNPs excelled in ABTS (2,2′-azinobis-(3-ethylbenzothiazoline-6-sulfonic acid)) scavenging. All PtNPs showed strong antimicrobial properties, particularly against Enterococcus faecalis, Escherichia coli, Candida krusei, and Candida auris. These findings suggest that Quercus-mediated PtNPs have significant potential for developing treatments against bacterial and fungal infections, with promising applications in medicine.
DOI: 10.15376/biores.19.4.8621-8641
Keywords: Biosynthesis; Platinum nanoparticles; Quercus; Rhytidome; Phenolic compounds; Antioxidant activity; Antibacterial activity; Antifungal activity
Contact information: a: Doctoral School of Medicine and Pharmacy, “George Emil Palade” University of Medicine, Pharmacy, Sciences and Technology of Târgu Mures, Târgu Mures, Romania; b: Department of General and Inorganic Chemistry, “George Emil Palade” University of Medicine, Pharmacy, Sciences and Technology of Târgu Mureș, 540139 Târgu Mureș, Romania; c: Research Center for Complex Physical Systems, Faculty of Sciences, Lucian Blaga University of Sibiu, 550012 Sibiu, Romania; d: Institute for Interdisciplinary Studies and Research (ISCI), Lucian Blaga University of Sibiu, 550024 Sibiu, Romania; e: Department of Pharmaceutical Botany, Faculty of Pharmacy, “Iuliu Hatieganu” University of Medicine and Pharmacy, 400337 Cluj-Napoca, Romania; f: Research Center of Medicinal and Aromatic Plants, “George Emil Palade” University of Medicine, Pharmacy, Sciences and Technology of Târgu Mures, 540139 Târgu Mures, Romania; g: Department of Microbiology, Faculty of Medicine, “George Emil Palade” University of Medicine, Pharmacy, Sciences and Technology of Târgu Mures, 540139 Târgu Mures, Romania; h: Chromatography and Mass Spectrometry Laboratory, Center for Advanced Medical and Pharmaceutical Research, “George Emil Palade” University of Medicine, Pharmacy, Sciences and Technology of Târgu Mures, 540139 Târgu Mures, Romania; i: Faculty of Technical and Human Sciences, Sapientia Hungarian University of Transylvania, 540485 Târgu Mureș, Romania; j: Department of Pharmaceutical Botany, Faculty of Pharmacy, “George Emil Palade” University of Medicine, Pharmacy, Sciences and Technology of Târgu Mures, 540139 Târgu Mures, Romania;
*Corresponding author: lavinia.berta@umfst.ro
GRAPHICAL ABSTRACT
INTRODUCTION
In recent years, there has been a growing interest in the formation of platinum nanoparticles (PtNPs) (Bhardwaj et al. 2020) due to their ability to fight bacteria (Eltaweil et al. 2022), as well as their anticancer (Bendale et al. 2017), catalytic (Karim et al. 2019), and antioxidant effects (Gupta and Chundawat 2019). Conventional techniques for their production usually require chemical procedures that involve high energy consumption or the use of harmful substances. Furthermore, PtNPs have been utilized in the creation of chemotherapy medications, such as carboplatin, cisplatin, and oxaliplatin, which are administered for treating forms of cancers such as ovarian cancer (Zeeshan et al. 2014). Nevertheless, these medications often lead to adverse effects in patients including kidney damage, nerve damage, and cell toxicity (Bendale et al. 2017). These adverse effects could potentially be mitigated by utilizing a biosynthesis method for producing PtNPs. The biosynthesis process of PtNPs mainly involves plants, bacteria, and fungi. The synthesis of metal nanoparticles from plant extracts is preferred, because it is faster and more ecological than that from fungi and bacteria (Siddiqi et al. 2018). The presence of flavonoids, protein-amine residues, and carboxylic acids in plants play a role, in reducing platinum ions to form PtNPs (Castro et al. 2015). Biosynthesized PtNPs have many advantages, they are used in different fields, especially the pharmaceutical and biomedical