Solanum Procumbens-Derived Zinc Oxide Nanoparticles Suppress Lung Cancer In Vitro through Elevation of ROS

Lung cancer is one of the cancers with high mortality rate. The current therapeutic regimens have only limited success rate. The current work highlights the potential of Solanum procumbens-derived zinc oxide nanoparticle (SP-ZnONP)-induced apoptosis in A549 lung cancer cells. Synthesized nanoparticles were confirmed by UV-Vis spectrophotometry, X-ray diffraction (XRD), dynamic light scattering analysis (DLS), scanning electron microscopy (SEM), Fourier transform infrared (FT-IR), and photoluminescence analysis. Lactate dehydrogenase (LDH), cytotoxicity, and cell viability assays revealed that the SP-ZnONP caused the cell death and the inhibition concentration (IC50) was calculated to be 61.28 μg/mL. Treatment with SP-ZnONPs caused morphological alterations in cells, such as rounding, which may have been caused by the substance's impact on integrins. Acridine orange/ethidium bromide dual staining revealed that the cells undergo apoptosis in a dose-dependent manner, which indicates the cell death. Furthermore, reactive oxygen species (ROS) were examined and it was shown that the nanoparticles elevated ROS levels, which led to lipid peroxidation. In short, the SP-ZnONPs increase the level of ROS, which in turn causes lipid peroxidation results in apoptosis. On the other hand, the SP-ZnONPs decrease nitric oxide level in A549 cells in a dose-dependent manner, which also supports the apoptosis. In conclusion, SP-ZnONPs would become a promising treatment option for lung cancer.


Introduction
Lung cancer is one of the leading causes of cancer-mediated deaths worldwide [1]. Although a variety of treatment strategies such as surgery, radiation therapy, chemotherapy, and targeted therapy has been followed to treat lung cancer, the outcome is poor [2]. Targeted therapy using inhibitors of angiogenesis, KRAS, EGFR, AKL, and BRAF has also been widely used to treat lung cancers. In spite of a variety of targeted therapeutic agents, the success is very much limited. erefore, we explored the possibility of Solanum procumbens-derived zinc oxide nanoparticle (SP-ZnONP) for treating lung cancer.
Experimentally, zinc oxide nanoparticles (ZnONPs) have already been shown to be effective in alleviating the cancer. Particularly, ZnONPs have become a one of the treatment options for cancer due to several reasons such as biocompatibility, selectivity, ease of synthesis, ability to induce cytotoxicity, and high surface area to volume ratio [3]. In addition, ZnONPs efficiently involve in the redox reaction system led to elevate the reactive oxygen species (ROS) [4]. Most importantly, selective cytotoxicity is enhanced by ZnONPs since ROS and related signalling molecules are produced more in cancer cells due to rapid metabolic rate compared with normal cells [5]. Recent reports suggest that ZnONPs are also effective in reducing the stemness of cancer stem cells in breast cancer [6].
Solanum procumbens Lour. (Solanaceae) is a tropical plant found in South East China, Vietnam, ailand, Laos, and Hainan. It has been widely used in traditional and folk medicines. Formulations containing this plant extract have been used for the treatment of ailments such as rheumatism, pain, detoxification, hepatitis, and cirrhosis. [7]. Spirosolane alkaloids, pregnane steroids, and steroidal saponins are major constituents of Solanum procumbens extracts [8]. In the present work, we prepared Solanum procumbens extract and used for the preparation ZnONPs and evaluated its potency to treat lung cancer.

Plant Extract Preparation.
e fresh leaves of Solanum procumbens (SP) were collected and thoroughly washed with distilled water to eliminate dirt particles and prevent contamination. With the help of mortar and pestle, around 5 g of Solanum procumbens leaves was prepared into fine paste and blended in 500 mL of distilled water and then heated at 70°C for 30 minutes. Further filtration of extract was carried out by muslin cloth followed by Whatman filter paper. e filtered plant extract stored at 5°C for further applications.

