Abstract
In recent years, the industrial use of ZnO quantum dots (QDs) and nanoparticles (NPs) has risen and there is a high chance of these nanoparticles affecting human health. In this study, different sizes of ZnO-NPs (6–100 nm) were prepared and characterized. The generation of reactive oxygen species (ROS) and its involvement in apoptosis when HepG2 cells were exposed to QDs (6 nm) and NPs of different sizes (15–20, 50, and 100 nm) was also investigated. At a concentration of 25–200 μg/mL, NPs induced dose-dependent cytotoxicity in HepG2 cells. The engineered NPs increased oxidative stress in a dose- and size-dependent manner, as seen by an increase in ROS production, lipid peroxidation, and glutathione reduction. Furthermore, cell-cycle analysis of HepG2 cells treated with different sizes of NPs showed an increase in the apoptotic peak after a 24-h exposure period. Quantitative real-time PCR data showed that the mRNA levels of apoptotic marker genes such as p53, bax, and caspase-3 were upregulated, whereas bcl-2, an anti-apoptotic gene, was downregulated; therefore, apoptosis was mediated through the p53, bax, caspase-3, and bcl-2 pathways, suggesting a possible mechanism by which QDs and NPs of ZnO mediate their toxicity.
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Introduction
The size of nanostructured materials is an important parameter in nanotechnology. Due to the small size of nanoparticles, their physicochemical properties such as volume, surface area, pore diameter, catalytic properties can change [1,2,3,4,5]. To date, various types of nanostructures in the form of quantum (QDs) [6], nanoparticles (NPs) [7], microparticles [8], thin films [9], and nanocomposites (NCs) have been created [10]. These fabricated structures are classified on the basis of their surface geometry such as zero, one, two, or three dimensional [11]. These structures are prepared by various chemical and physical methods, such as plasma-enhanced chemical vapor deposition [12], chemical vapor deposition [13], thermal evaporation [14], pulsed laser deposition [15], metal organic chemical vapor deposition [16], and cyclic feeding chemical vapor deposition [17]. Various physicochemical methods can also be used to prepare nanoparticles, such as template-assisted synthesis [18]; electrochemical [19], sol–gel [20], sonochemical [21], and surfactant-assisted growth methods [22]; hydrothermal synthesis [23]; and solvothermal [24], aqueous, and non-aqueous solution process [25]. The physical approaches are expensive as compared to the chemical methods, but provide nanomaterials in bulk [25]. Due to their small size and enhanced surface area, nanosized materials exhibit enormous fascinating properties, such as piezoelectric effect, high temperature tolerance, enhanced conductivity, and non-linear optical properties [26], which makes them excellent for a wide range of applications in the optoelectronic industry. These materials can be utilized in solar cells, dye-sensitized solar cells, fuel cells, hydrogen production, photocatalysis, adsorption, dye degradation, coatings, corrosion protectors, and semiconductor devices [25, 27,28,29].
Among numerous semiconductor metal oxides, zinc oxide (ZnO) is widely known for its versatile nature and can produce a series of nanostructures [30]. Zinc oxide has electronic properties, biocompatible nature, and can be used in various applications. However, there are limited reports on the use of different sized nanostructures, such as ZnO and TiO2 NPs, their biological activity and efficacy against cancer cells. Few studies have evaluated their toxic effects against human blood cells or have evaluated their effect on the cellular and genetic material and ROS generation [31]. Previously, ZnO-NPs have been prepared by mechano-chemical reaction processes, where the size of the NPs was within 15–40 nm range, and the UV absorbance effects on NPs was checked [32]. The size-controlled ZnO-NPs were employed to examine the toxicity within different cells and their effect on the human immune system was studied [33]. The cytotoxicity was also measured with two spherical shaped zinc oxide NPs in terms of particle size, concentration, and time dependence in normal cells and cancer cell lines from different histological origins [34]. The ZnO particles were prepared in nano and micro-ranges for toxicity studies in human lung epithelial cells (L-132) and human monocytes (THP-1), which were chosen for their ability to clear foreign particles [35]. Three different sizes of ZnO-NPs (30 nm, 80–150 nm, and 2 µm) were used to check the cytotoxic and embryotoxic effects in flounder gill cells and zebrafish embryos [36]. The biological effects of ZnO-NPs were checked on SHSY5Y cells incubated for 24 h with various concentrations of NPs [37]. In another work, the nano and micro sized zinc oxide particles were utilized to check the cell viability, phagocytosis, and cytokine induction in human monocytes, THP-1 cells, which exhibit monocyte like properties and are linked with the adaptive and innate immune responses [38].
