ORIGINAL ARTICLE Year : 2023  |  Volume : 13  |  Issue : 7  |  Page : 315-324

Characterization and antimicrobial, antioxidant, and anti-proliferative activities of green synthesized magnesium oxide nanoparticles with shoot extracts of Plicosepalus curviflorus

Reem Hamoud Alrashoudi1, Manal Abudawood1, Ayesha Mateen1, Hajera Tabassum1, Noura Ibrahem Alghumlas1, Sabiha Fatima1, Basmah Almaarik1, Farah Maqsood2, Nawal M Al Musayeib3, Musarat Amina3
1 Clinical Laboratory Sciences Department, College of Applied Medical Sciences, King Saud University, Riyadh 12372, Saudi Arabia
2 Department of Optometry and Vision Science, College of Applied Medical Science, King Saud University, Riyadh 11451, Saudi Arabia
3 Department of Pharmacognosy, College of Pharmacy, King Saud University, Riyadh 11495, P.O. Box 22452, Saudi Arabia

Date of Submission17-May-2023Date of Decision01-Jun-2023Date of Acceptance28-Jun-2023Date of Web Publication14-Jul-2023

Correspondence Address:
Ayesha Mateen
Clinical Laboratory Sciences Department, College of Applied Medical Sciences, King Saud University, Riyadh 12372
Saudi Arabia

Source of Support: None, Conflict of Interest: None

DOI: 10.4103/2221-1691.380563

Objective: To synthesize magnesium oxide nanoparticles using ethanol extract of shoots of Plicosepalus curviflorus (PC-MgONPs) and evaluate the antimicrobial, antioxidant, and anti-proliferative activities of PC-MgONPs.
Methods: The green synthesized PC-MgONPs were characterized by ultraviolet-visible (UV), Fourier-transform infrared spectroscopy, zeta potential, energy dispersive X-ray, and scanning electron microscopy. Furthermore, we investigated total antioxidant capacity and antimicrobial and anti-proliferative activities using breast cancer cell lines (MDA-231).
Results: The UV spectrum of PC-MgONPs showed a sharp absorption peak at 300 nm. The presence of magnesium, oxygen, and sodium was confirmed by energy dispersive X-ray analysis. Scanning electron microscopy revealed PC-MgONPs as roughly spherical granular structures with sizes ranging from 20.0 to 76.4 nm. PC-MgONPs showed considerable antimicrobial activities against Escherichia coli, Staphylococcus aureus, methicillin-resistant Staphylococcus aureus, Pseudomonas aeruginosa and Candida albicans with zones of inhibition of 11-17 mm. In addition, total antioxidant capacity and anti-proliferative activity of PC-MgONPs against MDA-231 cells were dose-dependent.
Conclusions: The synthesized PC-MgONPs could be a potent antimicrobial, antioxidant and anti-cancer agent, which needs further investigation.

Keywords: PC-MgONPs; Plicosepalus curviflorus; FTIR; Antimicrobial; Cell viability; Antioxidant

How to cite this article:
Alrashoudi RH, Abudawood M, Mateen A, Tabassum H, Alghumlas NI, Fatima S, Almaarik B, Maqsood F, Al Musayeib NM, Amina M. Characterization and antimicrobial, antioxidant, and anti-proliferative activities of green synthesized magnesium oxide nanoparticles with shoot extracts of Plicosepalus curviflorus. Asian Pac J Trop Biomed 2023;13:315-24
How to cite this URL:
Alrashoudi RH, Abudawood M, Mateen A, Tabassum H, Alghumlas NI, Fatima S, Almaarik B, Maqsood F, Al Musayeib NM, Amina M. Characterization and antimicrobial, antioxidant, and anti-proliferative activities of green synthesized magnesium oxide nanoparticles with shoot extracts of Plicosepalus curviflorus. Asian Pac J Trop Biomed [serial online] 2023 [cited 2023 Jul 15];13:315-24. Available from: https://www.apjtb.org/text.asp?2023/13/7/315/380563

Significance:
Magnesium oxide nanoparticles (MgONPs) have emerged as attractive nanomaterials with diverse biomedical applications due to their distinctive physicochemical features, including biocompatibility, high stability, biodegradability, cationic capacity, and redox properties. The current study reports the synthesis of MgONPs using ethanol extract of Plicosepalus curviflorus shoot and MgONPs show antibacterial, antioxidant, and anti-proliferative activities.

