Next Article in Journal
Contributions to Estimating the Water-Holding Capacity in Fresh Pork Hams Using NMR Relaxometry
Next Article in Special Issue
Exploring the Impact of Olive-Derived Bioactive Components on Gut Microbiota: Implications for Digestive Health
Previous Article in Journal
Reforming Food, Drug, and Nutraceutical Regulations to Improve Public Health and Reduce Healthcare Costs
Previous Article in Special Issue
Immunomodulation of Glycyrrhiza Polysaccharides In Vivo Based on Microbiome and Metabolomics Approaches
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Foods
Volume 14
Issue 13
10.3390/foods14132327
foods-logo
Submit to this Journal Review for this Journal Propose a Special Issue
Article Menu

Article Menu

share Share announcement Help format_quote Cite question_answer Discuss in SciProfiles
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Article

Dianthus superbus L. (QM) Extract-Assisted Silver Nanoparticle Gelatin Films with Antioxidant and Antimicrobial Properties for Fresh Fruit Preservation

by
Chenwei Zhang
1,
Yao Li
1,
Yue Huo
2,
Hongtao Wang
1 and
Dandan Wang
1,*
1
College of Life Sciences, Yantai University, Yantai 264005, China
2
School of Biological Science and Food Engineering, Chuzhou University, Chuzhou 239000, China
*
Author to whom correspondence should be addressed.
Foods 2025, 14(13), 2327; https://doi.org/10.3390/foods14132327
Submission received: 13 May 2025 / Revised: 27 June 2025 / Accepted: 28 June 2025 / Published: 30 June 2025
(This article belongs to the Special Issue Exploring the Nutritional and Functional Properties of Plant Food-Derived Bioactive Components)
Browse Figures
Versions Notes

Abstract

We synthesized QM-AgNPs (Dianthus superbus L.-AgNPs, Qu Mai-AgNPs) by an economical and environmentally friendly method using Dianthus superbus L. extract as a reducing and stabilizing agent. The resulting QM-AgNPs were comprehensively characterized and evaluated for their antioxidant, cytotoxic, and antibacterial activities. Herein, TEM analysis revealed that the QM-AgNPs were predominantly spherical, polydisperse, and exhibited a core particle size ranging from 11 to 18 nm. In contrast, DLS analysis showed a larger hydrodynamic diameter (primarily 60–87 nm), reflecting the hydrated shell and surface biomolecular corona. The crystalline nature of QM-AgNPs was confirmed by XRD and SAED spectra while FTIR spectroscopy indicated the presence of functional groups from the plant extract that may contribute to nanoparticle stabilization. Functional assessments demonstrated that QM-AgNPs exhibited strong antioxidant activity, with efficient DPPH radical scavenging, and selective cytotoxicity against A549 cancer cells while sparing normal cells. Moreover, QM-AgNPs showed significant antibacterial activity against both Staphylococcus aureus (Gram-positive) and Escherichia coli (Gram-negative), likely due to membrane disruption and the leakage of intracellular contents. To explore practical applications, we developed a GEL@AgNPs coating system for the postharvest preservation of grapes. As a result, the reduced weight loss and decay rate suggest a potential role for QM-AgNPs in extending fruit freshness. Comprehensive shelf-life studies are planned to further substantiate the potential of QM-AgNPs as an effective material for active food packaging applications.

Graphical Abstract

1. Introduction

Nanomaterials are extensively utilized in fields such as biotechnology, biomedicine, optoelectronics, pharmaceuticals, cosmetics, food industries, materials science, and agriculture [1,2,3,4]. Silver nanoparticles (AgNPs) have particle sizes ranging from 1 to 100 nm [5]. Compared with other nanoparticles, AgNPs have diverse biocompatibility and metal properties; these characteristics have led to widespread research and numerous applications of AgNPs in nanotechnology. Due to their antibacterial properties, AgNPs are frequently used as preservatives in the food industry [6]. They also serve as antioxidants and antibacterial agents in the cosmetics industry, as well as antibacterial agents and catalysts for chemical waste degradation in sewage treatment [7,8,9]. Additionally, AgNPs have unique physicochemical properties that enable specific targeting of tumor cells, without inducing genotoxic effects on human cells at low concentrations [10], thus laying the foundation for novel research in cancer treatment and drug delivery [11].
The main methods for synthesizing AgNPs include physical, chemical, and biological methods [12]. The particle size, morphology, and stability of AgNPs vary depending on the synthesis method used. With growing concerns over the environmental and health impacts of physical and chemical synthesis methods, green synthesis has gained considerable attention. In contrast, biosynthesis methods involve the use of extracts of biological organisms as reducing agents and stabilizers. No toxic substances remain in the product, as no toxic solvents are used [13]. The biological synthesis of silver nanoparticles frequently utilizes bacteria, fungi, yeasts, algae, and plants [14]. Bacterial synthesis of silver nanoparticles can be classified into intracellular and extracellular synthesis. In intracellular synthesis, silver ions penetrate the bacterial cell membrane and enter the cell, where they are reduced to silver atoms by enzymes or metabolic products, subsequently aggregating to form nanoparticles. Extracellular synthesis involves the adsorption of silver ions by extracellular polymers secreted by bacteria, which are then reduced to silver nanoparticles through enzymatic reactions or redox reactions, with the particles typically dispersed in the culture medium. Fungal synthesis of silver nanoparticles occurs through the adsorption of silver ions by functional groups on the fungal hyphal surface, followed by the reduction to silver nanoparticles via intracellular enzymes or extracellularly secreted organic acids, amino acids, and other compounds [15]. Plant-based synthesis methods leverage the active substances in plant extracts as reducing and capping agents, facilitating synthesis with naturally occurring compounds. Numerous studies have demonstrated the successful synthesis of silver nanoparticles from various plant extracts, with variations in size, shape, and surface functional molecules, resulting in diverse biological activities [16,17]. This method can promote waste utilization [10], and make the continued utilization of plant materials for the biosynthesis of AgNPs a prominent area in the recent research.
Dianthus superbus L. (QM) is a perennial plant of the Caryophyllaceae family [18]. As a plant with dual medicinal and edible value in TCM, Dianthus superbus L. is traditionally recognized for its ethnopharmacological properties, including anti-inflammatory effects (‘clearing heat’), diuretic activity, and historical use in regulating blood circulation-related menstrual disorders (‘breaking blood through menstruation’) [19]. Additionally, QM extracts exhibit inhibitory effects on Escherichia coli and Staphylococcus aureus [13,20]. Therefore, we utilized QM as the raw material for preparing AgNPs, the synthesis method of which is green and relatively simple. Furthermore, the high moisture content in fruits leads to a short shelf life and quality degradation during transportation, causing browning, rotting, and other issues [21]. Previous studies [22,23,24,25] have demonstrated that composite membranes prepared by combining AgNPs with other substances possess antibacterial effects.
Our study utilized the QM extract as a stabilizing and reducing agent to optimize the synthesis conditions for AgNPs. Cytotoxicity assays were performed to demonstrate the inhibitory effects of synthesized QM-AgNPs on A549 and Human Umbilical Vein Endothelial Cells (HUVECs). The bacteriostatic mechanisms, including zone of inhibition, minimum inhibitory concentration (MIC), minimum bactericidal concentration (MBC), growth dynamics curve, membrane permeability, reactive oxygen species (ROS), and antibiofilm activity, were conducted to confirm the bacteriostatic effects of QM-AgNPs against E. coli (ATCC 25922) and S. aureus (ATCC 29213). Finally, grapes were used to test the fruit preservation capabilities of QM-AgNPs, which confirmed the effect of QM-AgNPs in extending the shelf life of fruit [26], and provide certain reference values for the development of the fruit preservation industry [27].

2. Materials and Methods

2.1. Chemicals and Materials

Silver nitrate was purchased from Sinopharm Chemical Reagent Co., Ltd. (Shanghai, China), for use. All reagents used in our study were of analytical grade. Dianthus superbus L. roots were obtained from Yantai Herbal Market. LB broth medium (LB) and agar were provided by the laboratory of Yantai University. E. coli (ATCC 25922) and S. aureus (ATCC 29213) were obtained from the laboratory of Yantai University. The A549 and HUVECs were obtained from the Shanghai Cell Bank of the Chinese Academy of Sciences. The fruits used in the freshness preservation experiment were purchased from the fruit store at Yantai University.

2.2. Preparation of the QM Extraction

A total of 10 g QM powder was placed in a conical flask with 100 mL of deionized water (DDW) and heated in a water bath at 90 °C for 100 min. Moreover, the extracts were centrifuged at 10,611× g for 10 min using a high-speed centrifuge, then the supernatant was transferred to a refrigerator at 4 °C for storage and future use.

2.3. Green Synthesis of AgNPs

AgNO3 (1 mol/L) and QM extract were added to the conical flask (200 mL extract: 200 μL AgNO3). After thorough mixing, the reaction mixture was placed in a 90 °C water bath for 60 min. During the reaction, a color change occurred (from light yellow to brown black), indicating the synthesis of silver nanoparticles [28]. After the reaction, the mixture was centrifuged at 10,611× g for 10 min, and then washed repeatedly by centrifuging at 12,000 rpm for 15 min. The precipitate was dried at room temperature for subsequent use.

2.4. Optimization of QM-AgNP Synthesis Conditions

2.4.1. Single-Factor Design

To optimize the conditions for the synthesis of QM-AgNPs, we employed a single-factor design focusing on extract concentration, synthesis time, and reaction temperature. The optimal conditions for these three factors were determined by measuring the absorbance values.

2.4.2. Box–Behnken Design for Optimization

To optimize the synthesis conditions for silver nanoparticles, we focused on three variables: extract concentration, reaction time, and reaction temperature. Gradients for each variable were established, and experimental protocols were designed using Design-Expert 13 to optimize the synthesis conditions [29], as shown in Table 1. After the reaction, the mixtures were scanned using a dual-beam UV-visible spectrophotometer, and the resulting absorbance values were analyzed with the software. Finally, the optimized conditions were validated through experiments.