Synthesis and Characterization of Green-Synthesized
ZnONPs [9]. An aqueous solution of 95 ml zinc chloride (0.01 M) was mixed with 5 mL of plant extract of Solanum procumbens. e mixture was kept in a shaking incubator for 1 hour at 70°C with 150 rpm. At the end of the reaction, a white precipitate settled at the bottom of the flask. e supernatant was removed from the white precipitate and transferred to a 1.5-mL centrifuge tubes. e samples were washed with distilled water through centrifugation at 3000 rpm for 30 minutes and repeated process thrice to remove impurities completely and dried in a hot air oven at 90°C. e dried product was then ground into a powder using mortar and pestle and calcined at 500°C for 2 hrs. Finally, the resultant annealed powder stored in an airtight glass vial and labelled as SP-ZnONPs. e optical properties synthesized SP-ZnONPs were analysed using UV-Vis and photo-luminescence spectroscopy. Its physical nature and particle size were obtained by XRD and DLS. Furthermore, shape and surface morphology were identified using TES-CAN VEGA3 scanning electron microscopy (SEM). Fourier transform infrared (FTIR) spectroscopy was used to confirm the existence of functional groups in the synthesized nanoparticles.

Cell Viability by Trypan Blue Exclusion Assay.
e lethality of SP-ZnONPs on A549 cells was assessed by the trypan blue exclusion test (Crowley et al. ) [11]. Cells were seeded in 6-well plates with different concentrations of SP-ZnONPs as 10,20,30,40,50,60,70,80,90, and 100 μg/mL for 24 h of exposure in a humidified incubator (5% CO 2 , 37°C). ereafter, cells were trypsinized and resuspended in equal volume of culture medium and trypan blue stain. Viable (unstained) and nonviable (blue-stained) cells were counted using a haemocytometer to calculate the total number of live and dead cells.

Morphometric Analysis.
e morphological changes of apoptotic cells were analysed by the method reported elsewhere [12] with slight modifications. After seeding 5 × 10 5 cells, it was incubated for 24 hours and treated with three concentrations of SP-ZnONPs (50, 60, and 70 μg/mL) for another 24 hours. e medium was removed, and cells were washed with PBS and observed for morphological changes of the treated cells under inverted phase contrast microscope at 20X magnifications.

Analysis of Dual Staining.
e apoptotic cell death analysis was carried out by fluorescence microscope combining the methods by Reference [13,14]. SP-ZnONPstreated A549 cells were investigated by AO/EB fluorescence staining techniques for morphological alterations due to apoptosis. 1 × 10 5 cells were seeded in a 12-well plate over sterile coverslips coated with Poly-L-Ornithine solution and incubated in a CO 2 incubator overnight at 37°C for 24 hours. After removal of medium, the cells were treated with different concentrations of SP-ZnONPs (50, 60, and 70 μg/mL and control) and incubated for 48 hours. e medium was removed and washed with PBS. Coverslips were washed with 1 mL 1X DPBS and stained with 200 μL staining solution (1 mL of ethidium bromide (50 μg/mL) and 20 μL of acridine orange (20 μg/mL)) for 10 minutes. e staining solution was removed and observed under fluorescence spectroscopy with excitation at 560/40 nm and emission at 645/75 nm for EtBr and excitation 470/40 and emission 525/50 for acridine orange and recorded using ImageJ software.

ROS Estimation.
e NBT reduction assay was performed to estimate the ROS, which is slightly modified version of Abdulhamid and Morgan method [15]. 1 × 10 5 cells/mL cells were seeded and incubated for 24 hours. SP-ZnONPs were then added onto the appropriate well at different concentrations such as 50, 60, and 70 μg/mL and incubated for 24 hours and washed with PBS twice. 100 μL of 0.1% NBT solution was added and incubated for 1 hour followed by 70% of methanol thrice. About 120 μL of 2 Bioinorganic Chemistry and Applications 2 M potassium hydroxide (KOH) with 120 μl of DMSO was added and read using plate reader at 630 nm, and the DMSO was considered as blank.

Determining Nitric Oxide Concentration.
Nitric oxide concentration was estimated according to the method explained by Grdovicet al. [16]. 100 μl of (100 μM) of nitrite solution was added to each well of 96-well plate to perform nitrite standard reference curve. To achieve desired concentration, a series of dilutions was performed (100, 50, 25, 12.5, 6.25, 3.13, and 1.56 μM). e equilibration of sulphanilamide and NED solutions was performed at room temperature (15-30 minutes). 50 μL of each (various concentrations such as 50, 60, and 70 μg/mL of SP-ZnONPstreated solutions) was added to experimental supernatants to the wells as duplicates. Further 50 μL of the 1% sulphanilamide dissolved in 5% phosphoric acid was added to samples in dilution series as a standard. e reaction mixture was incubated for 5-10 minutes at room temperature and protected from light followed by 50 μL of the 0.1% NED solution to all wells. e absorbance was measured within 30 minutes after the colour generation at 520 nm and 550 nm.