  1. Introduction 

Magnesium oxide nanoparticles (MgONPs) are interesting nanomaterials with excellent surface reactivity, promising biomedical applications, remarkable stability under harsh conditions, and less harmful effects, and can be employed as economical precursors[1]. These nanomaterials have shown potential biomedical features, including, antioxidant, antimicrobial, anticancer, anti-inflammatory, anti-diabetic, bone regeneration, and analgesic effects[2],[3],[4]. MgONPs are utilized as ointments for the treatment of heart burns, wounds, and bone regeneration. These nanoparticles also exhibited excellent toxic properties against a wide range of human diseases that are resistant to many drugs[5]. Compared to other metal nanoparticles, MgONPs have many benefits, including non-toxicity, biocompatibility, cost-effectiveness, and stability, possessing important medical uses and potent antibacterial properties[6]. The Food and Drug Administration has determined that magnesium oxide (MgO) is generally recognized as safe for use in human food[7]. Moreover, recently, the Food and Drug Administration has authorized the use of magnesium sulphate injection in the treatment of preeclampsia in order to prevent seizures in patients[8].

Plicosepalus curviflorus (P. curviflorus) grows natively in Saudi Arabia, Yemen, East Africa, and Northeast Africa[9]. In Saudi Arabia, the entire plant has been used in traditional medicine to heal diabetes and in Yemen, the stem and heated twigs of this plant have been used in cancer treatment and as a poultice on the chest to cure pneumonia, respectively[10]. The flavane gallates, triterpenes, quercetin, catechin, and sterols found in the shoot extracts have antioxidant, hypoglycemic, antibacterial, cytotoxic, and anti-diabetic effects[11].

The aerial portions of P. curviflorus have been selected for green synthesis of MgONPs as the shoot part of the selected plant possesses active phenolic compounds (catechin, curviflorside, and curviflorin) with strong antibacterial and anti-proliferative activities, which we have isolated in our previous study[12]. Green synthesis of plant-based nanoparticles from metals, especially magnesium, and MgO, was used for numerous purposes[13],[14]. The study aims to synthesize MgONPs using shoot extracts of P. curviflorus (PC-MgONPs) as the above-mentioned compounds are involved in the reduction, capping, and stabilization of formed nanoparticles as well as enhancement of biological properties of biosynthesized MgONPs. The antimicrobial, antioxidant, and anti-proliferative effects of MgONPs were also evaluated.

  2. Materials and methods 

2.1. Preparation of P. curviflorus ethanol extracts

The ethanol extract was prepared by macerating dried powder of P. curviflorus shoots (500 g) in ethanol (2 L × 3, each) for 8 h using a Soxhlet apparatus at room temperature. The solvent was chosen based on its solubility, and safety, and solvents with polarity values close to solute polarity perform better extraction. The resultant ethanol extract was filtered and subsequently liberated from the organic solvent by rotary evaporation at 50 °C under decreased pressure, yielding dark green ethanol extract (14.0 g).

2.2. Green synthesis of MgONPs using biomass of P. curviflorus

The green synthesis of PC-MgONPs was carried out by adding freshly prepared 1.0 mM magnesium nitrate (1.02 g of magnesium nitrate dissolved in 100 mL of distilled water) solution into 100 mL of P. curviflorus solution (5 g dissolved in 200 mL of ethanol) and stirred continuously at 600 rpm at 80 °C for 6 h with a magnetic stirrer (HJ-3 Thermostatic Magnetic Stirrer, Jiangsu, China). Afterward, 10 mL of NaOH (1.0 M) was poured dropwise into the reaction mixture to form a precipitate. The color change from green to dark brown was used to monitor the creation of nanoparticles. The reaction mixture was then centrifuged at 5000 rpm for 15 min, the recovered precipitate was washed several times with ethanol to remove impurities, and dried PC-MgONPs (7.5 g) were calcined at 400 °C in a furnace. The mechanism of formation of PC-MgONPs was represented by the following equation:

2.3. Spectroscopic and microscopic characterization of PC-MgONPs

The formation of PC-MgONPs was confirmed by measuring the typical peak through a UV-Vis spectrophotometer at an absorption wavelength range of 200 to 800 nm (Shimadzu Corporation, Kyoto, Japan). FTIR analysis was performed to detect functional moieties and operated in a 400-4000 cm−1 spectral range (Spectrometer-vector 22, Bruker, Germany). The crystalline structure of pre-synthesized PC-MgONPs was confirmed by X-ray diffraction (XRD) using Miniflex 600, X-ray diffractometer, Holland and it was operated at 40 kV with a current of 30 mA using CuKα radiation at 2θ angle ranging from 20 °C to 80 °C. The stability and size distribution of the formed PC-MgONPs were assessed by zeta potential (ZP) and dynamic light scattering (DLS) using a particle size zeta potential analyzer based on laser light scattering (Zetasizer NS-3000, Malvern Analytical Ltd, Malvern, United Kingdom). The surface morphological features, including size, shape, and composition of PC-MgONPs, were monitored by scanning electron microscopy (SEM) equipped with energy-dispersive X-ray (EDX) spectroscopy using Zeiss SEM (Zeiss MultiSEM-505, Jena, Germany) with spectral images. Also, the elemental composition of the PC-MgONPs was estimated through EDX.