2.5. Characterization of QM-AgNPs

AgNPs were analyzed by UV-Vis spectrophotometry within the wavelength range of 300~700 nm. Moreover, the size, morphology, and crystal structure of the prepared AgNPs were characterized using transmission electron microscopy (TEM). The elemental composition of the sample microstructure was analyzed using energy-dispersive X-ray spectroscopy (EDX) [30]. The crystal structure of AgNPs was determined by X-ray diffraction [31] (XRD) and selected area electron diffraction (SAED). Furthermore, the particle size of QM-AgNPs was measured by dynamic light scattering (DLS) [32]. Attenuated total reflectance Fourier-transform infrared (ATR-FTIR) spectroscopy was used to obtain molecular bond information, with spectra recorded in the range of 500–4000 cm−1 using a diamond probe.

2.6. Antioxidant Activity of QM-AgNPs

Different concentrations of the QM-AgNP solution were added to each tube, with a 2,2-Diphenyl-1-picrylhydrazyl (DPPH) solution serving as the negative control group and vitamin C (Vc) as the standard control group. Furthermore, 2 mL of DPPH–ethanol solution (0.10 mmol/L) was added to each tube, and the mixture was vortexed to ensure even mixing. The reaction was allowed to proceed in the dark for 30 min, and the absorbance of each sample was measured at 517 nm. The formula for calculating the DPPH radical scavenging rate is as follows:
DPPH radical scavenging rate (%) = [1 − (As − A0)/A0] × 100%
In the formula, A0 represents the absorbance value of the DPPH–ethanol solution; As represents the absorbance value after the addition of QM-AgNPs; and Ac represents the absorbance value of the QM-AgNPs solution alone.

2.7. In Vitro Cytotoxicity

2.7.1. Cell Viability

A549 cancer cells and HUVECs were cultured in Dulbecco’s Modified Eagle Medium (DMEM) and RPMI-1640 medium supplemented with 10% fetal bovine serum (FBS) at 37 °C in a humidified atmosphere containing 5% CO2 and 95% air. The cytotoxicity of QM-AgNPs in A549 and HUVECs was determined using the the Methylthiazolyldiphenyl-tetrazolium bromide (MTT) assay.

2.7.2. Cell Apoptosis Detection

The slides were sterilized by soaking them in an ethanol solution and then rinsed repeatedly with sterile Phosphate Buffered Saline (PBS). Cells with a density of 1 × 105 were inoculated into six-well plates containing the cell culture slides and placed in an environment of 37 °C, 5% CO2 for 24 h. The next day, different concentrations of QM-AgNPs were added to the wells to treat lung cancer cells for 24 h. After 24 h of incubation, the previous culture medium was discarded, and a fixative was added to fix the cells for 20 min. After washing with PBS for 3 min, Hoechst staining solution was added and the cells were stained for 5 min at room temperature and protected from light. The staining solution was discarded and rinsed with PBS. A drop of anti-fluorescence quenching agent was added to the crawler sheet with a pipette, the culture slides with cells attached were covered, and the morphology was then observed and photographed under a fluorescence microscope.

2.8. Antibacterial Properties of QM-AgNPs

2.8.1. Determination of the Inhibition Zone

The paper-disk diffusion method [33] was employed to observe the sensitivity of Gram-negative bacteria E. coli, as well as Gram-positive bacteria S. aureus to QM-AgNPs and amikacin (positive control).

2.8.2. Minimum Inhibitory Concentration (MIC)

The MIC was determined using the microdilution method [34]. The activated bacterial suspension was diluted to 1 × 106 CFU/mL. Liquid medium, QM-AgNPs at concentrations ranging from 4 to 512 μg/mL, and a bacterial solution were added to the 96-well plate, ensuring that the final volume of each well was 200 μL. All samples were incubated at 37 °C for 24 h. On the following day, MTT solution (5 mg/mL) was added and then incubated for 4 h. The color of the reaction solution in the 96-well plate was observed, and the lowest concentration that did not change color was recorded as the MIC.

2.8.3. Minimum Bactericidal Concentration (MBC)

The bacterial solutions containing different concentrations of QM-AgNPs were pipetted onto the plates and spread evenly. The plates were then incubated at 37 °C for 16–20 h. The concentration was recorded as MBC when no colony growth or less than 5 colonies were observed on the plate.

2.8.4. Growth Dynamics Curve

The growth dynamics curve was created following an established protocol [35]. Bacteria cultured overnight were diluted to approximately 1 × 106 CFU/mL with sterile LB broth medium, and a certain concentration of QM-AgNPs was added to achieve final concentrations of 1/2MIC, 1MIC, and 2MIC for each bacterium. The same volume of PBS buffer was added to replace QM-AgNPs as a blank control. The absorbance of OD600 was measured every hour, and the growth dynamics curve of QM-AgNPs’ inhibition of bacteria was plotted.

2.8.5. Antibiofilm

Biofilm is a three-dimensional structure formed by extracellular polymers (EPs) secreted by bacteria, containing polysaccharides, proteins, and nucleic acids, which is the external environment for bacteria. The determination of antibacterial film is based on the previously described method [36]. Biofilm formation was induced by adding bacterial suspension (1 × 106 CFU/mL) to a 96-well plate and incubated at 37 °C for 48 h. The biofilm attached to the bottom of the wells was washed three times with PBS buffer. Different concentrations of QM-AgNPs were added to the wells, and the control group was incubated with culture medium for 24 h at 37 °C. The supernatant was discarded and the wells were washed with PBS buffer 2–3 times. Methanol was then added, and the biofilm was fixed for 30 min after discarding the methanol solution, and incubated for 15 min. The biofilm was washed 2–3 times with PBS buffer and 100 μL of 33% glacial acetic acid was added to each well for 15 min to decolorize the biofilm. The resulting supernatant was transferred to a new 96-well plate and the absorbance was measured at 570 nm using a microplate reader.

2.8.6. Reactive Oxygen Species (ROS) Detection

Bacterial suspension at a concentration of 1 × 106 CFU/mL was incubated with 2 × 10−5 mol/L 2′,7′-Dichlorofluorescin diacetate (DCFH-DA) in a constant-temperature incubator at 37 °C for 1 h. Excess extracellular DCFH-DA was removed by centrifugation at 4244× g for 10 min, and QM-AgNPs were added to achieve a final concentration of 1/2 MIC for each bacterium. Fluorescence intensity was measured using fluorescence spectrophotometry, with an excitation wavelength of 495 nm, an emission wavelength of 525 nm, and a slit width of 5 nm. This method is based on established oxidative stress detection protocols in bacteria [37].

2.8.7. Measurement of Intracellular Contents

The quantification of nucleic acid and protein leakage was based on the previously described method [38]. Bacterial suspension at a concentration of 1 × 106 CFU/mL was centrifuged at 10,611× g for 5 min to obtain the bacterial pellet. The supernatant was discarded, and the precipitate was washed 1–2 times with sterile PBS buffer. The bacterial pellet was resuspended in sterile PBS buffer and mixed with various concentrations of QM-AgNPs to achieve final concentrations of 1/2 MIC, MIC, and 2 MIC for each bacterium strain, followed by incubation at 37 °C for 4 h. The bacterial suspension was centrifuged at 10,611× g for 15 min every hour, and absorbance values at 260 nm and 280 nm were determined using a UV-visible spectrophotometer. (Sterile PBS buffer was used as a blank control in place of the QM-AgNPs solution).

2.8.8. AO/PI Staining

Activated bacteria were treated with different concentrations of QM-AgNPs, achieving final concentrations of 1/2MIC, MIC, and 2MIC for each bacterial strain. Sterile PBS buffer was used as the blank control. The mixture was incubated at 37 °C for 4 h. After incubation, an AO/PI staining solution was added to the bacterial solution and incubated for 15 min in the dark. The staining solution was discarded and the wells were washed with sterile PBS buffer 2–3 times to remove excess dye and QM-AgNPs. Then, the remaining liquid was aspirated onto a slide, covered with a coverslip, and observed under a fluorescence inverted microscope. The staining results are visualized via fluorescence microscopy, following the method described previously [39].

2.9. Application in Grape Packaging

Coating grapes for freshness was performed according to the experimental method of Bizymis et al. [40,41,42,43]. A quantity of gelatin (GEL) was added to deionized water to achieve a concentration of 8% (W/V), to which a quantity of AgNPs solution was added and placed on a magnetic stirrer for dissolution and mixing. After mixing, the solution was defoamed using an ultrasonic apparatus. The prepared GEL and GEL@QM-AgNPs were stored at room temperature.

2.9.1. Changes in Appearance

We selected grapes of uniform shape, size, and ripeness; washed and dried them; and randomly divided them into three groups: control, GEL, and GEL@ QM-AgNPs. The control group was not treated; the remaining two groups were immersed in the coating solution of GEL and GEL@ QM-AgNPs for 10 s, after which they were removed to dry naturally. The grapes were stored under ventilated conditions at room temperature and photographed daily for observation.

2.9.2. Weight Loss

The weight loss of grapes was determined using the weighing method. The grapes were weighed daily and then evaluated according to the following formula:
Weight loss (%) = (M0 − M1)/M0 × 100%
In the formula, M0 represents the initial weight (g); M1 represents the weight after a certain period of time.

2.9.3. Titratable Acidity

A total of 10 g of the sample was ground well and volumed to 50 mL with distilled water. A total of 0.1 mol/L of sodium hydroxide solution was titrated and a few drops of 1% phenolphthalein reagent were added until a slight red color developed and lasted for one minute without fading, repeating the process three times simultaneously. The formula was as follows:
The titratable acidity (%) = [C × (V − V0)]/[(V2/V1) × m] × 100%
where V is the volume of sodium hydroxide consumed in the titration of the sample (mL); V0 is the volume of sodium hydroxide consumed in the titration of the blank sample (mL); C is the concentration of the sodium hydroxide (mol/L); V1 is the raw volume; and V2 is the sample volume.

2.9.4. Total Sugar Content

A certain amount of the grape was weighed, and a small amount of water was added to grind the pulp evenly; meanwhile, water was added to a constant volume of 250 mL. The solution was diluted 100 times after calibration, then a 2% anthrone solution was added to a boiling water bath for 10 min, and removed after cooling to room temperature at a 620 nm wavelength absorbance value, into glucose standard curve [24]. The calculation formula is as follows:
The total sugar content (mg/kg) = (W × M)/(N × 1000)
In this formula, W is the total soluble sugar content obtained by substituting the glucose standard curve (μg); M is the dilution factor; and N is the weight of the sample.