fields, because of their compatibility with living organisms, ecological sustainability, and cost-effectiveness (Jiao et al. 2021; Zhang et al. 2023). Platinum nanoparticles (PtNPs) synthesized through green methods have demonstrated remarkable efficiency in inhibiting the growth of bacterial pathogens (Dhiman et al. 2021). For instance, the synthesis of PtNPs using extracts from Citrus hystrix DC., Ocimum basilicum Linn., and Pandanus amaryllifolius Roxb. produced nanoparticles with spherical morphologies and sizes ranging from 20 to 80 nm (Ponsanti et al. 2024). Recently, it has been shown that the peroxidase-like catalytic activity of PtNPs can be utilized for colorimetric detection methods of biomarkers, with a detection limit of 7.00 μM (Marvi et al. 2024). Additionally, PtNPs synthesized using extracts from Salvia rosmarinus and Panax ginseng have induced cell death in colon cancer cell lines, with PCR analysis of autophagy and apoptosis markers indicating a significant influence of the nanoparticles (Alinaghi et al. 2024). These examples highlight the considerable potential of PtNPs synthesized through green methods in biomedical and diagnostic applications, thereby underscoring the importance of our research in using Quercus extracts for the synthesis and stabilization of these nanoparticles.
Oak bark, sourced from Quercus dalechampii (QD), Q. frainetto (QF), and Q. petraea (QP) trees, are commonly utilized in the timber sector with their byproducts often repurposed for fuel (Tanase et al. 2023; Tsiripidis and Athanasiadis 2003).
To our knowledge, there is no evidence that extracts of Q. dalechampii, Q. frainetto, and Q. petraea have been used to synthesize platinum nanoparticles (PtNPs). In a previously published study, the authors demonstrated that oak bark extract is rich in polyphenols and flavonoids, having remarkable antibacterial and antifungal properties (Coman et al. 2024). This suggests that the use of this extract for the biosynthesis of PtNPs could lead to nanoparticles with activity significant antimicrobial. Additionally, oak bark is an abundant and sustainable material, making its use in nanoparticle synthesis both environmentally friendly and cost-effective. By highlighting these distinctive aspects of oak bark extract, the aim here is to emphasize the importance and relevance of this study in the current context of nanoparticle research. Thus, the main objectives of this study were: (1) biosynthesis of PtNPs using oak bark extracts as a natural resource; (2) to investigate the impact of key factors on the biosynthesis process of PtNPs, including variations in the concentration of H2PtCl6 (0.5, 1.0, and 5 mM), pH levels (7.5, 8, 9, and 10), the ratio of bark extract to H2PtCl6 (1:9, 2:8, 1:19), and temperature fluctuations (50 °C, 70 °C and 80 °C); (3) characterization of biosynthesized PtNPs by specific analyses; and (4) evaluate the antioxidant, antibacterial, and antifungal properties of the synthesized PtNPs.
EXPERIMENTAL
Plant Material
Bark fragments of Q. dalechampii, Q. frainetto, and Q. petraea were collected from mature trees (35 to 40 years old, 18 to 25 cm circumference at breast height) from the Zagra area of Bistrița Năsăud county, Romania. The species’ authenticity was confirmed by Dr. Corneliu Tănase from the Department of Pharmaceutical Botany at the Faculty of Pharmacy G. Emil Palade University of Medicine and Pharmacy, Târgu Mureș, Romania. The collected bark was air dried in a Nahita 631 drying oven at 50 °C for a day. Then, it was pulverized using a Pulverisette 15 cutting mill from Fritsch GmbH, Idar Oberstein, Germany. This powdered material was left unprocessed and deposited in the Research Center for Medicinal and Aromatic Plants, Târgu Mureș, Romania until further extraction procedures were performed.