2.4. Preparation of stock solutions

The working stock solution was prepared by weighing 100 mg of P. curviflorus ethanol extracts and dissolved in dimethyl sulfoxide at a concentration of 100 mg/mL. PC-MgONPs was weighed and dissolved in a solution containing sterile distilled water and nitric acid (4.8 mL water + 0.2 mL of nitric acid) to get the concentration of 10 mg/mL. The stock solution prepared were used to evaluate cell viability, antimicrobial and total antioxidant activity.

2.5. Microbial cultures

In the present study, five microbial strains were used to evaluate antimicrobial activity and minimum inhibitory concentration (MIC) of P. curviflorus ethanol extracts and PC-MgONPs. Three ATCC (American Type Culture Collection) microbial strains were used including Escherichia coli (E. coli, ATCC 25922), Staphylococcus aureus (S. aureus, ATCC 29213) and Candida albicans (C. albicans, ATCC 10231). Two clinical isolates [methicillin-resistant S. aureus (MRSA) and Pseudomonas aeruginosa (P. aeruginosa)] were used for the antimicrobial sensitivity.

2.6. Evaluation of antimicrobial activity

2.6.1. Agar well diffusion assay

The antimicrobial activity of PC-MgONPs was performed by agar well diffusion method. The bacterial cultures were grown in Muller Hinton broth (MHB) for 12-18 h and the turbidity of bacterial cultures was adjusted to a 0.5 McFarland standard (1×108 CFU/mL). One mL of bacterial culture (1×108 CFU/mL) was pipetted into the center of a sterile Muller Hinton agar (MHA) petri dish and spread on the plate using a spreader and wells were made into agar plates containing inoculums using a sterile cork borer (6 mm in diameter). Then, 100 µL of stock solution of the plant extract (100 mg/mL) and PC-MgONPs (10 mg/mL) were added to agar wells as test samples, and a disc of standard antibiotic (gentamycin) was used as a standard control.

The culture plates were incubated at 37 °C for 18-24 h. The zone of inhibition (including the diameter of the wells) was measured to detect antimicrobial activity[15].

2.6.2. MIC assay and IC50 calculation

The MIC of the plant extract (100 mg/mL) and PC-MgONPs (10 mg/mL) stock solution was determined by broth microdilution method, using sterile 96-well polystyrene cell culture plates. The microdilution plate was prepared by adding 100 μL MHB from well 2 to well 12. The first well contained 200 μL of the plant extract and PC-MgONPs and serial double dilution from wells 1 to 10 was performed by transferring 100 μL from each well. Finally, 10 μL of bacterial suspension was added to all the wells except well 12. Well 11 was kept as a positive control containing MHB and bacteria suspension, while well 12 was marked as a negative control containing only MHB. Next, the plates were incubated at 37 °C for 18-24 h. After incubation, a freshly prepared 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) reagent in sterile water at 0.5 mg/mL stock solution of volume 40 μL was added to each well and incubated at 37 °C for 30 min, and plates were measured at an absorbance of 600 nm in a microplate reader (SpectraMax plus 384). The experiment was done in triplicate[16],[17].

The IC50 calculations were performed using the online QuestGraph™ IC50 Calculator online link (https://www.aatbio.com/tools/IC50-calculator)[18].

2.7. Determination of total antioxidant capacity (TAC)

The in vitro antioxidant potential of PC-MgONPs was performed by TAC assay TAC using a total antioxidant capacity kit, MK-187, Sigma. Briefly, the test involves the reduction of Cu2+ ion to Cu+ by small molecules and proteins. The reduced Cu+ ion chelates with a colorimetric probe, giving a broad absorbance peak at 570 nm, which is proportional to TAC[19].

2.8. Determination of cell viability/proliferative activity

The cell viability of PC-MgONPs against a breast cancer cell line (MDA-231) was evaluated using the MTT assay. The cancer cells were grown in Dulbecco’s Modified Eagle Medium supplemented with 1% antibiotic and 10% of fetal bovine serum solution in a humidified incubator with 5% CO2 at 37 °C. To measure cell inhibition, an MTT assay was performed. The cancer cells were seeded in 96-well plates at a density of 1×105 and incubated at 37 °C for 1 d. During the incubation time, cells were treated with PC-MgONPs (500, 250, 125, 62.5, 31.25, and 15.62 μg/mL) and P. curviflorus (5000, 2500, 1250, 625, 312.5 and 156.25 μg/mL) for additional 24 h at 37 °C. Then, 10 µL of MTT reagent solution was added to each well, and the plates were incubated at 37 °C for 4 h. With the addition of 100 µL of dimethyl sulfoxide, the purple-colored formazan crystals were dissolved. The absorbance was measured at 570 nm using a multiplate reader[20].

The cell inhibition percentage was calculated with the equation: Cell inhibition (%) = 100 − (ODtest/ODcontrol × 100).

2.9. Statistical analysis

Statistical analyses were performed in triplicates using one-way ANOVA and data were presented as mean ± standard deviation. A P-value < 0.05 was considered significantly different. The GraphPad Prism Software 5th version for Windows, La Jolla, CA was used to perform statistical analysis.