2.9.5. Soluble Solids

The soluble solids content of the grapes was determined by squeezing the juice out of the grapes in each group and dropping the juice onto an Abbe refractometer.

2.9.6. Browning Degree

A homogenate was prepared by mixing 2.0 g of sample with 20 mL of phosphate buffer solution with pH = 7.4, then centrifuged at 106× g for 5 min. The supernatant was obtained to measure the absorbance at 410 nm, and the value derived from A 410 × 10 was taken as the browning value.

2.9.7. Spoilage Rate

The rate of decay was measured as the proportion of decay to the total number. The formula is as follows:
The spoilage rate (%) = (decaying fruit)/(total fruits) × 100

2.9.8. Microbiological Evaluation

When the coating preservation experiment was carried out to the last day, the grapes were taken from each group and the surface of the fruits was rinsed with aseptic water. After rinsing, the water was added to Petri dishes and they were incubated at 37 °C for 16–20 h to observe the growth of the colonies. The colony growth was used to evaluate the preservation effect of AgNPs on grapes.

2.10. Statistical Analysis

All data were evaluated with three, parallel one-way Analysis of Variance (ANOVA) tests and expressed as mean ± standard deviation (SD). The significance variations were indicated at a threshold value of p < 0.05. All data were analyzed by origin Statistical and IBM SPSS Statistics Version 26 software programs.

3. Results

3.1. Optimization of Conditions for Green Synthesis

Following the experimental methodology described above, the color changed to dark brown, indicating the successful synthesis of silver nanoparticles. Figure 1A shows the position of the characteristic absorption peak of QM-AgNPs. Figure 1B–D shows UV-vis spectra of silver nanoparticles synthesized under different conditions.
The UV-Vis spectra of AgNPs synthesized using QM extract at varying concentrations was illustrated. As seen in Figure 1B, with an increase in extract concentration, the number of bioactive ingredients in the system increases, accelerating the reaction rate and enhancing the absorption peak. The maximum absorption peak appeared at a concentration of 0.08 g/mL. When the concentration was increased to 0.1 g/mL, the absorption peak significantly decreased, likely due to the higher concentration of bioactive ingredients promoting the reduction of Ag+ and increasing the probability of agglomeration, thus reducing dispersibility and the absorption peak.
The ultraviolet spectra of AgNPs synthesized at different reaction temperatures are shown in Figure 1C. The absorption peak reached its maximum value at 90 °C, indicating that within certain limits, higher temperatures accelerated the reaction rate and promoted the synthesis of QM-AgNPs. However, further increasing the temperature caused a decrease in the absorption peak, likely due to the destruction of bioactive components in the extract at high temperatures, affecting the synthesis of QM-AgNPs.
Figure 1D depicts the UV-Vis spectra of AgNPs synthesized with an increase in synthesis time. The highest absorption peak was observed at 180 min, indicating the optimal reaction time for the maximum yield of QM-AgNPs. Extending the reaction time to 210 min resulted in a decrease in the absorption peak, possibly due to side reactions forming other substances that attached to the QM-AgNPs’ surface, leading to an increase in particle size and agglomeration, thereby reducing absorbance.

3.2. Analysis of Response Surface Results

The experimental factors and response surface analysis are shown in Figure 2A–F and Tables S1 and S2. The 3D surface plots and contour plots indicated that the response surface initially increased and then decreased with increasing extract concentration and time. The interaction between extract concentration and time was significant, as indicated by the dense contour lines. Regrading the contours, the greater the inclination, the more significantly it affected the synthesis, so the concentration of the extract and the reaction time had a somewhat greater effect on the synthesis of QM-AgNPs. Error analysis and validation experiments confirmed the feasibility of the results, leading to the determination of the optimal conditions for synthesizing silver nanoparticles.

3.3. Characterization Analysis of QM-AgNPs

TEM is one of the important characterization methods to observe the morphology and particle size of QM-AgNPs. Figure 3A shows the electron microscopic image of QM-AgNPs with a spheroid shape, which is consistent with the previous research findings. Meanwhile, the particle size is mainly distributed between 11 and 18 nm.
EDS technology is instrumental in determining elemental composition. For QM-AgNPs, EDS analysis (Figure 3B) revealed a significant absorption peak corresponding to silver, indicating that silver is the primary component. This confirmed the successful synthesis of QM-AgNPs, verifying their elemental composition as predominantly silver.
SAED and XRD were utilized to analyze the phase composition and crystallinity of QM-AgNPs. As shown in Figure 3C,D, the presence of narrow peaks at multiple positions indicates the high crystallinity of the QM-AgNPs. The diffraction pattern displayed several strong peaks at angles corresponding to the (111), (200), (220), (311), and (222) planes of a face-centered cubic (fcc) silver structure. These findings are consistent with those reported in the literature [44,45,46].
The particle size of QM-AgNPs was measured by the dynamic light scattering technique (DLS). As shown in Figure 3E, the particle size distribution of QM-AgNPs’ hydrodynamics is close to a normal distribution. The results indicate that the synthesized QM-AgNPs have good dispersion. This may be due to the active compounds contained in the QM extract, which formed a protective layer around the particles with a spherical shape during the synthesis of AgNPs, ensuring a uniform shape and size. The particle size measured by TEM is the core size, which reflects the actual geometric diameter of silver nanoparticles. DLS measures the hydrodynamic diameter, which includes the core of the nanoparticles, the surrounding solvation layer, and the surface-bound biomolecules. Therefore, the particle size measured by DLS is larger than that measured by TEM.
Figure 3F displays the FTIR spectra of the plant extracts and QM-AgNPs. The plant extracts exhibited distinct absorption peaks at 3436 cm−1, 2918 cm−1, 1632 cm−1, and 1052 cm−1, corresponding to the stretching of O-H, polyphenols, asymmetric stretching of C-H, and S=O in carbohydrates, respectively. Similarly, the spectra of QM-AgNPs showed the stretching of O-H in carbohydrates at 3392 cm−1 and polyphenols at 2917 cm−1. The peaks at 1632 cm−1 and 1052 cm−1 in the plant extracts match with those at 1636 cm−1 and 1031 cm−1 in QM-AgNPs, indicating a crosslink between the plant extracts and AgNPs, which confirmed the effective coverage of organic molecules from the plant extracts on AgNPs [47]. Under optimal conditions, the metal ions immediately interacted with organic substances containing -OH and -COOH functional groups, altering protein conformation and facilitating the synthesis of AgNPs. The flavonoids, proteins, and water-soluble biomolecules in the plant extracts acted as reducing and stabilizing agents in the synthesis of QM-AgNPs.

3.4. Antioxidant Analysis of QM-AgNPs

It can be seen from Figure 4 that QM-AgNPs exhibit the significant ability of scavenging DPPH free radicals in a concentration-dependent manner. Since QM itself is rich in flavonoids, polysaccharides, and other active ingredients that can scavenge free radicals, when QM-AgNPs was synthesized from the QM extract, these active ingredients adhered to the surface of nanoparticles, promoted the formation of QM-AgNPs, and allowed it to possess an excellent free radical scavenging ability. This result is consistent with what has been previously reported in the literature [48,49,50,51].

3.5. Cytotoxicity Studies

3.5.1. Cytotoxicity Evaluation

In this study, cancer cells (A549) and normal cells (HUVECs) were selected as test subjects and treated with different concentrations of QM-AgNPs, and the results are shown in Figure 5A. Cell viability decreased in a dose-dependent manner with an increase in the QM-AgNPs concentration. These results indicate that QM-AgNPs shows anticancer activity against A549 cancer cells, while demonstrating no apparent cytotoxicity to HUVECs, with excellent biocompatibility. QM-AgNPs were able to damage cell components, causing functional defects and interfering with biological functions [52], and exhibited selective toxicity, strongly inhibiting tumor cells while reducing damage to normal cells.

3.5.2. Cell Apoptosis Analysis

AgNPs have two main effects on cells: directly damaging the cell membrane and inducing reactive oxygen species (ROS) release, disrupting the cell’s molecular machinery through oxidative stress responses [53,54]. The apoptosis of lung cancer cells after treatment with different concentrations of QM-AgNPs was observed by Hoechst staining. As shown in Figure 5B, the nuclei of the control cells are larger and show a regular oval shape under the fluorescence microscope, whereas the cells treated with QM-AgNPs show apoptosis (the part of the cells highlighted by the arrows is whitish and glowing), and the number of apoptosis cells increases with the concentration. This may be due to the fact that AgNPs can induce cells to produce excessive reactive oxygen species (ROS), which leads to the damage of cellular organelles, such as mitochondria and lysosomes. In addition, AgNPs cause defective autophagy and inhibit mitochondrial autophagy, which ultimately activate the mitochondria-mediated apoptosis signaling pathway and cause cell death [55].

3.6. Antibacterial Activity of QM-AgNPs

3.6.1. The Inhibition Zone

The result of the inhibition zone is shown in Figure 6A,B, which can be concluded to increase with the increase in the concentration of AgNPs, indicating that the antibacterial effect of QM-AgNPs also improves with the increase in its concentration. Compared with the positive control, amikacin, QM-AgNPs showed similar antibacterial effects against both bacteria at the same concentration (30 μg/mL). However, it is not necessarily better with a higher concentration, and the dosage issue should also be considered [56].

3.6.2. MIC and MBC

The antibacterial results of QM-AgNPs measured by the 96-well plate method [57] are shown in Figure 7A–C. The MIC values of QM-AgNPs against S. aureus and E. coli were 32 μg/mL and 16 μg/mL, respectively, indicating that QM-AgNPs had outstanding resistance against both S. aureus and E. coli. The lower MIC value of E. coli reflected its higher sensitivity to QM-AgNPs compared to S. aureus. The main reason for the different resistance of the two bacteria is the difference in their cell structure [58]. There is no cell wall in Gram-negative bacteria and QM-AgNPs were more likely to enter the bacterial cell. The cell wall of Gram-positive bacteria is composed of thick peptidoglycan, and the peptidoglycan layer is composed of linear polysaccharides crosslinked with short peptides, which makes the penetration of QM-AgNPs more difficult. The results of MBC show that the inhibitory effect of QM-AgNPs on Gram-negative bacteria (64 μg/mL) is stronger than on Gram-positive bacteria (128 μg/mL).