Chemicals and Reagents
Potassium hexachloroplatinate(II) hexahydrate (K2PtCl6.6H2O, 99.9%), sodium hydroxide (NaOH), DPPH (2,2-diphenyl-1-picrylhydrazyl), ABTS (2,2′-azinobis(3-ethylbenzothiazoline-6-sulfonic acid)), FRAP (Ferric Reducing Ability of Plasma), CUPRAC (Cupric Ion Reducing Antioxidant Capacity), NR (neutral red) solutions were purchased from Sigma-Aldrich in Steinheim, Germany. Dimethyl sulfoxide (DMSO), and Folin-Ciocâlteu reagent were obtained from Merck (Darmstadt, Germany).
Microorganisms
Staphylococcus aureus ATCC 25923 and ATCC 43300, Enterococcus faecalis ATCC 29212, Escherichia coli ATCC 25922, Klebsiella pneumoniae ATCC 13883, Pseudomonas aeruginosa ATCC 27853, Candida albicans ATCC 10213, Candida krusei ATCC 6258, and Candida auris ATCC 10913 were obtained from the Department of Microbiology at the University of Medicine, Pharmacy, Sciences and Technology “George Emil Palade”, Târgu Mureș, Romania.
Preparation of Bark Extracts
Extraction was performed with distilled water at a ratio of 1:10, as previously described (Tanase et al. 2020). In short, 10 g of oak bark was put in a flask with 100 mL of water, ensuring thorough saturation of the plant material. The extraction process was conducted at a temperature of 60 °C for 30 min. Polyphenolic substances were obtained using an ultrasonic water bath (Professional Ultrasonic Cleaner MRC from Beijing, China) with the following settings: AC 150 H, 150 W, 40 kHz, and heating power 300 W. After extraction, the resulting extracts were filtered and centrifuged at a speed of 10,000 revolutions/min for about 10 min. The supernatant was used for the experiment. The extracts were used directly without any processing for the synthesis of PtNPs.
Chemical Characterization of Bark Extracts
Qualitative analysis of bark extracts
An UHPLC analysis (Ultra-High-Performance Liquid Chromatography) of the polyphenolic compounds was detailed by Tanase et al. (2018). The analysis utilized a Perkin Elmer UPLC Flexar FX 10 system, which included components, like a pump, inline degasser, autosampler, column thermostat, and a Flexar FX PDA UHPLC detector. High quality liquid chromatography-mass spectrometry (LC–MS)/MS grade solvents and the purest reagents available were used throughout the process. Samples were injected into a Luna C18 (2) column (3 µm particle size, 150 mm × 4.6 mm) at a flow rate of 1.0 mL/min. Elution was carried out using a gradient of 0.1% formic acid (phase A) and acetonitrile (phase B) with monitoring at 280 nm. Compound identification was achieved by comparing retention times and ultraviolet-visible(UV–Vis) spectra with reference standards. Before analysis all extracts underwent filtration through a 0.45-µm microporous cellulose syringe filter. UHPLC was used both to identify and quantify specific compounds from the extracts used and to identify and quantify the compounds remaining after the synthesis of PtNPs. It is important to determine the chemical composition of the extract and to understand how these compounds influence the synthesis and properties of the nanoparticles.
Quantitative Analysis of Bark Extracts
The method used to calculate total polyphenol content (TPC) from extracts and from nanoparticles followed the Folin Ciocalteu method adapted for the microplate reader, as described by Babota et al. (2021). The absorbance of the samples was measured at 760 nm after a 30 min incubation at room temperature. Results are expressed in mg gallic acid equivalents (GAE) per gram weight (dw) of lyophilized extract/nanoparticles (mg GAE/g dw). Gallic acid was used as a standard and each sample was measured in triplicate.