  3. Results 

3.1. UV–Vis spectral analysis

The formation of PC-MgONPs was confirmed by UV-Vis spectroscopy (wavelength range: 200-800 nm). A characteristic SPR absorbance peak was observed at 300 nm which verified the formation of PC-MgONPs [Figure 1].

Figure 1: UV-Vis spectra of magnesium oxide nanoparticles using shoot extracts of Plicosepalus curviflorus (PC-MgONPs).

Click here to view

3.2. FTIR spectroscopy

FTIR profile of P. curviflorus extract [Figure 2]A illustrated 13 peaks positions at 3440.58, 2995.75, 2912.76, 2194.79, 2015.64, 1660.45, 1436.25, 1406.56, 1310.31, 1018.46, 951.96, 697.67 and 667.22 cm−1, whereas the PC-MgONPs reaction mixture elucidated 6 absorbance peaks sites at 3292.18, 2165.33, 2150.41, 1992.65, 1633.88, and 1338.33 cm−1[Figure 2]B. The absorbance peaks located between 3000-3600 cm−1 were allocated to the stretching vibrations of hydroxyl (-OH) amine (-NH) and (-CH) groups where -NH was characterized by a lower peak value than -OH.

Figure 2: FTIR analysis of (A) Plicosepalus curviflorus and (B) PC-MgONPs.

Click here to view

According to FTIR data, the amide linkage of protein had a higher potential to bond with magnesium, resulting in the formation of a protein coating around MgONPs that prevents agglomeration and stabilizes the medium. In this study, the involvement of hydroxyl groups, amide group, and alkene functional groups in the bio-reduction process could be confirmed through the shift of the deformation vibration of O-H, -N-H, and –C=C groups positioned at 3440.58 cm−1, 2194.79 cm−1, and 1660.45 cm−1 to 3292.18 cm−1, 2165.33 cm−1, and 1633.88 cm−1, respectively. Thus, it is reasonable to conjecture that hydroxyl, amine alkene, and alkyne functional groups present in the extract of P. curviflorus possibly perform both the capping and reduction process of nanoparticle formation.

XRD spectra analyzed the crystallinity and purity of biogenic-formed PC-MgONPs [Figure 3]A, and the major XRD peaks of 2θ values were 36.8°, 42.4°, 61.8°, 74.9°, and 78.6°. The characteristic Bragg reflections were indexed location to (111), (200), (220), (311), and (222) lattice planes of face-centered cubic structure as compared with the standard reference (JCPDS file no.39-7746)[21] and these peaks confirmed the existence of MgONPs. The sharp diffraction pattern of pre-synthesized PC-MgONPs confirmed its high crystallinity and nano-size. Debye Scherrer’s equation was applied to calculate the size of biogenic PC-MgONPs by using the width of the strongest peak (200) located at 42.4° (2θ value). The results revealed that the average crystallite size was 25 nm.

Figure 3: (A) X-ray diffraction spectrum and (B) size distribution analysis of PC-MgONPs.

Click here to view

The average size distribution of the PC-MgONPs in the solution and the thickness of the capping or stabilizing compound enveloping metallic particles was determined by DLS. The results showed average particle size and polydispersity index (PDI) were 126.2 nm and 0.287 respectively [Figure 3]B. The formed PC-MgONPs had a PDI of less than 0.7 demonstrating their high quality and reasonably well-defined dimensions with high monodispersity (PDI). The surface charge of pre-synthesized PC-MgONPs and the magnitude of charge were calculated by zeta potential and found to be 86.79 value.

3.3. Microscopic characterization of PC-MgONPs

SEM images of PC-MgONPs revealed that the particles had a spherical form and well-dispersed nanorods of PC-MgONPs that lacked any aggregation, with sizes ranging from 20.0 to 76.4 nm. In addition to producing a spherical shape that was well distributed and had a high ratio of surface area to volume, larger clusters were generated [Figure 4]A. EDX spectra were used to analyze the elemental composition of PC-MgONPs [Figure 4]B. The EDX graph revealed that the photo-mediated PC-MgONPs were exceedingly pure, displaying weight and atomic percentages of Mg (31.01%, 38.1%), O (55.1%, 51.3%), and Na (13.8%, 10.6%).

Figure 4: (A) Scanning electron microscopy and (B) energy dispersive X-ray analysis of biogenic PC-MgONPs. The arrow in the image represents the size of the particles (nm).

Click here to view

3.4. Antimicrobial activity, TAC, and anti-proliferative activity of PC-MgONPs

3.4.1. Antimicrobial activity

The antimicrobial activity of P. curviflorus extract and green synthesized PC-MgONPs was evaluated against E. coli, S. aureus, MRSA, P. aeruginosa, and C. albicans. PC-MgONPs were found to be effective against E. coli and C. albicans with a zone of inhibition of 17 and 16 mm, respectively [Figure 5] and [Table 1].

Figure 5: Antimicrobial effect of PC-MgONPs on the microbial strains by Agar well assay. G: gentamicin.