3.6.3. Growth Kinetic Analysis

As shown in Figure 8A,B, in the blank control group, the growth kinetics of bacteria follows a typical pattern, including the lag phase, exponential phase, and stationary phase of bacterial growth, with the fastest growth rate in the first 4 h, after which the rate gradually decreases or even ceases, and finally reaches a plateau, and the growth curve shows an S-shape. In the presence of AgNPs, although the curves still conformed to the typical law, the growth of bacteria showed strong concentration dependence. When the concentration of AgNPs was lower than 1 × MIC, as the concentration of AgNPs increased, the growth of the two kinds of bacteria was delayed to a certain extent. When the concentration of QM-AgNPs reached MIC and 2MIC, the tested bacteria showed little signs of growth. The above results show that QM-AgNPs can inhibit the growth and reproduction of the tested bacteria, and demonstrate a dose-dependent effect. The reason for this phenomenon was mainly due to the fact that QM-AgNPs stimulated the bacteria, causing cell rupture, and thus led to the death of the bacteria. When the concentration of QM-AgNPs was relatively low, it had a certain inhibitory effect on the bacteria at the initial stage of action, but with the increase in the time of action, the reproduction rate of the bacteria became greater than the rate of action of the QM-AgNPs, which resulted in the rapid increase in the bacteria. And when the concentration of QM-AgNPs was high, all the bacteria present in the system could be killed in the reaction period, so the concentration of the bacterial solution would not increase with the increase in the action time.

3.6.4. Antibiofilm Analysis

As shown in Figure 8C, after treatment with QM-AgNPs, the OD570 values of the four tested bacteria show a downward trend, and their biofilm clearance ability is enhanced with the increase in QM-AgNP concentration. When the concentration of QM-AgNPs reached 2MIC, the OD570 of the tested bacteria was much lower than that of the control group. The results show that QM-AgNPs have good biofilm clearance on both strains. When the concentration of QM-AgNPs was low, the inhibitory effect on bacteria was not obvious, and only a small amount of bacterial biofilm was destroyed, and it no longer had an effect after reaching a certain threshold. With an increase in the concentration of QM-AgNPs, all the bacteria present in the system could be destroyed, resulting in biofilm damage. This was due to the fact that as the QM-AgNP concentration increased, the stimulatory effect on the bacteria was more intense, leading to the destruction of more bacterial cells, which in turn caused the bacterial biofilm to rupture.

3.6.5. ROS

Previous studies [31,59,60] have shown that nano-based antimicrobial mechanisms are mostly related to inducing intracellular ROS production. According to previous studies, the pathways of AgNP-induced ROS can be summarized as follows: (1) In the extracellular environment, AgNP particles can induce the production of oxygen radicals (O·) and superoxide oxygen radicals (O2·) during leaching, which are considered to be an important cause of cell membrane rupture; (2) at the cell membrane, AgNPs are likely to induce the leakage of electrons from the respiratory chain enzymes in the membrane into the cytoplasm and react with oxygen (O2) in the cytoplasm to form superoxide radicals (O2·); and (3) intracellularly, the formation of superoxide radicals (O2·) can destroy Fe-S clusters, release Fe2+, and participate in the Fenton reaction to reduce hydroxyl radicals (OH·). Ultimately, free radicals or ROS led to conformational changes in membrane proteins and DNA structure, ultimately leading to cell death. In this study, the relationship between the antibacterial activity of QM-AgNPs and ROS production was further investigated. The intracellular ROS production of bacteria treated with QM-AgNPs was detected using a DCFH-DA probe. As shown in Figure 8D, the fluorescence intensity of the tested bacteria without nano-treatment was low, indicating a low content of reactive oxygen species. After QM-AgNPstreatment, the fluorescence intensity increased sharply, indicating a surge in ROS content in the bacteria. The results show that the ROS content in E. coli increased further, due to the cell wall of Gram-negative bacteria being thinner, and QM-AgNPs being easier to enter, thus promoting the generation of reactive oxygen species and leading to the death of bacteria.

3.6.6. Membrane Permeability Analysis

As described in other research [61,62,63], AgNPs can alter the permeability and respiratory characteristics of cell membranes, thereby inhibiting bacterial growth. When bacteria are damaged under the influence of nanoparticles, components such as proteins and nucleic acids leak out of the cell. As can be seen in Figure 9A–D, the OD260 nm and OD280 nm values of the blank control group, which were not treated with QM-AgNPs, did not change significantly during the reaction time, indicating that the bacterial membranes remained intact, and the bacteria maintained normal growth; whereas, under the treatment with QM-AgNPs, as the reaction time was prolonged, the OD260 nm and OD280 nm values increased gradually. This indicates that the bacterial intracellular substances progressively leaked out with the extension of the reaction time, indicating that bacterial growth was inhibited with the concentration-dependent effect. The increase in the leakage of bacterial intracellular substances indicates that the leakage of bacterial intracellular substances further emphasizes that this leakage was time-dependent. On the other hand, the leakage of bacterial intracellular substances was dose-dependent, which was consistent with the observed antibacterial activity of QM-AgNPs. Therefore, E. coli and S. aureus treated with QM-AgNPs exhibited membrane damage and the leakage of intracellular substances, which are important factors leading to bacterial death.

3.6.7. AO/PI

To further confirm that QM-AgNPs can cause bacterial cell membrane rupture and lead to bacterial death, AO/PI fluorescence staining experiments were conducted [39]. Figure 10A,B shows that the bacteria treated without QM-AgNPs do not exhibit apoptosis and display green fluorescence. With the addition of QM-AgNPs, the bacterial cell membrane was disrupted, leading to bacterial death, which caused PI to stain the nucleus, resulting in red fluorescence. As the concentration of nanoparticles increased, more bacterial apoptosis occurred. Under the fluorescence microscope, most bacteria exhibited yellow–green or red fluorescence, which may be attributed to the binding of fluorescent dyes to nucleic acids in apoptotic or dead bacterial cells. When the concentration of QM-AgNPs reached 2MIC, all the bacteria died, and only red fluorescence appeared in the visual field. These results indicate that QM-AgNPs have a destructive effect on the bacterial cell membrane, leading to the deterioration of bacterial survival and ultimately causing bacterial death, which is consistent with the findings of previous studies [64,65].
Based on the above studies of antibacterial mechanisms, we can briefly guess the mechanism by which QM-AgNPs cause bacterial rupture as follows (Figure 11): firstly, the nanoparticles will accumulate on the bacterial surface in large quantities, destroying the structural integrity of the cell membrane and leading to the leakage and denaturation of proteins in the cell; secondly, they can penetrate the bacteria to enter the intracellular space, directly damaging the DNA of the genetic material. What is more important is that the QM-AgNPs will attack the mitochondria in a targeted manner, inhibiting the activity of key enzymes of the respiratory chain. At the same time, QM-AgNPs induced a large accumulation of reactive oxygen species (ROS), resulting in oxidative stress damage. This multi-target, multi-level combined effect makes it difficult for bacteria to develop drug resistance, which ultimately leads to their death.

3.7. Fruit Preservation

3.7.1. Appearance Changes Analysis

As shown in Figure 12, a certain degree of decay appeared on the fourth day in the blank group without any treatment. With the increase in time, the number of decayed grapes gradually increased, and even fruit flies and larvae appeared on the surface of grapes [66]. By the seventh day, most grapes exhibited severe decay with visible signs of spoilage, including mold growth and tissue maceration. The surface of the GEL-treated grape samples wrinkled to a certain extent due to water loss in the last few days, but no decay occurred, indicating that GEL could slow down the decay of the grapes to a certain extent. In the samples treated by GEL@QM-AgNPs, there were still more well-preserved grape samples on day 8, and no mildew spots appeared.

3.7.2. Weight Loss Analysis

Weight loss rate is an important parameter to measure the shape and quality of fruit during storage. Figure 13A shows the variation in the weight loss rate of grape samples under different treatment conditions. During storage, the weight loss rate of untreated grape samples was significantly higher than that of the other two groups, mainly due to the evaporation of water caused by the respiration and transpiration of the grapes during storage. The GEL group could not adhere to the grape’s surface because of its low adhesion, which could only reduce water loss to a certain extent. With the addition of AgNPs, the GEL@QM-AgNPs group altered the passage of water vapor, which reduced water loss to some extent [67]. The reason for this change in the weight of the grapes in the different groups is that the coating minimizes the contact of the grapes with the atmosphere and slows down the conversion of the pectin substances that maintain the structure of the cell walls to the non-adhesive pectic acid, which ultimately slows down the dehydration and wrinkling of the grapes. This phenomenon suggests that it is the barrier effect of the film coating that plays a dominant role in the apparent changes in film-coated grapes. In conclusion, the use of film coatings to preserve grapes seals the surface of the grapes and reduces their contact with the atmosphere, which in turn attenuates the degree of water loss and respiration.

3.7.3. Analysis of Titratable Acidity

Titratable acidity measures the change in acidity of fruit during storage. As shown in Figure 13B, the titratable acidity of all grape samples decreased with storage time, resulting in a decrease in acidity between the blank control group and the coated group. The reason for the difference between the blank control group and the film-coated treatment group may be the respiration of the grapes in the blank control group was not hindered [68], so their titratable acids were converted into sugars at a faster rate. The difference in grapes between the film-coated treatment groups may be due to the different components of each film-coated treatment group: AgNPs in the GEL@QM-AgNP film have an antioxidant capacity, which can reduce the respiratory rate of grapes and delay the process of post-ripening in grapes. The results show that GEL@QM-AgNP coating on the fruit surface could inhibit the respiration of the fruit and reduce the consumption of organic acids.