Quantification of Lipid Peroxidation.
e lipid peroxidation was quantified through spectrophotometrically by the complex formation of [17] malondialdehyde with thiobarbituric acid. e cells at the density of 1 × 10 4 were seeded and incubated for 24 hours and treated with various concentrations of SP-ZnONPs (50, 60, and 70 μg/ mL). e treated cells were taken, and the pellet was washed and redispersed into 0.2 mL of 8.1% SDS. en, 1.5 mL of 20% acetic acid was added to this suspension and incubated for 10 minutes, and then added with 1.5 mL of 0.8% TBA buffer and 0.7 mL of distilled water. is reaction mixture was incubated at 95°C for 1 hour, cooled to 25°C, and subjected to centrifugation at 5000 rpmg for 15 minutes to remove cell debris. Finally, the absorbance spectra were recorded at 532 nm along with blank and control.
2.10. Measurement of LDH Activity. LDH activity was determined according to the slightly modified version of reported method [18]. e cells at the density of 1 × 10 4 cells/ well were seeded and incubated for 24 hours followed by treatment with various concentrations (50, 60, and 70 μg/ mL) of SP-ZnONPs. e supernatant of treated cells was separated by centrifugation at 4°C for 10 minutes at 3000 rpm. LDH leakage was measured in a 3.0 mL of reaction mixture (28 mL of 100 mM potassium phosphate buffer pH 7.5, 1.20 mL of 100 mM sodium pyruvate, and 0.8 mL of 13.1 mM NADH; 3 mL of mixture incubated at 37°C for 3 minutes) with 10 μL supernatant. e absorbance was recorded at 1-minute interval up to 4 minutes at 340 nm. e amount of LDH released is expressed as U/mg of protein in culture media.

Statistical Analysis.
e triplicate results of all experiments were subjected to statistical analysis using GraphPad Prism version 5.1. Data are presented as mean ± standard deviation by one-way analysis of variance (ANOVA) with Tukey's multiple t-test.

Characterization of Green-Synthesized SP-ZnONPs
3.1.1. UV-Visible Spectroscopy. Zinc ions in the solution converted into o zinc oxide due to the presence of secondary metabolites in plant extract. Here, the plant extract acts as a pH altering and stabilizing agent. e UV-Vis absorption spectrum of SP-ZnONPs shows peak at 372 nm, which is around 7 nm red shifted compared with the bulk ZnO that shows peak at 365 nm, which confirms the formation of SP-ZnONPs ( Figure 1).

XRD and DLS Analysis.
e generation of SP-ZnONPs was confirmed by XRD with Bragg's reflection, which corresponds to (100) Figure 3. e reason for the higher particle size observed in DLS than that of in XRD is due to its hydrodynamic character. Figure 4 shows photoluminescence spectrum of SP-ZnONPs with the excitation wavelength at 325 nm.

SEM Analysis of Nanoparticles.
e scanning electron microscope (SEM) was used to characterize the morphology of green-synthesized SP-ZnONPs. Figure 5 shows the SEM image of the prepared nanoparticles, which reveals that the nanoparticles are well distributed and, more significantly, that they have an aggregative nature. 3.3. FTIR Analysis. FTIR spectrum of Solanum procumbens extract and SP-ZnONPs was shown in Figure 6(a) and 6(b), respectively. e peak at 495 cm −1 in the Figure 6(b) confirms the presence of SP-ZnONPs because the peak between 400 and 600 cm −1 region responsible for stretching frequency of Zn-O bond in ZnONPs.
e broad peak at 3436 cm −1 in both Figures 6(a) and 6(b) confirms the presence of alcohol and phenolic OH groups; it is clearly understood that phenols and alcohols present in the extract are caped with the nanoparticles.

Cytotoxicity Assay.
In order to understand the ability of green-synthesized SP-ZnONPs on the cancer treatment, these nanoparticles are treated with A549 lung cancer cell line. In the MTT assay, a dose-dependent cell death was observed. At a higher concentration of the nanoparticles (200 μg/mL), 100% of cell death is observed. At lower concentrations (5 μg/mL), there were little effects on cells in terms of viability ( Figure 7). Overall, there was a dose-dependent cell death observed with green-synthesized nanoparticles and the IC 50 was calculated to be 61.28 μg/mL. With this result, it is apparent that the nanoparticle is highly effective in inhibiting the cell proliferation of lung cancer cells.