Biosynthesis of PtNPs Using Polyphenolic Extracts
The synthesis of PtNPs was monitored and optimized by recording the UV-Vis spectra of the reaction mixtures in the wavelength range of 250 to 450 nm (Tanase et al. 2019) on a Specord 210 Plus 190 spectrophotometer (Analytik Jena, Jena, Thuringia, Germany). To enhance the production efficiency of PtNPs, various parameters were adjusted during the synthesis, including the pH levels (7.5, 8, 9, and 10), H2PtCl6 concentration (0.5, 1.0, and 5 mM), ratio of bark extract to H2PtCl6 (1:9, 2:8, 1:19), temperature variations (50, 70, and 80 °C) and different reaction durations (30, 60, 90, and 120 min). The pH level was regulated using NaOH solution at a concentration of 1.0 mM. After finishing the optimization studies, the synthesis of PtNPs was performed using the optimal parameters. The solutions of QD-PtNPs, QF-PtNPs, and QP-PtNPs were freeze dried using a BK-FD12S freeze dryer (Biobase Biodustry Co., Ltd., Shandong, China). The pellets of QD-PtNPs, QF-PtNPs, and QP-PtNPs were then stored at +4 °C until use.
Characterization of PtNPs
The PtNPs were examined using Fourier transform infrared spectroscopy (FTIR), dynamic light scattering (DLS), and transmission electron microscopy (TEM). Attenuated total reflectance-FTIR (ATR-FTIR) spectroscopy (Bruker Alpha-P ATR FTIR spectrometer, Bruker, Ettlingen, Germany) was used to identify functional groups on the surface of PtNPs, which are part of compounds found in bark extracts that serve as coating or stabilizing agents. Briefly, the freeze-dried extracts and PtNPs pellets were subjected to ATR-FTIR spectroscopy in the range of 4000 to 400 cm⁻¹ with a resolution of 4 cm⁻¹ (Chicea et al. 2023). The morphology and size of the PtNPs were studied through TEM and DLS analyses. Thus, PtNPs solution was used for TEM and DLS analyses. Briefly, for TEM analysis, a drop of each PtNPs was placed on carbon coated copper grids (300 mesh). The specimens were vacuum dried for 24 h, at room temperature (Tanase et al. 2019). The size of the synthesized PtNPs was determined using DLS, where a beam of light is directed at particles suspended in a solvent to generate patterns that are captured by a detector (Chicea et al. 2024).
Assessment of Antioxidant Activity for PtNPs
The antioxidant potential of synthesized PtNPs was evaluated by DPPH, ABTS, FRAP, and CUPRAC reagents using the procedures described by Babota et. al. (2022) and Mocan et al. (2016). The QD-PtNPs, QF-PtNPs, and QP-PtNPs were dissolved in a mixture of 50% ethanol with 5% DMSO to obtain a concentration of 1.0 mg/mL, which was then further diluted. Subsequently, samples were assessed in 96 well plates using a SPECTROstar® Nano Multi-Detection microplate reader, from BMG Labtech located in Ortenberg, Germany.
DPPH radical scavenging assay
This assay involved mixing 30 μL of each sample with a 0.004% methanol solution of 1,1-diphenyl-2-picrylhydrazyl reagent. After an incubation period of 30 min, at room temperature in the dark the absorbance was measured at 517 nm. The outcomes of DPPH scavenging activity were reported as mg of Trolox equivalents per gram of freeze-dried powder (mg TE/g dw) (Babotă et al. 2018).
ABTS radical scavenging assay
A 7 mM 2,2′-azino-bis(3-ethylbenzothiazoline) 6-sulfonic acid solution was mixed with 2.45 mM potassium persulfate. It was left to stand in the dark at room temperature for 12 to 16 h. Before conducting the test, the ABTS solution was diluted with water until it reached an absorbance of 0.700 ± 0.02 at 734 nm. The diluted samples were then combined with the ABTS solution. Then, it was mixed thoroughly. After a 30 min incubation period at room temperature, the absorbances of the samples were measured at 734 nm. The results of the ABTS scavenging activity were reported as milligrams of Trolox equivalents, per gram of freeze-dried powder (mg TE/g dw).
FRAP activity
The ferric reducing antioxidant power testing was accomplished through the combination of 25 µL of the sample with 175 µL of the FRAP reagent. The resulting mixture was left to incubate for 30 min at room temperature, following which the absorbance was measured at 593 nm. The prepared FRAP reagent consisted of a blend of buffer (300 mM, pH 3.6) TPTZ solution (10 mM TPTZ in 40 mM HCl), and FeCl3 solution (20 mM FeCl3·6H2O in 40 mM HCl) in specific proportions. The outcomes were stated as milligrams of Trolox equivalents, per gram of freeze-dried powder (mg TE/g dw).