3.7.4. Total Sugar Content Analysis

Figure 13C reflects the changes in the total soluble sugar content in grapes under different treatment conditions. The total soluble sugar content of grape samples in the different treatment groups decreased. Sugar respiration in plants is transformed into other substances through glycolysis and other processes; the stronger the respiration, the more sugar and other substances are consumed, and the more energy is generated, making it difficult for fruits and vegetables to be preserved for a long time. Although other substances can be converted into glucose through gluconeogenesis and other pathways, the level of conversion was insufficient to offset consumption, resulting in the total sugar content showing a downward trend. Compared with the control group, the changes in total sugar content in the experimental group were significantly slowed down, indicating that the coating could inhibit respiration to a certain extent, thus slowing the decline in total sugar content. The GEL@QM-AgNP coating effectively maintains the total sugar content of grapes at a high level, thereby prolonging the storage time of grapes.

3.7.5. Analysis of Soluble Solids

Figure 13D shows the change in the soluble solid content of grape samples in different treatment groups. The soluble solids of all grape samples showed a tendency to decrease. The glycogen conversion of grape samples during storage is insufficient to replenish soluble sugars and other substances consumed by respiration, resulting in the reduction in soluble solids [69]. The coating of the experimental group can effectively inhibit respiration and reduce the consumption of soluble sugars and other components in grape samples, thus slowing down the change in soluble solids and inhibiting the corruption of grape samples. The results show that the soluble solids in the GEL@QM-AgNPs group decreased the most slightly, indicating that the coating of this treatment group could effectively inhibit the respiration of fruits and prolong the storage life of fruits.

3.7.6. Browning Analysis

Browning degree is one of the criteria to evaluate the freshness of fruit. As can be seen from Figure 14A, with the prolongation of the storage time, the browning degree in the blank group is the greatest, and GEL@QM-AgNPs is the lowest. The reason may be that GEL@QM-AgNPs can greatly reduce the respiration of grape samples. The reduction of sugar consumption inside the fruit, as well as the addition of QM-AgNPs, can inhibit the microorganisms on the surface of the fruit, thus slowing down the browning of grape samples and extending the preservation time [70].

3.7.7. Spoilage Rate Analysis

The spoilage rate is the most intuitive parameter to measure the freshness of fruit. Figure 14B shows the changes in the spoilage of grape samples in different treatment groups. The spoilage rate of all treatment groups increased with the storage time. When the grape samples were corrupted without any treatment, all of them were spoiled on the seventh day. The GEL group was able to form a coating on the surface of the grape samples, thereby reducing respiration and minimizing spoilage. However, due to its poor adhesion, the coating was separated from the grape epidermis as the grape samples lost water and shrank [71]. QM-AgNPs were added to the GEL@QM-AgNPs group to inhibit microorganisms on the grape’s surface, thus prolonging the storage time. The results show that the GEL@QM-AgNP coating can reduce respiration, inhibit microbial activity, and prolong the storage time of grapes to a certain extent.

3.7.8. Microbiological Analysis

Figure 14C shows the microbial culture on the surface of different treatment groups on day 8. The number of bacterial colonies in the blank and GEL groups was significantly higher than that in the GEL@QM-AgNPs group, which was mainly due to the following reasons: firstly, the blank group lacked any antimicrobial components, providing an ideal growth environment for the microorganisms; and secondly, the simple GEL group, although it had a certain physical barrier effect, had limited antimicrobial activity, and was unable to effectively inhibit the reproduction of microorganisms. In contrast, the uniformly dispersed silver nanoparticles (QM-AgNPs) in the GEL@QM-AgNPs membrane were able to continuously release silver ions, and these silver ions significantly inhibited bacterial growth and reproduction by disrupting the microbial cell membranes, interfering with energy metabolism, and inducing oxidative stress, among other mechanisms [72]. Therefore, the total number of bacterial colonies in the AgNPs composite membrane group was lower, indicating that the GEL@QM-AgNPs membrane could greatly inhibit the growth and reproduction of microorganisms on the surface of the grapes, thus reducing the rotting of the grapes and prolonging the preservation time of the grapes.
The above experimental results demonstrate that the grapes treated with GEL@QM-AgNPs performed better than the other two groups. The possible reason for this is that the addition of QM-AgNPs reduced the pore area of the gel, stabilized the GEL@QM-AgNPs’ structure, and thus reduced the evaporation of water vapor and the diffusion of oxygen. At the same time, it weakened the respiration and transpiration of the fruit, reduced the consumption of nutrients in the fruit during storage, and achieved the purpose of extending the storage time. The effect of nano-silver on fruit preservation was verified.

4. Conclusions

Our study demonstrated that QM extract can be effectively used as both a reducing agent and a capping agent in the green synthesis of silver nanoparticles. SAED and XRD analyses confirmed that the QM-AgNPs possessed a cubic crystalline and metallic structure, while TEM analysis revealed their spherical morphology. FTIR analysis indicated that the active substances in the extract were successfully encapsulated around the silver nanoparticles. Cytotoxicity tests showed that QM-AgNPs had good biocompatibility and significant inhibitory effects on tumor cells. Additionally, the synthesized QM-AgNPs exhibited antibacterial activity against both Gram-positive S. aureus and Gram-negative E. coli. Furthermore, the coating treatment of grapes with QM-AgNPs extended their shelf life and reduced spoilage rates. This study provides a solid foundation for exploring the synthesis and biological applications of silver nanoparticles, contributing to the advancement of nanomaterial synthesis with broad development prospects.

Supplementary Materials

The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/foods14132327/s1, Table S1: Response surface test design and results; Table S2: Analysis of variance of regression model.

Author Contributions

C.Z.: Methodology, Software, Formal analysis, Investigation, and Writing—original draft preparation; Y.L.: Validation and Data curation; Y.H.: Validation and Formal analysis; H.W.: Conceptualization and Supervision; D.W.: Conceptualization, Resources, Writing—review and editing, Project administration, and Funding acquisition. All authors have read and agreed to the published version of the manuscript.

Funding

This work was funded by a grant from the Natural Science Foundation of Shan-dong Province (ZR2022MH270).

Data Availability Statement

The datasets generated for this study are available on request to the corresponding authors.

Conflicts of Interest

The authors declare no conflicts of interest.