Click here to view

In addition, S. aureus showed the least MIC value of 15.62 μg/mL and IC50 value of 7.17 µg/mL, whereas E. coli and C. albicans showed MICs of 31.25 and 62.50 μg/mL with IC50 values of 10.59 and 15.84 μg/mL, respectively [Table 2]. P. curviflorus extracts showed the highest MIC values (1250 and 2500 μg/mL) against S. aureus and MRSA and showed a partial zone of inhibition.

Table 2: Minimum inhibitory concentration (MIC) and IC50 values of PC- MgONPs and PC µg/mL).

Click here to view

3.4.2. TAC

The results of TAC assay are illustrated in [Figure 6]A. The green synthesized PC-MgONPs displayed excellent antioxidant potential. As reflected in the figure, a dose-dependent pattern was observed in the antioxidant activity ranging from 0.042-0.360 nmol/mL. Moreover, 10 mg/mL of PC-MgONPs exhibited the highest TAC.

Figure 6: (A) Total antioxidant capacity and (B-C) anti-proliferative activity of PC-MgONPs and PC against breast cancer MDA-231 cells. *P<0.05.

Click here to view

3.4.3. Anti-proliferative activity

PC-MgONPs and P. curviflorus extract showed a concentration-dependent decline in cell viability (P < 0.05). In addition, PC-MgONPs exhibited more significantly inhibitory effects against MDA-231 cell viability compared to P. curviflorus extract [Figure 6]B [Figure 6]C.

  4. Discussion 

A biological approach for the synthesis of metal and metal oxide nanoparticles can be employed as an alternative to chemical and physical methods[22]. The benefits of biological synthesis, including its low cost, environmental friendliness, biocompatibility, scalability, and evasion of tough synthesis conditions like high temperature and pH, can be credited with this phenomenon[22]. Among biological entities, plants are recognized as promising entity for the biogenic synthesis of nanoparticles due to the presence of chemical components and high metal tolerances[23]. MgONPs are acknowledged by the FDA as a safe alternative to antibiotics with highly efficient antibacterial properties[7],[24]. The ethanol extract of P. curviflorus shoots is a rich source of different types of bio-constituents including flavonoids, phenols, terpenes, steroids, proteins, and carbohydrates[12]. These phytocomponents might have contributed to the reduction, stabilization, and capping of produced PC-MgONPs, which plays a crucial role in the reduction of Mg(NO3)2•6H2O to MgO-NPs. The hydroxyl and carbonyl groups of phytoconstituents serve as reducing and stabilizing substances[25]. The formation of biogenic PC-MgONPs initiates once the P. curviflorus extract is introduced into 1.0 mM Mg(NO3)2 solution. The gradual color change of Mg(NO3)2/P. curviflorus solution from dark green to dark brown indicates the formation of PC-MgONPs. This color change can be attributed to the role of P. curviflorus metabolites in the reduction of NO3– to NO2 followed by the reduction of Mg2+ to Mg(OH)2 by liberated electrons. The maximum color intensity was attained due to the reduction of a large number of metal ions. The as-prepared Mg(OH)2 was calcinated at 400 °C to form PC- MgONPs[26]. The formation of PC-MgONPs was further confirmed by different spectroscopic (UV-Vis, FTIR, XRD, ZI, DLS) and microscopic (SEM and EDX) techniques.

The UV-Vis spectroscopy analysis showed a characteristic SPR absorbance peak at 300 nm, which satisfies the standard MgO absorption pattern because all oxide nanomaterials have wide band gaps and a propensity for shorter wavelengths. The formation of PC-MgONPs was confirmed by UV-Vis spectroscopy (wavelength range: 200-800 nm)[27].

FTIR analysis was performed to identify the potential biomolecules that contributed to the bioreduction of magnesium oxide and stabilization of PC-MgONPs[28]. The presence of peaks between 2100-2250 cm−1 corresponds to alkyne (C≡C, C≡N) functional groups, and the peak appearance at 2194.79 cm−1 in P. curviflorus extract and 2 165.33 cm−1 in PC-MgONPs indicates the presence of unsaturated hydrocarbons in the extract as well as in biogenic PC-MgONPs[29]. The appearance of prominent peaks at around 1662-1626 cm−1 is characteristic of the C=C stretching vibration type for disubstituted alkene. The peak shifting in the spectral profile of PC-MgONPs could be attributed to the interactions between those chemical functional groups and MgONPs[30]. It is reported in the literature that free amide groups in the protein molecules allow them to interact with MgONPs[31]. Our results exhibited broad distinctive spectral bands at 3292.18-3440.58 cm−1 are characteristics of the O-H stretching vibration type of hydroxyl functional moiety in polyphenols and N-H stretching vibration in primary and secondary amines (amino acids, proteins, and peptides) as well as hydrocarbons[32]. The results also indicate that some organic residues, such as hydroxyl and carboxyl groups, are present on the surface of the prepared PC-MgONPs.