Cell Viability Assay.
e relative proportion of viable cells was analysed using trypan blue exclusion assay. At 10 μg/mL concentration, there were 93% cell viability, and at 100 μg/mL, a majority of cells were died (Figure 8). 50% of cell death was observed at 60 μg/mL concentration, which surprisingly correlates with value found in MTT assay.

Morphological Analysis.
As the nanoparticles induced cell death in a dose-dependent manner, the cells were visualized under microscope to check for any morphological changes. Consistent with earlier observations, there was a dose-dependent reduction in cell number when observed under microscope. In addition, there is a significant difference in the morphology of A549 cells observed under the microscope. ere is a significant decrease in the number of cells on treatment with SP-ZnONPs at concentrations of 50,    (Figure 9(b)-9(d)). e normal architecture was observed in untreated cells (Figure 9(a)). 5 μg/mL of standard control cisplatin showed an increased number of apoptotic cells (Figure 9(e)).

Dual Staining-Acridine Orange/EtBr Staining.
e signs of apoptosis were evaluated using acridine orange/ethidium bromide dual staining. Morphological changes in cancer cell nuclei were observed by fluorescent microscopy, which differentiates between normal and apoptotic cells. e observations in the fluorescent micrograph reveal that the death of A549 cells increased at high dosage of SP-ZnONPs (70 μg/mL) (Figure 10(d)) compared with untreated cells (Figure 10(a)); it is showing that greater number of apoptotic cells were observed with blebbing of cell membrane and chromatin condensation in a dose-dependent manners. At 50 μg/mL concentration, cells with various morphologies with varying stages of apoptosis such as healthy cells and early apoptotic cells could be observed. Necrotic cells could also be observed rarely (Figure 10(b)). In the 60 μg/mL concentration, all types of cells such as viable cells, early apoptotic cells, and late apoptotic cells including some necrotic cells were evidenced (Figure 10(c)). Relative proportion of viable cells decreased with higher incidence of early and late apoptotic cells in 70 μg/mL concentration (Figure 10(d)).

Estimation of ROS Level.
e ROS level in A549 cell line was evaluated using NBT reduction assay. 50, 60, and 70 μg/ mL concentrations of SP-ZnONPs were chosen for assay and treated with the A549 cells. A dose-dependent significant increase in ROS level with increasing concentration of SP-

Bioinorganic Chemistry and Applications
ZnONPs was observed (P value > 0.0001). ROS level is apparently increasing when exposing SP-ZnONPs on A549 cells (Figure 11).

Nitric
Oxide Assay. Cellular nitric oxide level decreased with increasing concentration of SP-ZnONPs. Upon exposing SP-ZnONPs at a concentration of 50, 60, and 70 μg/ mL on the A549 cell line, there is a dose-dependent decrease in nitric oxide (NO) level ( Figure 12). When compared with control cell line, NO level in treated cells was significantly decreased. e decrease NO level was further studied through the complete cellular mechanism of NO generation. Results are expressed as mean and SD. Results were subjected to one-way ANOVA (Tukey multiple comparison test) and showed significant difference between control and treated cells. Treated cells showed high significance compared with control cells (P < 0.0001).

Determination of Lipid Peroxidation Activity.
iobarbituric acid reactive substance (TBARS) assay was performed to quantify the extent of lipid peroxidation induced by the exposure of SP-ZnONPs on to the A549 cell line.
e concentrations of 50, 60, and 70 μg/mL of SP-ZnONPs were chosen for the quantification. ere was a significant dose-dependent increase in the lipid peroxidation levels ( Figure 13). is evaluation revealed that the nanoparticles were quite efficient in elevating the lipid peroxidation. Treated cells show higher significance compared with control cells (P < 0.0001).

Measurement of Lactate Dehydrogenase Activity.
Lactate dehydrogenase activity (LDH) signifies the cell lysis. Upon cell lysis, the enzyme is exposed to the outside of the cell. Upon treating the A549 cancer cell lines with 50, 60, and 70 μg/mL of SP-ZnONPs, it increases lactate dehydrogenase activity. A drastic dose-dependent increase in the LDH activity was evidenced in A549 cell lines after exposing to the SP-ZnONPs (Figure 14). Treated cells show higher significance compared with control cells (P < 0.0001).