CUPRAC assay
A modified protocol of previously reported method (Özyürek et al. 2011) was used. During this process each sample was mixed with a solution containing CuCl2, neocuproine, and ammonium acetate at a pH level of 7.0. Following a 30 min waiting period the absorbance of the mixture was gauged at 450 nm. The findings were then expressed as milligrams of Trolox equivalents, per gram of freeze-dried powder (mg TE/g dw).
Assessment of Antimicrobial Activity for PtNPs
The effectiveness of QD-PtNPs, QF-PtNPs, and QP-PtNPs, against bacteria was assessed through the microdilution technique following a previously described method (Tanase et al. 2018; Coman et al. 2023) with slight modifications. The study measured the efficacy of PtNPs pellets by determining minimum inhibitory concentration (MIC, required for microbial growth inhibition) and fungicidal concentrations (MFC) using a method known as microdilution. Briefly, 150 mg of lyophilized material was mixed with 15 mL of 5% DMSO solution (concentration of 10 mg/mL). After, 200 µL of this solution was added to the wells of the first column of a 96-well plate. The solutions were then diluted using distilled water (final volume 100 µL) followed by the addition of 100 µL of bacterial / fungicidal suspension to each well. Each substance and bacterial/fungal strain were tested three times for accuracy. The microdilution plates were placed in an incubator at 37 °C for a period of 24 h. The MIC or MFC were assessed in wells where there was no bacterial growth or fungal growth by optical examination.
Statistical Analysis
Statistical analysis was performed with GraphPad Prism 8 (GraphPad Software, San Die-go, CA, USA). The significance level chosen was α = 0.05. The normality of data distribution was checked using the Shapiro-Wilk test. The TPC and antioxidant activity was performed using the one-way analysis of variance (ANOVA) test, and Tukey’s post hoc test was used to compare groups. Any p value < 0.05 was considered significant.
RESULTS AND DISCUSSION
Chemical Characterization of Bark Extracts
The aqueous extracts obtained were characterized by UV-Vis spectroscopy (Fig. 1a). The maximum absorption for the Q. dalechampii extract was at 272 nm, for the Q. frainetto extract at 277 nm, and for the Q. petraea extract at 274 nm. The aqueous extracts were also examined to determine the total content of phenolic compounds (TPC) and the specific components present in the extracts. As a result, Q. dalechampii showed a TPC value of 402 mg GAE/g extract, while Q. frainetto showed 438 mg GAE/g extract, and Q. petraea had 325 mg GAE/g extract. The collected samples were initially examined to identify the characteristics and possible applications of these substances. As illustrated in Supplementary Table S1, ellagic acid appeared as a component in the tested samples with concentrations of 1480 μg/mL in Q. dalechampii, 8080 μg/mL in Q. frainetto, and 4900 μg/mL in Q. petraea. Another predominant compound in Q. dalechampii was quercetin (124 μg/mL), while epicatechin (162 μg/mL) was prominent in Q. frainetto and gallic acid (40.79 μg/mL) stood out in Q. petraea. Phenolic compounds and compounds identified from Quercus extracts act as reducing agents in the biosynthesis process of PtNPs. By providing the necessary electrons, these compounds contribute to the reduction of platinum ions (Pt2+) to their zero-valent state (Pt0), thereby facilitating the biosynthesis of nanoparticles. This refers to the transformation of platinum ions from a positive oxidation state to a neutral, metallic state. In the green biosynthesis process of platinum nanoparticles, compounds in plant extracts, such as polyphenols and flavonoids, act as efficient reducing agents, donating electrons to the platinum ions and reducing them to the zero-valent state (Pt0). In addition to their reducing role, phenolic substances also have a role in maintaining the colloidal stability of PtNPs. Because of their chemical groups, these substances can bind to the surface of the nanoparticles, which prevents agglomeration, keeps the nanoparticles evenly dispersed in the solution, ensuring that they remain stable for a long time. Also, components found in Quercus extracts can influence the shapes and sizes of PtNPs created through biosynthesis (Nasrollahzadeh et al. 2020; Salem et al. 2021).