Here, we have described the preparation and characterization of different sized NPs. The study was designed to investigate the effect of NPs in liver cancer cells (HepG2) with different sized NPs, from 6 to 100 nm. HepG2 cells were used, because they are a well-established model system to study xenobiotic induced cell death. Different sized NPs were used to induce cell death/apoptosis in cancer cells. The MTT assay was used to check the % of viable and non-viable cells before and after interaction with nanomaterials, whereas apoptosis was measured via the flow cytometry. RT-PCR analysis of apoptotic gene p53, bax, caspase-3, and bcl-2 was also done.
Materials and methods
Synthesis of ZnO nanoparticles ranging from 6 to 100 nm was carried out at different conditions using different precursors. Four different kinds of particles were synthesized.
Synthesis of different sized zinc oxide nanoparticles
Quantum dots (ZnO-QDs) (Size ~ 6 ± 2 nm)
The ZnO-QDs were synthesized using analytical grade chemicals, purchased from Aldrich Chemical Co. Ltd. Zinc acetate dihydrate (Zn(Ac)2·2H2O, 0.3 M), sodium hydroxide (NaOH, 0.3M) and aniline (C6H5NH2, 20 mL) were mixed with 100 mL of methanol (MeOH) and stirred for 30 min. The inital pH of the solution was maintained at 6.87 using a pH meter (Cole Parmer, USA) and it increases up to 12.5 once the NaOH was incorporated. The stirred solution was refluxed in a glass pot at ~ 65 °C for 6 h. The organic impurities were removed from the solution by centrifugation (3000 rpm for 10 min). No precipitate was seen in the refluxing pot before 6 h. After refluxing was complete, a white precipitate was obtained in the refluxing pot. The solution was dried in a petri dish and cooled at 25 °C [39].
Synthesis of ~ 15 ± 20-nm ZnO-NPs
Synthesis of ZnO-NPs, ranging from 15 to 20 nm, was done using Zn(Ac)2·2H2O and octadecylamine (CH3(CH2)17NH2). Briefly, 0.8 M CH3(CH2)17NH2 and 0.3 M Zn(Ac)2·2H2O were dissolved in 100 mL MeOH. The solution was stirred for 30 min on a hot plate equipped with a rotor. Zn(Ac)2·2H2O and octadecylamine were purchased from Aldrich Chemical Corporation. The pH of the solution was measured to be 12.3. After complete dissolution of the chemicals, the solution was transferred to a three-necked refluxing pot and refluxed at ~ 65 °C for 6 h. A white-colored precipitate was observed at the bottom of refluxing pot after 6 h. Solution temperature was monitored and controlled using a temperature controller. Thereafter, the white powdery precipitate was washed with MeOH several times. The NPs obtained were air dried at room temperature and their structural and chemical properties were characterized, as described previously [39].
Synthesis of 45 ± 5-nm ZnO-NPs
Bigger sized NPs were obtained by the reacting Zn(AC)2·2H2O and thiourea (NH2CSNH2) via solution process as previous [5, 20]. Briefly, 0.3 M Zn(AC)2·2H2O and 2 M NH2CSNH2 were dissolved in 100 mL deionized water and stirred for 30 min. The solution was then transferred to a glass pot and refluxed at 90 °C for 12 h. Before transferring the solution to the flask, the pH was measured at 12.6. After refluxing, the white aqueous solution was washed with MeOH several times to remove ionic impurities and then dried at 25 °C for further analysis. The dried powder was annealed in ambient air at 500 °C for 1 h at 5 °C/min. Thereafter, the morphological and chemical properties of NPs were characterized, as described previously [5, 20].