The surface charge of pre-synthesized PC-MgONPs and the magnitude of charge were calculated by zeta potential and found to be 86.79 value, which illustrates the nanoparticle stability in dispersion by developing specific charge groups on their surface[33]. The result revealed that PC-MgONPs produced by P. curviflorus shoot extracts exhibited a charge on the surface of the PC-MgONPs, possibly due to free nitrate ions in the reaction mixture that provides repulsive force as electrostatic force stabilization[34]. Furthermore, no particle agglomeration was seen, as the formed PC-MgONPs were well dispersed. These results indicate that phytocomponents of the plant extract served not only as a reducing agent but also as a stabilizer, which protects the aggregation of MgONPs.

SEM analysis displayed spherical and well-dispersed nanorods of PC-MgONPs with sizes ranging from 20 to 76.4 nm[35]. The EDX graph revealed that the PC-MgONPs were exceedingly pure, displaying weight and atomic percentages of Mg (31.01%, 38.1%), O (55.1%, 51.3%), and Na (13.8%, 10.6%), which corresponds to the synthesis of MgO via ethanol extract of P. curviflorus[36].

PC-MgONPs were also found to be effective against E. coli and C. albicans with a zone of inhibition of 17 and 16 mm in contrast to other studies of MgONPs antibacterial activity which showed zero zones of inhibition against E. coli and S. aureus[37]. PC-MgONPs exhibited very effective effects in comparison with MgONPs[37]. Whereas, in our previous study, the biogenic green synthesis of MgONPs using Saussurea costus biomasses exhibited the highest MIC values for E. coli and P. aeruginosa in contrast to those of PC-MgONPs in our present research work[38].

Among the Gram-negative bacteria, E. coli was most sensitive to PC-MgONPs, because the Gram-negative bacteria are coated with lipopolysaccharide molecules, which have a negative charge and bind with positively charged MgO ions on the surface of PC-MgONPs, possibly leading to increased uptake of ions that damages the intracellular structures of Gram-negative bacteria[39].

As reported in the previous research, three compounds quercetin, catechin, and flavane gallate 2S, 3R-3,3′,4′, 5, 7-pentahydroxyflavane-5-O-gallate were isolated from the aerial parts of P. curviflorus[16], flavane gallate and catechin possess antimicrobial activity against various Gram-positive and Gram-negative pathogenic bacterial strains by binding to the lipid bilayer which damages bacterial membrane leading to inactivation and inhibition of intracellular and extracellular enzymes synthesis[40].

Numerous studies indicate that the antimicrobial activity of MgO is generally attributed to the production of reactive oxygen species (ROS), causing membrane breakdown and cellular content leakage. It has been shown that bacterial cells treated with MgONPs produce deep craters on their membrane surface, indicating that structural damage to the membrane leads to cellular content leakage. Whereas, our results showed PC-MgONPs had better antimicrobial activity than the plant extract which only showed antibacterial effects against S. aureus and MRSA. Nanoformulation of catechin and other active plant components had strong antibacterial activity, but in the present study, the plant extract exhibited less antimicrobial activity against the pathogenic microbial strains[41].

Although cellular oxidation is essential for cell proliferation, it also has some negative side effects due to the production of free radicals and ROS. Overproduction of these free radicals has severe consequences on the protective antioxidant system, which in turn causes cellular damage by oxidizing essential macromolecules, ultimately resulting in apoptosis/cell death. TAC analysis confirmed PC-MgONPs possess superior antioxidant capability, which may be due to the capping effect of phytochemicals like flavonoids, which have several hydroxyl groups and phenolic functional groups on their surface, making synergistic effects. Our results both confirm and extend the work of previous researchers[42].

Moreover, curviflorin, curviflorside, flavonoids, and naphthalene were found in shoot parts of P. curviflorus[11], which possess strong antioxidant activity. Previous studies on the extracts of P. curviflorus and PC-MgONPs support our present findings. PC-MgONPs exhibited strong antioxidant activity which involves the redox potential of phytochemicals and the active compounds found in the P. curviflorus extract and the MgO antioxidant capability[43].

In our results, a decrease in cell viability of MDA-231 cells was observed as the concentration of PC-MgONPs and P. curviflorus extract increased, which may be attributed to the generation of ROS by PC-MgONPs, resulting in damages to mitochondrial membrane integrity and thus activation of the apoptotic pathway leading to cell death. The result was consistent with that found in a previous study in which P. curviflorus extract showed the expression of apoptosis-regulating genes including caspase-3, -8, -9, p53, Bax, and Bcl-2[29]. Contrary to what has been shown in the past, the toxicity of PC-MgONPs may be directly related to their size, with smaller-size PC-MgONPs being more hazardous because they generate more ROS that interact with cellular components and penetrate cell membranes, releasing Mg+ ions[36],[44]. Among the phytochemicals, phenolic compounds such as catechin showed an anti-proliferative effect against lung cancer A549 cells by inhibiting cyclin E1 and p-AKT and induction of a potent cyclin kinase inhibitor. Moreover, epicatechin induces apoptosis in breast and prostate carcinomas[45].