References

  1. Liu, J.Z.; Zhang, H.J.; Yan, L.Y.; Kerr, P.G.; Zhang, S.H.; Wu, Y.H. Electron transport, light energy conversion and proteomic responses of periphyton in photosynthesis under exposure to AgNPs. J. Hazard. Mater. 2021, 401, 123809. [Google Scholar] [CrossRef] [PubMed]
  2. Liu, R.; Luo, C.; Pang, Z.Q.; Zhang, J.M.; Ruan, S.B.; Wu, M.Y.; Wang, L.; Sun, T.; Li, N.; Han, L.; et al. Advances of nanoparticles as drug delivery systems for disease diagnosis and treatment. Chin. Chem. Lett. 2023, 34, 107518. [Google Scholar] [CrossRef]
  3. Panda, P.K.; Kumari, P.; Patel, P.; Samal, S.K.; Mishra, S.; Tambuwala, M.M.; Autt, D.; Hilscherová, K.; Mishra, Y.K.; Varma, R.S. Molecular nanoinformatics approach assessing the biocompatibility of biogenic silver nanoparticles with channelized intrinsic steatosis and apoptosis. Green Chem. 2022, 24, 1190–1210. [Google Scholar] [CrossRef]
  4. Kareem, A.A.; Polu, A.R.; Rasheed, H.K.; Rasheed, T. Effect of silver nanoparticles on structural, thermal, electrical, and mechanical properties of poly (vinyl alcohol) polymer nanocomposites. Polym. Compos. 2023, 44, 3281–3287. [Google Scholar] [CrossRef]
  5. Vijayaram, S.; Razafindralambo, H.; Sun, Y.-Z.; Vasantharaj, S.; Ghafarifarsani, H.; Hoseinifar, S.H.; Raeeszadeh, M. Applications of Green Synthesized Metal Nanoparticles—A Review. Biol. Trace Elem. Res. 2024, 202, 360–386. [Google Scholar] [CrossRef]
  6. Thiruvengadam, M.; Rajakumar, G.; Chung, I.-M. Nanotechnology: Current uses and future applications in the food industry. Biotech 2018, 8, 74. [Google Scholar] [CrossRef] [PubMed]
  7. Ying, N.; Liu, S.S.; Zhang, M.M.; Cheng, J.; Luo, L.H.; Jiang, J.Y.; Shi, G.F.; Wu, S.; Ji, J.; Su, H.Y. Nano delivery system for paclitaxel: Recent advances in cancer theranostics. Colloid Surf. B Biointerfaces 2023, 228, 113419. [Google Scholar] [CrossRef]
  8. Hashemitabar, G.; Aflakian, F.; Sabzevar, A.H. Assessment of antibacterial, antioxidant, and anticancer effects of biosynthesized silver nanoparticles using Teucrium polium extract. J. Mol. Struct. 2023, 1291, 136076. [Google Scholar] [CrossRef]
  9. Le, T.T.H.; Ngo, T.H.; Nguyen, T.H.; Hoang, V.H.; Nguyen, V.H.; Nguyen, P.H. Anti-cancer activity of green synthesized silver nanoparticles using Ardisia gigantifolia leaf extract against gastric cancer cells. Biochem. Biophys. Res. Commun. 2023, 661, 99–107. [Google Scholar] [CrossRef]
  10. Ghaseminezhad, S.M.; Hamedi, S.; Shojaosadati, S.A. Green synthesis of silver nanoparticles by a novel method: Comparative study of their properties. Carbohydr. Polym. 2012, 89, 467–472. [Google Scholar] [CrossRef]
  11. Lee, S.H.; Jun, B.-H. Silver Nanoparticles: Synthesis and Application for Nanomedicine. Int. J. Mol. Sci. 2019, 20, 865. [Google Scholar] [CrossRef] [PubMed]
  12. Ahmed, A.H.A.; Mahmoud, A.H.M.; Hiroyuki, K.; Mahmoud, A.Y. Exploring the green synthesis of silver nanoparticles using natural extracts and their potential for cancer treatment. 3 Biotech 2024, 14, 274. [Google Scholar] [CrossRef]
  13. Azizi-Lalabadi, M.; Garavand, F.; Jafari, S.M. Incorporation of silver nanoparticles into active antimicrobial nanocomposites: Release behavior, analyzing techniques, applications and safety issues. Adv. Colloid Interfac. Sci. 2021, 293, 102440. [Google Scholar] [CrossRef] [PubMed]
  14. Beyene, H.D.; Werkneh, A.A.; Bezabh, H.K.; Ambaye, T.G. Synthesis paradigm and applications of silver nanoparticles (AgNPs), a review. Sustain. Mater. Technol. 2017, 13, 18–23. [Google Scholar] [CrossRef]
  15. Vadakkan, K.; Rumjit, N.P.; Ngangbam, A.K.; Vijayanand, S.; Nedumpillil, N.K. Novel advancements in the sustainable green synthesis approach of silver nanoparticles (AgNPs) for antibacterial therapeutic applications. Coord. Chem. Rev. 2024, 499, 215528. [Google Scholar] [CrossRef]
  16. Dogru, E.; Demirbas, A.; Altinsoy, B.; Duman, F.; Ocsoy, I. Formation of Matricaria chamomilla extract-incorporated Ag nanoparticles and size-dependent enhanced antimicrobial property. J. Photochem. Photobiol. B Biol. 2017, 174, 78–83. [Google Scholar] [CrossRef]
  17. Jemilugba, O.T.; Sakho, E.H.M.; Parani, S.; Mavumengwana, V.; Oluwafemi, O.S. Green synthesis of silver nanoparticles using Combretum erythrophyllum leaves and its antibacterial activities. Colloid Interfac Sci. Commun. 2019, 31, 100191. [Google Scholar] [CrossRef]
  18. Ma, L.; Gu, Y.-C.; Luo, J.-G.; Wang, J.-S.; Huang, X.-F.; Kong, L.-Y. Correction to Triterpenoid Saponins from Dianthus versicolor. J. Nat. Prod. 2024, 87, 2908. [Google Scholar] [CrossRef]
  19. Kim, D.H.; Park, G.S.; Nile, A.S.; Kwon, Y.D.; Enkhtaivan, G.; Nile, S.H. Utilization of Dianthus superbus L. and its bioactive compounds for antioxidant, anti-influenza and toxicological effects. Food Chem. Toxicol. 2019, 125, 313–321. [Google Scholar] [CrossRef]
  20. Alghuthaymi, M.A.; Patil, S.; Rajkuberan, C.; Krishnan, M.; Krishnan, U.; Abd-Elsalam, K.A. Polianthes tuberosa-Mediated Silver Nanoparticles from Flower Extract and Assessment of Their Antibacterial and Anticancer Potential. Plants 2023, 12, 1261. [Google Scholar] [CrossRef]
  21. Otoni, C.G.; Avena-Bustillos, R.J.; Azeredo, H.M.; Lorevice, M.V.; Moura, M.R.; Mattoso, L.H.; Mchugh, T.H. Recent advances on edible films based on fruits and vegetables—A review. Compr. Rev. Food Sci. Food Saf. 2017, 16, 1151–1169. [Google Scholar] [CrossRef] [PubMed]
  22. Pandian, H.; Senthilkumar, K.; Naveenkumar, M.; Samraj, S. Azadirachta indica leaf extract mediated silver nanoparticles impregnated nano composite film (AgNP/MCC/starch/whey protein) for food packaging applications. Environ. Res. 2023, 216, 114641. [Google Scholar] [CrossRef] [PubMed]
  23. Ponnusamy, A.; Sr, R.R.; Rajan, R.; Ashraf, F. Chitosan silver nanoparticle inspired seaweed (Gracilaria crassa) biodegradable films for seafood packaging. Algal Res. 2024, 78, 103429. [Google Scholar] [CrossRef]
  24. Zhang, D.-Y.; Yang, J.-X.; Liu, E.-J.; Hu, R.-Z.; Yao, X.-H.; Chen, T.; Zhao, W.-G.; Liu, L.; Fu, Y.-J. Soft and elastic silver nanoparticle-cellulose sponge as fresh-keeping packaging to protect strawberries from physical damage and microbial invasion. Int. J. Biol. Macromol. 2022, 211, 470–480. [Google Scholar] [CrossRef] [PubMed]
  25. Alharbi, A.A.; Alghamdi, A.M.; Al-Goul, S.T.; Allohibi, A.; Baty, R.S.; Qahl, S.H.; Beyari, E.A. Valorizing pomegranate wastes by producing functional silver nanoparticles with antioxidant, anticancer, antiviral, and antimicrobial activities and its potential in food preservation. Saudi J. Biol. Sci. 2024, 31, 103880. [Google Scholar] [CrossRef]
  26. Lieu, M.D.; Dang, T.K.T.; Nguyen, T.H. Green synthesized silver nanoparticles, a sustainable approach for fruit and vegetable preservation: An overview. Food Chem. X 2024, 15, 101664. [Google Scholar] [CrossRef]
  27. Jagtiani, E. Advancements in nanotechnology for food science and industry. Food Front. 2022, 3, 56–82. [Google Scholar] [CrossRef]
  28. Goh, H.T.; Cheok, C.Y.; Yeap, S.P. Green synthesis of silver nanoparticles using banana peel extract and application on banana preservation. Food Front. 2023, 4, 283–288. [Google Scholar] [CrossRef]
  29. Nguyen, T.C.; Nguyen, T.T.T.; Do, Q.T.; Nguyen, D.B.; Tran, T.M.; Tran, L.C.; Tran, T.T.; Nguyen, T.A.; Thai, H. Optimizing the synthesis of hydrotalcite-silver nanoparticles-Allium tuberosum L. hybrid material and its application in chitosan membranes. Inorg. Chem. Commun. 2025, 178, 114535. [Google Scholar] [CrossRef]
  30. Mutalib, M.A.; Rahman, M.A.; Othman, M.H.D.; Ismail, A.F.; Jaafar, J. Scanning Electron Microscopy (SEM) and Energy-Dispersive X-Ray (EDX) Spectroscopy. In Membrane Characterization; Elsevier: Amsterdam, The Netherlands, 2017; pp. 161–179. [Google Scholar] [CrossRef]
  31. Khan, H.; Yerramilli, A.S.; D’oliveira, A.; Alford, T.L.; Boffito, D.C.; Patience, G.S. Experimental methods in chemical engineering: X-ray diffraction spectroscopy—XRD. Can. J. Chem. Eng. 2020, 98, 1255–1266. [Google Scholar] [CrossRef]
  32. Jia, Z.X.; Li, J.T.; Gao, L.; Yang, D.Z.; Kanaev, A. Dynamic light scattering: A powerful tool for in situ nanoparticle sizing. Colloids Interfaces 2023, 7, 15. [Google Scholar] [CrossRef]
  33. Sharifi-Rad, M.; Elshafie, H.S.; Pohl, P. Green synthesis of silver nanoparticles (AgNPs) by Lallemantia royleana leaf Extract: Their Bio-Pharmaceutical and catalytic properties. J. Photochem. Photobiol. A Chem. 2024, 448, 115318. [Google Scholar] [CrossRef]
  34. Khan, S.S.; Ullah, I.; Ullah, S.; An, R.P.; Xu, H.J.; Nie, K.L.; Liu, C.Y.; Liu, L. Recent advances in the surface functionalization of nanomaterials for antimicrobial applications. Materials 2021, 14, 6932. [Google Scholar] [CrossRef] [PubMed]
  35. Protima, R.; Siim, K.; Stanislav, F.; Erwan, R. A Review on the Green Synthesis of Silver Nanoparticles and Their Morphologies Studied via TEM. Adv. Mater. Sci. Eng. 2015, 9, 682749. [Google Scholar] [CrossRef]
  36. Mei, J.; Xu, D.; Wang, L.; Kong, L.; Liu, Q.; Li, Q.; Zhang, X.; Su, Z.; Hu, X.; Zhu, W.; et al. Biofilm microenvironment-responsive self-assembly nanoreactors for all-stage biofilm associated infection through bacterial cuproptosis-like death and macrophage Re-rousing. Adv. Mater. 2023, 35, 2303432. [Google Scholar] [CrossRef]
  37. Oparka, M.; Walczak, J.; Malinska, D.; Oppen, L.M.P.E.; Szczepanowska, J.; Koopman, W.J.H.; Wieckowski, M.R. Quantifying ROS levels using CM-H2DCFDA and HyPer. Methods 2016, 109, 3–11. [Google Scholar] [CrossRef]
  38. Shi, Y.; Bian, L.; Zhu, Y.; Zhang, R.; Shao, S.; Wu, Y.; Chen, Y.; Dang, Y.; Ding, Y.; Sun, H. Multifunctional alkyl ferulate esters as potential food additives: Antibacterial activity and mode of action against Listeria monocytogenes and its application on American sturgeon caviar preservation. Food Control 2019, 96, 390–402. [Google Scholar] [CrossRef]
  39. Ong, K.S.; Cheow, Y.L.; Lee, S.M. The role of reactive oxygen species in the antimicrobial activity of pyochelin. J. Adv. Res. 2017, 8, 393–398. [Google Scholar] [CrossRef]
  40. Bizymis, A.P.; Kalantzi, S.; Mamma, D.; Tzia, C. Addition of Silver Nanoparticles to Composite Edible Films and Coatings to Enhance Their Antimicrobial Activity and Application to Cherry Preservation. Foods 2023, 12, 4295. [Google Scholar] [CrossRef]
  41. Zhang, Z.; Jiang, Q.; Yang, G.; Zhang, X.; Jiang, X.; He, B.; Chen, J. TEMPO-oxidized nanocellulose immobilized AgNPs modified chitosan composite film with durable antibacterial and preservative properties for fruits and vegetables package. Ind. Crops Prod. 2023, 205, 117430. [Google Scholar] [CrossRef]
  42. Qi, Z.; Xie, P.; Yang, C.; Xue, X.; Chen, H.; Zhou, H.; Yuan, H.; Yang, G.; Wang, C. Developing fisetin-AgNPs incorporated in reinforced chitosan/pullulan composite-film and its application of postharvest storage in litchi fruit. Food Chem. 2023, 407, 135122. [Google Scholar] [CrossRef] [PubMed]
  43. Wu, J.; Zhang, Y.; Zhang, F.; Mi, S.; Yu, W.; Sang, Y.; Wang, X. Preparation of chitosan/polyvinyl alcohol antibacterial indicator composite film loaded with AgNPs and purple sweet potato anthocyanins and its application in strawberry preservation. Food Chem. 2025, 463, 141442. [Google Scholar] [CrossRef] [PubMed]
  44. Yu, X.X.; Li, J.Y.; Mu, D.S.; Zhang, H.; Liu, Q.X.; Chen, G.J. Green synthesis and characterizations of silver nanoparticles with enhanced antibacterial properties by secondary metabolites of Bacillus subtilis (SDUM301120). Green Chem. Lett. Rev. 2021, 14, 190–203. [Google Scholar] [CrossRef]
  45. Erenler, R.; Chaoui, R.; Yildiz, I.; Genc, N.; Gecer, E.N.; Temiz, C.; Akkal, S. Biosynthesis, Characterisation, and Antioxidant Activity of Silver Nanoparticles using Schinus molle L. Trends Sci. 2023, 20, 6105. [Google Scholar] [CrossRef]
  46. Tran, N.D.N.; Bui, T.H.; Nguyen, A.P.; Nguyen, T.; Nguyen, V.M.; Duong, N.L.; Nguyen, T. The ability of silver-biochar green-synthesized from Citrus maxima peel to adsorb pollutant organic compounds and antibacterial activity. Green Chem. Lett. Rev. 2022, 15, 18–27. [Google Scholar] [CrossRef]
  47. Mohammed, W.A.; Edbey, K.; Farhat, H.E.; Shah, P.; Shamsi, S.S.; Bhattarai, A. Facile green synthesis of novel AgNPs using Hyoscyamus leaf extract as capping agent: Characterization and their potential antibacterial activities. Inorg. Chem. Commun. 2025, 173, 113893. [Google Scholar] [CrossRef]
  48. Raghupathy, S.; Sivalinga, A.M.; Brahma, N.; Alex, A. Phytochemical Analysis of Silver Nanoparticles of Psidium guajava Leaf Extract and Evaluation for Its Antibacterial Property. J. Pharm. BioAllied Sci. 2024, 16 (Suppl. S2), S1256–S1262. [Google Scholar] [CrossRef]
  49. Bedlovičová, Z.; Strapáč, I.; Baláž, M.; Salayová, A. A brief overview on antioxidant activity determination of silver nanoparticles. Molecules 2020, 25, 3191. [Google Scholar] [CrossRef]
  50. Palithya, S.; Gaddam, S.A.; Kotakadi, V.S.; Penchalaneni, J.; Challagundla, V.N. Biosynthesis of silver nanoparticles using leaf extract of Decaschistia crotonifolia and its antibacterial, antioxidant, and catalytic applications. Green Chem. Lett. Rev. 2021, 14, 137–152. [Google Scholar] [CrossRef]
  51. Magdum, A.B.; Waghmode, R.S.; Shinde, K.V.; Mane, M.P.; Kamble, M.V.; Kamble, R.S.; Jangam, A.; Pawar, K.; Sonawane, K.D.; Patil, P. Biogenic synthesis of silver nanoparticles from leaves extract of Decaschistia trilobata an endemic shrub and its application as antioxidant, antibacterial, anti-inflammatory and dye reduction. Catal. Commun. 2024, 187, 106865. [Google Scholar] [CrossRef]