Synthesis of ~ 100-nm ZnO-NPs via the using solution method
The synthesis of ZnO-NPs (> 50 nm) was carried out using Zn(AC)2.2H2O and p-xylene (C6H4(CH3)2), purchased from Aldrich Chemical Co. Ltd. Briefly, 0.3 M Zn(Ac)2.2H2O and 20 mL C6H4(CH3)2 were mixed together in MeOH and stirred for 30 min. The pH of the solution was measured at 12.4. The stirred solution was transferred to the refluxing pot and refluxed at ~ 65 °C for 6 h followed by cooling at room temperature. The impurities, such as by-products of organic chemicals, were removed from the solution via centrifugation (3000 rpm for 5 min). The dried sample was annealed in ambient air at 700 °C for 1 h at 5 °C/min. Thereafter, the morphological and chemical properties of the sample were characterized [5, 20].
Characterization of different sized QDs and NPs prepared via solution process
The powders, with diverse sized particles, were morphologically and chemically characterized. Morphological evaluation of the white powder was made by field emission scanning electron microscopy (FESEM) and transmission electron microscopy (TEM). For FESEM, the white powders were uniformly sprayed on carbon tape and coated with a thin layer of osmium oxide (OsO4) for 5 s. For TEM measurement, powder samples were sonicated in ethanol for 10 min. To this solution, copper grid was inserted for 2–3 s and dried at room temperature. The crystallinity and phase of the white powders were characterized with an X-ray powder diffractometer (XRD) with CuKα radiation (λ = 1.54178 Å) in the range of 20°–65° at 6°/min scanning speed.
Cell culture and their treatment of ZnO-NPs
Human liver HepG2 cells were purchased from ATCC, USA. Cells were cultured in DMEM/F-12 medium with 10% FBS and 100 U/mL penicillin–streptomycin in 5% CO2 at 37 °C. The cells were harvested at 85% confluence using 0.25% trypsin and sub-cultured as required for the experiments. Cells were allowed to attach to the surface before treatment for 24 h. ZnO-QDs and NPs were suspended in culture medium and diluted to suitable concentrations. The dilutions of different sized NPs were then sonicated to avoid their agglomeration prior to their being applied to the cells.
MTT assay
Percent viability of HepG2 cells was assessed by exposing them to different concentrations of ZnO-NPs of various sizes, using the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay, as described previously [40]. The assay evaluated cell viability by quantifying viable cells that reduced MTT to form a blue formazan product. In brief, 1 × 104 cells/well were incubated with 0, 1, 2, 5, 10, 25, 50, and 100 µg/mL QDs and NPs for 24 h. Subsequently, the medium in each well was exchanged with fresh medium, containing MTT at a final concentration of 10%, and incubated for 3 h at 37 °C for the purple color to develop. The formazan product so formed was dissolved in acidified isopropanol. The plate was centrifuged for 5 min at 2500 rpm for the QDs and NPs to settle at the bottom. Thereafter, 100 µL supernatant was taken from each well, transferred to fresh 96-well plate, and absorbance was quantified at 570 nm using a microplate reader (Synergy-HT, BioTek). Percent viability of HepG2 cells was calculated using the formula,
NRU assay
Neutral red uptake (NRU) assay was done as described by Borenfreund and Puerner (1984) [41], with some modifications [42]. In brief, 1 × 104 cells/well were seeded in 96-well plates, and incubated with 0, 1, 2, 5, 10, 25, 50, and 100 µg/mL QDs and NPs for 24 h. Thereafter, the supernatant was removed, the cells were washed with PBS, and incubated for 3 h in medium containing 50 µg/mL neutral red. The solution was removed promptly and the cells were washed with medium containing 0.5% formaldehyde and 1% calcium chloride. Subsequently, the cells were incubated for 20 min at 37 °C in a solution of 1% acetic acid and 50% EtOH to remove the dye. Finally, absorbance was measured at 540 nm using a microplate reader (Synergy-HT, BioTek).