Fig. 1. UV spectrum of the aqueous solution of Q. dalechampii, Q. frainetto, Q. petraea (a) and the solution of K2PtCl6 (b)
Optimization of Synthesis Parameters
The formation process of QD-PtNPs, QF-PtNPs, and QP-PtNPs involved a crucial optimization step, where several parameters were investigated and adjusted. Among these parameters were included: the concentration of the K2PtCl6 solution, the pH of the solution, the ratio of extract:K2PtCl6 solution, and the temperature of nanoparticle formation. The PtNPs formation was tracked by noting the shift in color of the mixture during the reaction. The initial light-yellow color transitioned (Fig. 2b) to dark brown (Fig. 2c) as the reaction advanced. This alteration in color signifies the transformation from Pt(IV) to Pt(II) and Pt(II) to Pt(0), indicating the creation of PtNPs. The change in color observed is believed to be linked to the surface response of Metal-NPs caused by the movement of electrons, on its surface (Nishanthi et al. 2019).
Fig. 2. Color shift during reaction: 1mM K2PtCl6 solution and Q. frainetto extract (Fig. 2a), solution color at time T0 (Fig. 2b), color shift to dark brown as the reaction progressed (Fig. 2c)
Determination of the Optimal Concentration of the Reducing Agent and K2PtCl6 / Extract Ratios
The first step studied in the formation of QD-PtNPs, QF-PtNPs, and QP-PtNPs determined the concentration of the K2PtCl6 solution. Initially, 2 mL of the extract was mixed with 18 mL of K2PtCl6 at different concentrations (0.1, 1, and 5 mM), at initial pH. Afterwards, the mixture was ultrasonicated in a bath at 70 °C for 2 h. The formation of PtNPs were validated using UV-Vis spectroscopy. The absorption spectra of the precursor platinum (Pt) salts displayed a peak at 262 nm, which occurred due to the dissociation and formation of 2H+ and PtCl62- in water (Fig. 1b). Upon introducing Q. dalechampii, Q. frainetto, and Q. petraea extracts, the plasmon peak of the Pt salt vanished, indicating a reduction of the Pt salt to zero valent platinum (Fig. 3). The experiments conducted indicated that using a higher concentration of K₂PtCl₆ (5 mM) inhibited the synthesis process, as shown in Fig. 3. This phenomenon is due to several interdependent factors. At high concentrations, the rapid increase in nucleation can lead to the formation of a large number of nanoparticle nuclei in a very short time, causing particle aggregation due to frequent collisions between nuclei. This inhibits the formation of uniform and stable nanoparticles (Rehman et al. 2022). Additionally, high concentrations of platinum ions can generate an ionic screening effect, where the extra ions in the solution reduce the efficiency of reducing and stabilizing agents, slowing down or completely inhibiting the reduction process of platinum ions to zero-valent platinum atoms (Pt0), which are essential for nanoparticle formation (Fahmy et al. 2020). Similar effects were observed when using higher ratios of K2PtCl6/extract (1:19) as shown in Fig. 3. Therefore, it was determined that the ratio of 1:4 mL extract/mL K2PtCl6, at a concentration of 1 mM along with a reaction time of 2 h represented the conditions to produce QD-PtNPs and QP-PtNPs. In contrast, for QF-PtNPs biosynthesis a ratio of 1:9 mL extract/mL K2PtCl6 at a concentration of 1 mM with a reaction time of 2 h were the suitable conditions.