To conclude, PC-MgONPs were successfully synthesized using P. curviflorus shoot extract. PC-MgONPs showed antimicrobial, antioxidant, and anti-proliferative properties. However, in vivo studies are needed to further verify their effects.

Conflict of interest statement

The authors declare that they have no conflict of interest.

Acknowledgments

The authors extend their appreciation to the Research Supporting Project number (RSPD2023R656), King Saud University, Riyadh, Saudi Arabia.

Funding

This work was funded by the Researchers Supporting Project Number (RSPD2023R656), King Saud University, Riyadh, Saudi Arabia.

Authors’ contributions

RHA theorized and designed the research study, reviewed the literature, acquired data, and critically commented on the original draft of the manuscript. MA reviewed and edited the final draft of the manuscript. AM contributed to the conceptualization and design of the study, interpreted the results, and wrote the manuscript. HT designed the study and contributed to the discussion of the study. NIA managed data collection and analysis. SF interpreted the results. BA critically revised and edited the final version of the manuscript. FM critically commented on and edited the final version of the manuscript. NMA managed data collection. MA interpreted the results. All the authors have read and agreed with the published version of the manuscript.

 

  References 
1.Thakur N, Ghosh J, Pandey SK, Pabbathi A, Das J. A comprehensive review of biosynthesis of magnesium oxide nanoparticles, and their antimicrobial, anticancer, and antioxidant activities as well as toxicity study. Inorg Chem Commun 2022; 146. doi: 10.1016/j.inoche.2022.110156.  
    2.Chen B, Lin Z, Saiding Q, Huang Y, Sun Y, Zhai X, et al. Enhancement of critical-sized bone defect regeneration by magnesium oxide-reinforced 3D scaffold with improved osteogenic and angiogenic properties. J Mater Sci Technol 2023; 135: 186-198.  
    3.Navya N, Ambika AV, Suresha BL. Synthesis, characterization, and anti-cancer potential study of Ag-MgO nanocomposite. Inorg Chem Commun 2022; 142: 109671.  
    4.Raissa U, Muhammad Abbas Qassem H, Ahmed M, Abdullateef Alzubaidi M, A Dawood F, Abdulamir Abdullah Y, et al. Investigating the effect of streptozotocin-induced diabetes on the ovarian tissue of NMRI mice following the injection of MgO and MgONPs. J Nanostructures 2023; 13(1): 1-7.  
    5.De Silva RT, Mantilaka M, Goh KL, Ratnayake SP, Amaratunga GAJ, de Silva KM. Magnesium oxide nanoparticles reinforced electrospun alginate-based nanofibrous scaffolds with improved physical properties. Int J Biomater 2017; 2017. doi: 10.1155/2017/1391298.  
    6.Akram MW, Fakhar-e-Alam M, Atif M, Butt AR, Asghar A, Jamil Y, et al. In vitro evaluation of the toxic effects of MgO nanostructure in Hela cell line. Sci Rep 2018; 8(1): 4576.  
    7.U.S. Food and Drug Administration. CFR—Code of federal regulations Title 21. [Online] Available from: https://www.accessdata.fda.gov/scripts/cdrh/cfdocs/cfcfr/CFRSearch.cfm?fr=184.1431 [Accessed on 20th Dec 2022].  
    8.Skylar Kenney AE. FDA approves magnesium sulfate injection from milla pharmaceuticals. Pharm Times 2022; 88(1). [Online] Available from: https://www.pharmacytimes.com/view/fda-approves-magnesium-sulfate-injection-from-milla-pharmaceuticals [Accessed on 20th Dec 2022].  
    9.Sher H, Alyemeni MN. Pharmaceutically important plants are used in the traditional system of Arab medicine for the treatment of livestock ailments in Saudi Arabia. Afr J Biotechnol 2011; 10(45): 9153-9159.  
    10.Al-Fatimi M, Wurster M, Schröder G, Lindequist U. Antioxidant, antimicrobial and cytotoxic activities of selected medicinal plants from Yemen. J Ethnopharmacol 2007; 111(3): 657-666.  
    11.Al Musayeib NM, Ibrahim SRM, Amina M, Al Hamoud GA, Mohamed GA. Curviflorside and curviflorin, new naphthalene glycoside, and flavanol from Plicosepalus curviflorus. Z Für Naturforschung C 2017; 72(5-6): 197-201.  
    12.Amina M, Al Musayeib NM, Alarfaj NA, El-Tohamy MF, Al-Hamoud GA, Alqenaei MK. The fluorescence detection of phenolic compounds in Plicosepalus curviflorus extract using biosynthesized ZnO nanoparticles and their biomedical potential. Plants 2022; 11(3): 361.  