Discussion
Lung cancer is one of the leading causes of death among all cancers. A variety of treatment strategies including surgery, chemotherapy, radiation therapy, and targeted therapy have been followed; however, the success rate is low. Greensynthesized nanoparticles are being actively explored as an anticancer drug. Especially, the potential of anticancer activity of ZnONPs has been thoroughly investigated. ZnONPs nanoparticles have been established as an anticancer drug [19][20][21] because of their selective killing efficiency on proliferating cell lines [4,22,23]. Solanum procumbens has been extensively used in folk medicine in South East Asian countries. erefore, we synthesized ZnONPs using Solanum procumbens extract. Further, we evaluated the synthesized SP-ZnONPs as an antilung cancer drug. e absorbance of the sample depends on several factors, such as band gap, oxygen deficiency, surface roughness, and impurity. e UV-Vis absorption spectrum of SP-ZnONPs shows an absorption maximum at 372 nm, which is blue shifted to 365 nm for bulk ZnONPs confirms the generation SP-ZnONPs [24]. e X-ray diffraction pattern of SP-ZnONPs is shown in Figure 2.  [25]. e average crystallite size of the sample was calculated using Debye-Scherrer's formula [26].

Average Crystallite Size D � kλ/β_Dcosθ.
Where D is the size in nanometres, λ is the wavelength of the radiation (1.5406Å for CuKα), k is a constant (0.94), and βD is the peak width at half-maximum in radian along (101) plane and in the Bragg's diffraction angle. e ZnONPs average particle size is 52 nm. To obtain the particle size information, the hydrodynamic diameter of green-synthesized SP-ZnONPs was determined using dynamic light scattering (Figure 3). e size of the SP-ZnONPs was measured at 154 nm; because the NPs were surrounded by water, the DLS particle size was larger than the XRD results. is is referred to as hydrodynamic size. Figure 4 shows the photoluminescence spectra of greensynthesized SP-ZnONPs excited at 325 nm. e emissions were observed at 388, 421, 445, 459, 479, and 523 nm. e peak observed at 388 nm (near band edge), due to the free exciton-exciton collision process's radiative recombination [27]. e electron transition from the surface donor level of the zinc interstitials (Zni) to the top level of the valence band is responsible for the violet emission observed at 421 nm [28]. e three blue emission bands at 445, 459, and 479 nm correspond to the singly ionized Zn vacancies (VZn) [29]. e peak at 523 nm corresponds to the oxygen vacancies (Ov) [30].
SEM image of green-synthesized SP-ZnONPs is shown in Figure 5. From the image, it is clear that the SP-ZnONPs formed a spherical structure with agglomerated nanostructures due to the reduction of surface free energy by increasing their size and decreasing their surface area. e average particle size is found to be 30-60 nm, which is agreed well with the value determined by XRD. e IR spectrum of Solanum procumbens extract and SP-ZnONPs was shown in Figures 6(a) and 6(b), respectively. e broad peak at 3436 cm −1 in both Figures 6(a) and 6(b) confirms the presence of alcohol and phenolic OH groups; it is clearly understood that both phenols and alcohols present in the extract are caped with the nanoparticles. In addition, the peak at 495 cm −1 in the Figure 6(b) confirms the presence of SP-ZnONPs because the peak between 400 and 600 cm −1 regions responsible for stretching frequency of Zn-O bond in ZnONPs [31]. Most importantly, the peaks responsible for different functional groups such as -N-H and -C=O in the extract as shown in Figure 6(a) are completely disappeared in the case of SP-ZnONPs as shown in Figure 6(b). It clearly indicates that the compounds containing both alcoholic and phenolic OH groups in the extract are responsible for the generation of ZnONPs and remaining compounds present in the extract are leaching out while giving repeated washings.
Cytotoxic nature of the synthesized nanoparticles was evaluated by MTT assay (Figure 7). e cell viability was evaluated after treatment with SP-ZnONPs. In both the assays, the nanoparticle concentrations ranging between 5 and 200 μg/mL were used against A549 cell lines. e results of cell viability assay correlated well with the cytotoxic assay ( Figure 8). IC 50 of the SP-ZnONPs was calculated to be 61.28 μg/mL for MTT assay and 60 μg/mL for cell viability assay. e morphological changes during the cell death induced by SP-ZnONPs were evaluated by phase contrast microscopy. It was found that there is a dose-dependent reduction in the cell number; the optimized dose range is between 50 and 70 μg/mL. When compared with control, drastic