Fig. 3. Effect of K2PtCl6 concentration, ratio between the volumes of plant extract, and K2PtCl6 on the synthesis of QD-PtNPs (A, D), QF-PtNPs (B, E), and QP-PtNPs (C, F)
Determining the Optimal Temperature and pH
After establishing the K2PtCl6 concentration and ratio, another important factor studied in the formation of PtNPs was the solution temperature and pH. Temperature is one of the most important factors for nanoparticle synthesis of the extraction medium. The formation of PtNPs did not occur at low temperatures, and the color of the solution remained unchanged. However, a noticeable shift in color was seen as the temperature rose slowly to 70 °C. Additionally the vanishing of the peak at 260 nm suggested the creation of PtNPs (Fig. 4). As the temperature reached 80 °C, the solution clouded over and transitioned from brown to black. This change also occurred with the increased time spent in the bath, possibly indicating the aggregation of nanoparticle clusters of various sizes. The solution became turbid as the aggregated nanoparticles grew in size, leading to increased light scattering in the solution. Nanoparticle aggregation can be caused by van der Waals interactions between particles, which become more pronounced as the reaction time increases. This phenomenon is well-documented in the literature, highlighting the importance of controlling synthesis time to prevent aggregation and maintain the colloidal stability of nanoparticles (Latif et al. 2018; Stavinskaya et al. 2019). Another important factor studied in the formation of PtNPs was the pH of the solution. It plays a role in the plant mediated production of nanoparticles impacting their size, shape, and synthesis rate. The increase in pH is linked to a rise in nucleation centers formation, which influences the reduction of metal ions into metal nanoparticles. Moreover, as the pH level rises there is an increase in core center expansion and electron donation due to protonation deprotonation effects. Additionally, the solutions’ pH level regulates the functionality of groups, within the plant extract, which ultimately determines how quickly metal salt reduction occurs (Jameel et al. 2020). The effect of pH on PtNPs synthesis was investigated at pH = 7.5; pH = 8; pH = 9, and at pH = 10. The results indicate that PtNPs formation occurred rapidly in a basic environment (pH 10) compared to a neutral solution (pH 7.5). In general, the synthesis of PtNPs increases with alkalinity levels in the dispersion medium. Thus, in the case of QD-PtNPs and QF-PtNPs pH 10 is the most favorable, in contrast, in the case of QP-PtNPs a pH 9 being the most favorable. Increasing time had no significant effect on PtNPs synthesis at different pHs, but PtNPs synthesis reached equilibrium after 2 h. The findings were supported by Nishanthi et al. (2019) and Soundarrajan et al. (2011). Nishanthi et al. (2019) examined how varying pH levels (4 to 8) impacted the PtNPs synthesis with Garcinia mangostana L. peel extract. Thus, at acidic pH (pH of 4) it led to the formation of larger PtNPs, while at alkaline pH (pH 10) it led to the formation of smaller PtNPs (Nishanthi et al. 2019). Soundarrajan et al. (2011) utilized Ocimum sanctum plant leaf extract for PtNPs synthesis at elevated temperatures highlighting that higher temperatures are optimal for PtNPs formation. The resulting PtNPs measured a size of 23 nm and exhibited irregular shapes (Soundarrajan et al. 2011).
Fig. 4. Effect of temperature and pH on the synthesis of QD-PtNPs (A, D), QF-PtNPs (B, E), and QP-PtNPs (C, F)
Following the optimization process, three solutions of PtNPs were obtained. These solutions were: QD-PtNPs (ratio 1:4 mL extract/mL K2PtCl6 at a concentration of 1 mM, pH 10, at 70 °C), for QF-PtNPs (ratio 1:9 mL extract/mL K2PtCl6 at a concentration of 1 mM, pH 10, at 70 °C), and QP-PtNPs (ratio 1:4 mL extract/mL K2PtCl6 at a concentration of 1 mM, pH 9, at 70 °C). After synthesizing the platinum nanoparticle (PtNPs) solutions, they were lyophilized to remove the water content, a process that significantly contributes to the stabilization of the chemical structure and the prevention of degradation. Lyophilization thus ensures effective preservation of the intrinsic properties of the nanoparticles. The resulting dry matter was then used for detailed assessments of biological activity, enabling accurate and reproducible analyses in laboratory studies. This method is essential for maintaining the integrity of compounds during testing and subsequent application in various biomedical fields.