    13.Huma T, Hakimi N, Younis M, Huma T, Ge Z, Feng J. MgO heterostructures: From synthesis to applications. Nanomaterials 2022; 12(15): 2668.  
    14.Silva AA, Sousa AMF, Furtado CR, Carvalho NM. Green magnesium oxide prepared by plant extracts: Synthesis, properties, and applications. Mater Today Sustain 2022; 20. doi: 10.1016/j.mtsust.2022.100203.  
    15.Balouiri M, Sadiki M, Ibnsouda SK. Methods for in vitro evaluating antimicrobial activity: A review. J Pharm Anal 2016; 6(2): 71-79.  
    16.Orfali R, Perveen S, Siddiqui NA, Alam P, Alhowiriny TA, Al-Taweel AM, et al. Pharmacological evaluation of secondary metabolites and their simultaneous determination in the arabian medicinal plant Plicosepalus curviflorus using HPTLC validated method. J Anal Methods Chem 2019; 2019. doi: 10.1155/2019/7435909.  
    17.National Committee for Clinical Laboratory Standards, Barry AL. Methods for determining bactericidal activity of antimicrobial agents: Approved guideline. Wayne, PA: National Committee for Clinical Laboratory Standards; 1999.  
    18.AAT Bioquest, Inc. Quest Graph™ IC50 Calculator. AAT Bioquest. [Online] Available from: https://www.aatbio.com/tools/ic50-calculator [Accessed on 20th February 2022].  
    19.Gupta S, Finelli R, Agarwal A, Henkel R. Total antioxidant capacity— Relevance, methods and clinical implications. Andrologia 2021; 53(2). doi: 10.1111/and.13624.  
    20.Kamiloglu S, Sari G, Ozdal T, Capanoglu E. Guidelines for cell viability assays. Food Front 2020; 1(3): 332-349.  
    21.Balakrishnan G, Velavan R, Batoo KM, Raslan EH. Microstructure, optical and photocatalytic properties of MgO nanoparticles. Results Phys 2020; 16. doi: 10.1016/j.rinp.2020.103013.  
    22.Jeevanandam J, Kiew SF, Boakye-Ansah S, Lau SY, Barhoum A, Danquah MK, et al. Green approaches for the synthesis of metal and metal oxide nanoparticles using microbial and plant extracts. Nanoscale 2022; 14(7): 2534-2571.  
    23.Ahmed SF, Mofijur M, Rafa N, Chowdhury AT, Chowdhury S, Nahrin M, et al. Green approaches in synthesising nanomaterials for environmental nanobioremediation: Technological advancements, applications, benefits and challenges. Environ Res 2022; 204: 111967.  
    24.Kumar H, Bhardwaj K, Kuča K, Kalia A, Nepovimova E, Verma R, et al. Flower-based green synthesis of metallic nanoparticles: Applications beyond fragrance. Nanomaterials 2020; 10(4): 766.  
    25.Madkour LH. Biogenic–biosynthesis metallic nanoparticles (MNPs) for pharmacological, biomedical and environmental nanobiotechnological applications. Chron Pharm Sci J 2018; 2(1): 384-444.  
    26.Adeyemi JO, Oriola AO, Onwudiwe DC, Oyedeji AO. Plant extracts mediated metal-based nanoparticles: Synthesis and biological applications. Biomolecules 2022; 12(5): 627.  
    27.Tanabe I, Tanaka YY, Watari K, Inami W, Kawata Y, Ozaki Y. Enhanced surface plasmon resonance wavelength shifts by molecular electronic absorption in far-and deep-ultraviolet regions. Sci Rep 2020; 10(1): 9938.  
    28.Ammulu MA, Vinay Viswanath K, Giduturi AK, Vemuri PK, Mangamuri U, Poda S. Phytoassisted synthesis of magnesium oxide nanoparticles from Pterocarpus marsupium rox. b heartwood extract and its biomedical applications. J Genet Eng Biotechnol 2021; 19(1): 21.  
    29.Eltamany EE, Goda MS, Nafie MS, Abu-Elsaoud AM, Hareeri RH, Aldurdunji MM, et al. Comparative assessment of the antioxidant and anticancer activities of Plicosepalus acacia and Plicosepalus curviflorus: Metabolomic profiling and in silico studies. Antioxidants 2022; 11(7): 1249.  
    30.Omdurman S. Synthesis and characterization of carbon nanotubes incorporated with MgO nanoparticles. J Ovonic Res Voi 2021; 17(5): 429-435.  
    31.Limo MJ, Sola-Rabada A, Boix E, Thota V, Westcott ZC, Puddu V, et al. Interactions between metal oxides and biomolecules: from fundamental understanding to applications. Chem Rev 2018; 118(22): 11118-11193.  
    32.Petit S, Decarreau A, Martin F, Buchet R. Refined relationship between the position of the fundamental OH stretching and the first overtones for clays. Phys Chem Miner 2004; 31(9): 585-592.  
    33.Negrescu AM, Killian MS, Raghu SN,