  52. Salih, R.; Bajou, K.; Shaker, B.; Elgamouz, A. Antitumor effect of algae silver nanoparticles on human triple negative breast cancer cells. Biomed. Pharmacother. 2023, 168, 115532. [Google Scholar] [CrossRef] [PubMed]
  53. Thakkar, A.B.; Subramanian, R.; Thakkar, V.R.; Bhatt, S.V.; Chaki, S.; Vaidya, Y.H.; Patel, V.; Thakor, P. Apoptosis induction capability of silver nanoparticles capped with Acorus calamus L. and Dalbergia sissoo Roxb. Ex DC. against lung carcinoma cells. Heliyon 2024, 10, 26. [Google Scholar] [CrossRef] [PubMed]
  54. Venmani, S.; Kesavan, M.P.; Ayyanaar, S.; Muniyappan, N. Cymodocea serrulata-capped silver nanoparticles for battling human lung cancer, breast cancer, hepatic cancer: Optimization by full factorial design and in vitro cytotoxicity evaluation. Heliyon 2023, 9, 27. [Google Scholar] [CrossRef]
  55. Sanfelice, R.A.D.S.; Bortoleti, B.T.D.S.; Tomiotto-Pellissier, F.; Silva, T.F.; Bosqui, L.R.; Nakazato, G.; Castilho, P.M.; De, B.L.D.; Garcia, J.L.; Lazarin-Bidóia, D.; et al. Biogenic silver nanoparticles (AgNp-Bio) reduce Toxoplasma gondii infection and proliferation in HeLa cells, and induce autophagy and death of tachyzoites by apoptosis-like mechanism. Acta Trop. 2021, 222, 106070. [Google Scholar] [CrossRef]
  56. Ferdous, Z.; Nemmar, A. Health impact of silver nanoparticles: A review of the biodistribution and toxicity following various routes of exposure. Int. J. Mol. Sci. 2020, 21, 2375. [Google Scholar] [CrossRef]
  57. CLSI (Ed.) Methods for Dilution Antimicrobial Susceptibility Tests for Bacteria that Grow Aerobically, 11th ed.; CLSI Document M07; Clinical and Laboratory Standards Institute: Wayne, PA, USA, 2018. [Google Scholar]
  58. Al-mehdhar, A.A.; Alarjani, K.M.; Aldosari, N.S.; Alghamdi, M.A. Antibacterial Efficacy of AgNPs synthesized from Aloe vera extract and Staphylococcus aureus Culture Supernatant. J. King Saud Univ. Sci. 2024, 36, 103464. [Google Scholar] [CrossRef]
  59. Farooq, M.A.; Hannan, F.; Islam, F.; Ayyaz, A.; Zhang, N.; Chen, W.-Q.; Zhang, K.N.; Huang, Q.; Xu, L.; Zhou, W.J. The potential of nanomaterials for sustainable modern agriculture: Present findings and future perspectives. Environ. Sci. Nano 2022, 9, 1926–1951. [Google Scholar] [CrossRef]
  60. Fadaka, A.O.; Sibuyi, N.R.S.; Madiehe, A.M.; Meyer, M. Nanotechnology-based delivery systems for antimicrobial peptides. Pharmaceutics 2021, 13, 1795. [Google Scholar] [CrossRef]
  61. Netala, V.R.; Hou, T.Y.; Sana, S.S.; Li, H.Z.; Zhang, Z.J. Rosmarinic Acid-Rich Perilla frutescens Extract-Derived Silver Nanoparticles: A Green Synthesis Approach for Multifunctional Biomedical Applications including Antibacterial, Antioxidant, and Anticancer Activities. Molecules 2024, 29, 1250. [Google Scholar] [CrossRef]
  62. Oh, S.-J.; Kim, H.; Liu, Y.Q.; Han, H.-K.; Kwon, K.; Chang, K.-H.; Park, K.; Kim, Y.; Shim, K.; An, S.S.A.; et al. Incompatibility of silver nanoparticles with lactate dehydrogenase leakage assay for cellular viability test is attributed to protein binding and reactive oxygen species generation. Toxicol. Lett. 2014, 225, 422–432. [Google Scholar] [CrossRef]
  63. Çiğdem, U.; Yılmaz, Ö.B.; Dağ, İ. Biosynthesis, Characterization and Optimization of Silver Nanoparticles with Strong Antibacterial Activity Using Cell Extracts of Cyanobacterial Chroococcus sp. ChemistrySelect 2024, 9, e202304895. [Google Scholar] [CrossRef]
  64. Martínez-Esquivias, F.; Gutiérrez-Angulo, M.; Pérez-Larios, A.; Sánchez-Burgos, J.A.; Becerra-Ruiz, J.S.; Guzmán-Flores, J.M. Anticancer activity of selenium nanoparticles in vitro studies. Anti-Cancer Agents Med. Chem. 2022, 22, 1658–1673. [Google Scholar] [CrossRef] [PubMed]
  65. Tiwari, M.; Kumar, P.; Tejavath, K.K.; Tiwari, V. Assessment of Molecular Mechanism of Gallate-Polyvinylpyrrolidone-Capped Hybrid Silver Nanoparticles against Carbapenem-Resistant Acinetobacter baumannii. ACS Omega 2020, 5, 1206–1213. [Google Scholar] [CrossRef]
  66. Liu, Y.; Yuan, Y.; Duan, S.; Li, C.; Hu, B.; Liu, A.; Wu, D.; Cui, H.; Lin, L.; He, J.; et al. Preparation and characterization of chitosan films with three kinds of molecular weight for food packaging. Int. J. Biol. Macromol. 2020, 155, 249–259. [Google Scholar] [CrossRef]
  67. Meng, X.; Li, B.; Liu, J.; Tian, S. Physiological responses and quality attributes of table grape fruit to chitosan preharvest spray and postharvest coating during storage. Food Chem. 2008, 106, 501–508. [Google Scholar] [CrossRef]
  68. Du, Y.; Yang, F.; Yu, H.; Cheng, Y.; Guo, Y.; Yao, W.; Xie, Y. Fabrication of novel self-healing edible coating for fruits preservation and its performance maintenance mechanism. Food Chem. 2021, 351, 129284. [Google Scholar] [CrossRef] [PubMed]
  69. Hajji, S.; Younes, I.; Affes, S.; Boufi, S.; Nasri, M. Optimization of the formulation of chitosan edible coatings supplemented with carotenoproteins and their use for extending strawberries postharvest life. Food Hydrocoll. 2018, 83, 375–392. [Google Scholar] [CrossRef]
  70. Lin, Y.; Lin, H.; Zhang, S.; Chen, Y.; Chen, M.; Lin, Y. The role of active oxygen metabolism in hydrogen peroxide-induced pericarp browning of harvested longan fruit. Postharvest Biol. Technol. 2014, 96, 42–48. [Google Scholar] [CrossRef]
  71. Kou, X.; He, Y.; Li, Y.; Chen, X.; Feng, Y.; Xue, Z. Effect of abscisic acid (ABA) and chitosan/nano-silica/sodium alginate composite film on the color development and quality of postharvest Chinese winter jujube (Zizyphus jujuba Mill. cv. Dongzao). Food Chem. 2019, 270, 385–394. [Google Scholar] [CrossRef]
  72. Valenzuela, C.; Tapia, C.; López, L.; Bunger, A.; Escalona, V.; Abugoch, L. Effect of edible quinoa protein-chitosan based films on refrigerated strawberry (Fragaria × ananassa) quality. Electron. J. Biotechnol. 2015, 18, 406–411. [Google Scholar] [CrossRef]
Foods 14 02327 g001
Figure 1. The UV-Vis absorption spectra of AgNO3, QM-extraction, and QM-AgNPs (A); UV-Vis absorption spectra of QM-AgNPs showing the effects of extract concentration (B); temperature (C); time (D).
Figure 1. The UV-Vis absorption spectra of AgNO3, QM-extraction, and QM-AgNPs (A); UV-Vis absorption spectra of QM-AgNPs showing the effects of extract concentration (B); temperature (C); time (D).
Foods 14 02327 g001
Foods 14 02327 g002
Figure 2. Response surface plots of the 2D contour and 3D surface plots of the QM-AgNPs. Temperature and time (A,B); extract concentration and temperature (C,D); extract concentration and time (E,F).
Figure 2. Response surface plots of the 2D contour and 3D surface plots of the QM-AgNPs. Temperature and time (A,B); extract concentration and temperature (C,D); extract concentration and time (E,F).
Foods 14 02327 g002
Foods 14 02327 g003
Figure 3. TEM images of spherical QM-AgNPs (A); EDX spectra of QM-AgNPs (B); XRD (C) and SAED (D) spectra of QM-AgNPs; particle size distributions of QM-AgNPs with respect to intensity (E); FTIR spectra of QM-AgNPs and QM power (F).
Figure 3. TEM images of spherical QM-AgNPs (A); EDX spectra of QM-AgNPs (B); XRD (C) and SAED (D) spectra of QM-AgNPs; particle size distributions of QM-AgNPs with respect to intensity (E); FTIR spectra of QM-AgNPs and QM power (F).
Foods 14 02327 g003
Foods 14 02327 g004
Figure 4. DPPH radical scavenging activity analysis of QM-AgNPs. Note: The DPPH radical scavenging effect of QM-AgNPs (5, 10, 25, 50, 100, 250, 500 μg/mL) was detected by DPPH radical scavenging assay; Vc (vitamin C) (5, 10, 25, 50, 100, 250, 500 μg/mL) was used as the positive control. Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Figure 4. DPPH radical scavenging activity analysis of QM-AgNPs. Note: The DPPH radical scavenging effect of QM-AgNPs (5, 10, 25, 50, 100, 250, 500 μg/mL) was detected by DPPH radical scavenging assay; Vc (vitamin C) (5, 10, 25, 50, 100, 250, 500 μg/mL) was used as the positive control. Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Foods 14 02327 g004
Foods 14 02327 g005
Figure 5. The results of the proliferation of QM-AgNPs (0, 5, 25, 125 μg/mL) on A549 and HUVECs (A); cell apoptosis of QM-AgNPs (0, 5, 25, 125 μg/mL) in lung cancer cells by Hoechst nuclear staining (B). Note: A549 and HUVECs were incubated with QM-AgNPs for 24 h. Cell viability was detected with MTT reagent. The arrows in the figure indicate apoptotic cells. Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Figure 5. The results of the proliferation of QM-AgNPs (0, 5, 25, 125 μg/mL) on A549 and HUVECs (A); cell apoptosis of QM-AgNPs (0, 5, 25, 125 μg/mL) in lung cancer cells by Hoechst nuclear staining (B). Note: A549 and HUVECs were incubated with QM-AgNPs for 24 h. Cell viability was detected with MTT reagent. The arrows in the figure indicate apoptotic cells. Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Foods 14 02327 g005
Foods 14 02327 g006
Figure 6. Zones of inhibition of N-30 and QM-AgNPs (15, 30, 45 μg/disc) against E. coli and S. aureus (A,B). Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Figure 6. Zones of inhibition of N-30 and QM-AgNPs (15, 30, 45 μg/disc) against E. coli and S. aureus (A,B). Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Foods 14 02327 g006
Foods 14 02327 g007
Figure 7. Analysis of MIC results against E. coli and S. aureus by QM-AgNPs (A). Analysis of MBC results against E. coli (B) and S. aureus (C) by QM-AgNPs. Note: The red boxes on the figure represent the MIC and MBC values of the corresponding bacteria. The boxes in other colors are only used to distinguish between different treatment groups.
Figure 7. Analysis of MIC results against E. coli and S. aureus by QM-AgNPs (A). Analysis of MBC results against E. coli (B) and S. aureus (C) by QM-AgNPs. Note: The red boxes on the figure represent the MIC and MBC values of the corresponding bacteria. The boxes in other colors are only used to distinguish between different treatment groups.
Foods 14 02327 g007
Foods 14 02327 g008
Figure 8. Growth curves of different bacteria under the action of QM-AgNPs, E. coli (A); S. aureus (B); anti-biofilm effects of QM-AgNPs (C); DFCH-DA measurement of ROS results (D). Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Figure 8. Growth curves of different bacteria under the action of QM-AgNPs, E. coli (A); S. aureus (B); anti-biofilm effects of QM-AgNPs (C); DFCH-DA measurement of ROS results (D). Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Foods 14 02327 g008
Foods 14 02327 g009
Figure 9. Effect of QM-AgNPs on extracellular nucleic acid leakage from different bacteria: E. coli (A); S. aureus (B). Effect of QM-AgNPs on extracellular nucleic acid leakage from different bacteria: E. coli (C); S. aureus (D). Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Figure 9. Effect of QM-AgNPs on extracellular nucleic acid leakage from different bacteria: E. coli (A); S. aureus (B). Effect of QM-AgNPs on extracellular nucleic acid leakage from different bacteria: E. coli (C); S. aureus (D). Data are expressed as mean ± standard error (n = 3); different letters indicate significant differences (p < 0.05), based on one-way ANOVA followed by Tukey’s HSD test. (The analysis is focused on comparisons within the same group, that is, comparing the same sample at different concentrations).
Foods 14 02327 g009
Foods 14 02327 g010
Figure 10. AO/PI staining results of QM-AgNPs acting on E. coli (A) and S. aureus (B).
Figure 10. AO/PI staining results of QM-AgNPs acting on E. coli (A) and S. aureus (B).
Foods 14 02327 g010
Foods 14 02327 g011
Figure 11. Mechanism of bacterial death caused by QM-AgNPs.
Figure 11. Mechanism of bacterial death caused by QM-AgNPs.
Foods 14 02327 g011
Foods 14 02327 g012
Figure 12. The changes in the appearance of different grape samples during storage. Note: The marks in the picture indicate where the grapes have rotted.
Figure 12. The changes in the appearance of different grape samples during storage. Note: The marks in the picture indicate where the grapes have rotted.
Foods 14 02327 g012
Foods 14 02327 g013
Figure 13. The weight loss of grapes in different types of film (A); changes in the titratable acidity of different types grapes (B); changes in the total sugar content of grape samples (C); changes in the soluble solids of grape samples (D).
Figure 13. The weight loss of grapes in different types of film (A); changes in the titratable acidity of different types grapes (B); changes in the total sugar content of grape samples (C); changes in the soluble solids of grape samples (D).
Foods 14 02327 g013
Foods 14 02327 g014
Figure 14. The changes in the browning degree of grape samples (A); changes in the corruption rate of grape samples (B); biological evaluation of the surface of grapes (C).
Figure 14. The changes in the browning degree of grape samples (A); changes in the corruption rate of grape samples (B); biological evaluation of the surface of grapes (C).
Foods 14 02327 g014
Table 1. Experimental factors and levels of the independent test variables.
Table 1. Experimental factors and levels of the independent test variables.
Test ParametersLevels of Test Parameters
−101
Temperature (°C)859095
Time (min)150180210
Material–liquid ratio (%)6810
Disclaimer/Publisher’s Note: The statements, opinions and data contained in all publications are solely those of the individual author(s) and contributor(s) and not of MDPI and/or the editor(s). MDPI and/or the editor(s) disclaim responsibility for any injury to people or property resulting from any ideas, methods, instructions or products referred to in the content.