Characterization of PtNPs
After determining the optimal conditions mentioned above, additional analytical techniques were employed to ensure the formation and quality of the PtNPs. Transmission Electron Microscopy (TEM) confirmed the morphology and uniform size of the nanoparticles. Dynamic Light Scattering (DLS) measured the size distribution and ensured colloidal stability, while Fourier Transform Infrared Spectroscopy (FTIR) verified the chemical composition and the presence of functional groups on the nanoparticle surface, confirming their stability. Additionally, the obtained PtNPs were acquired underwent an examination, during which the overall quantity of polyphenols was assessed utilizing the Folin Ciocalteu technique. Further, the substances found in Quercus extracts and generated during the biosynthesis of PtNPs were identified through high-performance liquid chromatography (HPLC). These investigations provided insights into the composition and characteristics of PtNPs, along with the significance of polyphenols in the biosynthesis procedure and their possible uses.
Another important role of extractive materials is to act as stabilizers for nanoparticles, preventing their collision and aggregation. In this study, the bioactive compounds present in the extracts of Q. dalechampii, Q. frainetto, and Q. petraea significantly contributed to the stabilization of platinum nanoparticles (PtNPs). These compounds, such as polyphenols, tannins, and flavonoids, adsorb onto the surface of the nanoparticles, forming a protective layer that prevents their aggregation and keeps them well dispersed in solution. Efficient stabilization of nanoparticles is essential for maintaining their functional properties and ensuring optimal biological activity.
The FTIR analyses were performed to identify the biomolecules involved in the reduction of Pt2+ ions and the synthesis of PtNPs in the three different extracts. The FTIR spectra for each extract and the PtNPs synthesized with them are shown in Fig. 6 for a more accurate comparison and better identification of features. The observations suggest that the PtNPs synthesized using the extracts had similar chemical groups, highlighted by similar peaks in the spectra. The intense peaks between 3500 to 3200 cm-1 (peaking at 3294 cm-1 for QD-PtNPs, 3316 cm-1 for QF-PtNPs, and 3253 cm-1 for QP-PtNPs) are associated with the vibrations of O-H groups in the organic phase of the extracts, due to the abundant presence of polyphenolic structures in them (Nandiyanto et al. 2019). This connection suggests a correlation between PtNPs and all three Quercus extracts. Additionally, the peaks observed in the region 3200 to 3000 cm-1 correspond to C-H and CH2-, CH3– vibrations of polysaccharides, present in significant amounts in Quercus extracts. The absorbance bands at: 1702 cm-1 for QD-PtNPs, 1705 cm-1 for QF-PtNPs, and QP-PtNPs are attributed to C=O groups, indicating an association between PtNPs and compounds, such as quercetin, epicatechin, and gallic acid, identified in Quercus extracts. Other observations include the presence of primary amine at 1605 cm-1 and absorbance bands at 1518 and 1445 cm-1 indicate aromatic compounds. In addition, the appearance of peaks at 1372 and 1230 cm-1, especially in QD-PtNPs, suggests their formation through the interaction of the organic extract with the metal particles. Similarly, for QF-PtNPs, the absorbance peaks at 1369 and 1264 cm-1 indicate the synthesis process. In the case of QP-PtNPs, fewer peaks associated with reduction were observed, but the peaks at 1235 cm-1 confirm the interaction between the Quercus petraea extract and the metal. These observations highlight the complexity of the interactions between organic extracts and metal particles during the synthesis of PtNPs.
Figure 5 shows the TEM images and the average sizes generated by DLS of the PtNPs. In all cases, the PtNPs show a spherical and monodisperse morphology. The dimensions of QF-PtNPs and QP-PtNPs are approximately the same (41.6 ± 7.6 nm and 41 ± 5.3 nm), in contrast, the dimensions of QD-PtNPs are a bit larger, respectively 58.5 ± 7.6 nm.