ROS measurements
For the determination of ROS, HepG2 cells were exposed to 25 µg/mL QDs and NPs for approximately 24 h. Intracellular ROS production was measured using 2, 7-dichloro fluorescin diacetate (DCFH-DA) [43, 44], which can passively cross the cell membrane and react with ROS to produce a colored compound called dichlorofluorescein (DCF). Briefly, a 10 mM DCFH-DA stock solution was diluted in the culture medium, without other additives, to prepare a 100 µM working medium. After exposure to QDs and NPs, the cells were washed twice with HBS (HEPES buffered saline), and incubated with medium containing 100 µM DCFH-DA at 37 °C for 30 min. Intercellular fluorescence was analyzed using a fluorescence microscope (Olympus CKX 41; Olympus) at 20X magnification.
Measurement of mitochondrial membrane potential (MMP)
MMP was measured using the procedure described by Zhang et al. [45]. Briefly, HepG2 cells were exposed to 25 µg/mL QDs and NPs for 24 h. Subsequently, the cells were washed twice with PBS and treated with 10 μg/mL Rh 123, a fluorescent dye, for 1 h at 37 °C in the dark. The fluorescence of Rh 123 was measured using a fluorescence microscope (OLYMPUS CKX 41).
Glutathione level
For GSH measurement, HepG2 cells were cultured in 25 cm2 culture flasks. The cells were exposed to 10, 25, and 50 μg/mL of (~ 6 ± 2 nm), (~ 15–20 nm), (~ 45–50 nm), and (~ 100 nm) Zn NPs for 24 h. Thereafter, the cells were lysed in cell lysis buffer [1 × 20 mM Tris–HCl (pH 7.5), 150 mM NaCl, 2.5 mM sodium pyrophosphate, 1 mM Na2EDTA, and 1% Triton]. The supernatant, obtained after centrifugation at 15,000 × g for 10 min at 4 ºC, was kept on ice until assayed following Ellman’s method [46]. Briefly, a mixture of 0.1 mL of cell extract (supernatant) and 0.9 mL of 5% TCA was centrifuged (2300 × g for 15 min at 4 °C). Thereafter, 0.5 mL of supernatant was added to 1.5 mL of 0.01% 5, 5-dithio-bis-(2-nitrobenzoic acid) (DTNB) and measured spectrophometrically at 412 nm.
Lipid peroxidation (LPO)
LPO was assayed by the method of Ohkawa et al. (1979) [47]. HepG2 cells were exposed to 10, 25, and 50 μg/mL of (~ 6 ± 2 nm), (~ 15–20 nm), (~ 45–50 nm), and (~ 100 nm) ZnO-NPs for 24 h. Briefly, 0.1 mL of cell extract and 1.9 mL of 0.1 M sodium phosphate buffer (pH 7.4) were incubated at 37 °C for 1 h. After incubation, cells were precipitated with 5% TCA and then centrifuged to 2300 × g for 15 min, to collect the supernatant. After incubation, 1.0 mL of 1% TBA was added to the supernatant and put in hot water for 15 min. After cooling, the absorbance was taken at 532 nm.
Analysis of cell-cycle progression by flow cytometry
Cell-cycle analysis was performed by a method described by Saquib et al. [48]. The cells were exposed to 50 μg/mL of ~ 6 ± 2 nm, ~ 15–20 nm, ~ 45–50 nm, and ~ 100 nm ZnO-NPs for 24 h and centrifuged at 1000 rpm for 4 min. The cells were fixed with 500 µL of 70% ice-cold ethanol, incubated at 4 °C for 1 h, washed with PBS, and stained using 500 µL of PBS, containing 50 µg of propidium iodide (PI)/mL, 0.1% Triton X-100, and 0.5 mg/mL RNAase. PI signal was measured by flow cytometry with a Beckman Coulter flow cytometer (Coulter Epics XL/Xl-MCL, USA) through a FL 3 filter (585 nm) and 10,000 events were acquired. The data were evaluated using Coulter Epics XL/ XL-MCL, System II Software, Version 3.0.