Share and Cite

MDPI and ACS Style

Zhang, C.; Li, Y.; Huo, Y.; Wang, H.; Wang, D. Dianthus superbus L. (QM) Extract-Assisted Silver Nanoparticle Gelatin Films with Antioxidant and Antimicrobial Properties for Fresh Fruit Preservation. Foods 2025, 14, 2327. https://doi.org/10.3390/foods14132327

AMA Style

Zhang C, Li Y, Huo Y, Wang H, Wang D. Dianthus superbus L. (QM) Extract-Assisted Silver Nanoparticle Gelatin Films with Antioxidant and Antimicrobial Properties for Fresh Fruit Preservation. Foods. 2025; 14(13):2327. https://doi.org/10.3390/foods14132327

Chicago/Turabian Style

Zhang, Chenwei, Yao Li, Yue Huo, Hongtao Wang, and Dandan Wang. 2025. "Dianthus superbus L. (QM) Extract-Assisted Silver Nanoparticle Gelatin Films with Antioxidant and Antimicrobial Properties for Fresh Fruit Preservation" Foods 14, no. 13: 2327. https://doi.org/10.3390/foods14132327

APA Style

Zhang, C., Li, Y., Huo, Y., Wang, H., & Wang, D. (2025). Dianthus superbus L. (QM) Extract-Assisted Silver Nanoparticle Gelatin Films with Antioxidant and Antimicrobial Properties for Fresh Fruit Preservation. Foods, 14(13), 2327. https://doi.org/10.3390/foods14132327

Note that from the first issue of 2016, this journal uses article numbers instead of page numbers. See further details here.

Article Metrics

Back to TopTop