changes in the cellular morphology were also observed (Figures 9(a)-9(e). e cells were rounded up the sign of detachment from the substrate, which is an evidence for the morphologic hallmarks of apoptosis [32][33][34]. Integrins are involved in cell-matrix interaction through focal adhesion and linked kinases. Induction of apoptosis led to inactivation of focal adhesion [35] and linked kinases [36]. Overall, it could be concluded that the SP-ZnONPs cause cell deaths in the lung cancer cells through the apoptosis. erefore, to confirm the apoptosis, induction AO/EB dual staining was carried out. Acridine orange stain has the propensity to penetrate into the normal and early apoptotic cells where the cell membrane is intact. It gives a fluorescent green colour upon binding to the DNA. On the other hand, ethidium bromide stain can only damage cells and gives orange red colour fluorescence when bound to the DNA [37]. e fluorescent images ( Figure 10) indicate that the SP-ZnONPs induces a dose-dependent effect on lung cancer cells. At lower concentrations, viable and early apoptotic cells were observed with a scanty number of late apoptotic and necrotic cells, whereas at medium dose, the number of viable cells decreased with equal proportion of early and late apoptotic cells. Upon increasing the concentration, the number of apoptotic cells can be visualized with very rare viable cells. Overall, it is clear that SP-ZnONPs are effective in causing cell deaths by inducing apoptosis. Further, mechanism of induction of apoptosis was evaluated through the analysis of ROS because apoptosis is a main cause for the ROS increment. ZnONPs are well known for its efficacy in raising ROS [19]. Cellular ROS is capable of inducing cell cycle arrest, senescence, and subsequently apoptosis in cancer cells. Interestingly, ROS has been demonstrated to suppress metastasis also [38]. In the chemotherapy for cancer, exhausting antioxidant mechanism to elevate ROS through apoptosis is one of the effective strategies being followed [5]. SP-ZnONPs induced a significant increase in ROS through apoptosis in a dose-dependent manner. Even with 50 μg/mL dose of SP-ZnONPs, there was a 1.5-fold increase in ROS, and with 70 μg/mL dose, there was more than 3-fold increase in ROS level ( Figure 11). It is clear that the apoptosis induced by SP-ZnONPs is an origin in the elevation of ROS level. NO is a negative regulator of apoptosis in a number of cell types including lung cancer. Hence, suppression of NO is very important for the activation of Bax through slug, especially in A549 cell lines [39]. In the current experiment, SP-ZnONPs significantly suppresses the NO level in A549 cell line in a dose-dependent manner ( Figure 12). ese results correlate well with the dose-dependent increase in apoptosis by SP-ZnONPs.
Lipid peroxidation is a result of oxidative stress, which leads to breakage of lipids. Ultimately, lipid peroxidation can lead to alterations in the fluidity and permeability of membranes since membranes are made of lipid bilayers and thus can cause loss of cellular integrity [40]. Furthermore, the end products of lipid peroxidation can also induce apoptosis [41]. Results indicate that SP-ZnONPs are effective in inducing lipid peroxidation in a dose-dependent manner ( Figure 13). erefore, it is reasonable to conclude that SP-ZnONPs-mediated lipid peroxidation caused apoptosis in lung cancer cells. e presence of lactate dehydrogenase enzyme (LDH) in assay medium indicates that the cells undergo lysis. Estimation of LDH for the doses 50, 60, and 70 μg/mL of SP-ZnONPs revealed that the nanoparticles increase the LDH to a greater extent in a dose-dependent manner. Approximately 40-fold increase in LDH was seen with 70 μg/mL of SP-ZnONPs treatment. is is a strong proof that the green-synthesized nanoparticles are able to induce cell death in A549 cancer cell lines.
In conclusion, SP-ZnONPs effectively induced apoptosis in A549 lung cancer cell line with the IC 50 value of 61.28 μg/ mL. Further, SP-ZnONPs caused detachment and rounding up of cell lines. Apoptosis induction by the green-synthesized nanoparticles was confirmed by AO/EB dual staining. e apoptosis was mediated by elevated ROS generation, which further caused lipid peroxidation and resulted in induction of apoptosis. erefore, SP-ZnONPs can be used for the treatment of lung cancer. However, further in vivo studies are required to validate the clinical application of the nanoparticles.

Data Availability
e research data used to support the findings of this study are included within the article.

Conflicts of Interest
e authors declare that they have no conflicts of interest.