Quantitative real-time PCR analysis of apoptotic markers
HepG2 cells were cultured in 6-well plates and treated with ZnO QDs and NPs at a concentration of 50 µg/mL for 24 h. Total RNA was extracted both from treated and untreated cells by RNeasy mini Kit (Qiagen), as per the manufacturer’s instructions. RNA concentration was evaluated using Nanodrop 8000 spectrophotometer (Thermo-Scientific). cDNA was prepared from 1 µg of total RNA using M-MLV kit (Promega), as per the kit’s protocol. Real-time quantitative PCR (RT-PCR) was done using Roche® LightCycler®480 (96-well block) (IN, USA), following the recommended cycling program. For the reaction mixture, 2 μL of cDNA was taken in a final volume of 20 µL of reaction mix. The RT-PCR program included a denaturation step at 95 °C for 10 min, followed by 40 cycles of denaturation at 95 °C for 15 s, annealing at 60 °C for 20 s, and elongation at 72 °C for 20 s. Expressed genes were normalized to GAPDH, the housekeeping control gene. All experiments were performed in triplicate and data were expressed as the mean of at least three experiments.
Results
Morphological analysis by FESEM
Morphological changes in the prepared QDs and NPs can be seen in the FESEM images (Fig. 1). Figure 1a, b shows FESEM images at lower and higher magnification, respectively, of the synthesized QDs and NPs, which confirmed that the synthesized ZnO products were of different sizes. The less magnified (Fig. 1a) image clearly demonstrated that the grown structures were high in density. Most QDs exhibited spherical shapes with an average diameter range of 6 ± 2 nm. Additionally, some QDs were ellipsoidal, as seen in the FESEM micrograph (Fig. 1b). The size of the NPs increased under different processing conditions, as described in Materials and methods. The NPs were elongated and triangular (Fig. 1c, d). The average size of each NP was in the range of ~ 15–20 nm (Fig. 1d). Upon annealing, NPs form aggregates or crystals. At high-temperature annealing (at 500 °C in air for 1 h), the powders resulted in random shapes of NPs, such as spherical, triangular, or circular, approximately 45–50 nm in size (Fig. 1e, f). A higher annealing temperature (˂ 500 °C) resulted in agglomeration of particles (~ 90–100 nm in size) to form bigger NPs, as shown in Fig. 1g, h. At higher temperature, small NPs merged with each other and in between other particles [19, 20, 25].
Morphological analysis by TEM
Further morphological investigation of QDs and NPs was performed with TEM. Figure 2a–d shows TEM images of particles grown to different sizes. The shapes were nearly spherical and were similar to those seen with FESEM (Fig. 1). As seen in the TEM image (Fig. 2a), the synthesized NPs were spherical and ellipsoidal in shape. The size of each QD was in the range of ~ 6 ± 2 nm, which was consistent with the FESEM data (Fig. 1b). In the second case, the size of NPs reached up to ~ 20 nm (Fig. 2b) and had similar morphology as depicted in the previous results (Fig. 1c, d). In the third case, the size of the NPs was seen to be up to ~ 45–50 nm (Fig. 2c) (at 500 °C for 1 h in air under ambient conditions) and the results were consistent with those from FESEM (Fig. 1e, g). At higher temperatures (above 500 °C for 1 h), the NPs aggregated with each other and formed bigger sized structures (~ 90–100 nm) (Fig. 2d) [7, 19, 20, 25].
Crystallinity, phase and size examination (XRD results)
Figure S1 presents the X-ray diffraction patterns (XRD) of synthesized NPs at different processing conditions. The main indexed peaks <1010> , <0002> , <10 11> clearly showed the crystalline property of the nanoproducts. All indexed peaks in the spectrum obtained were well matched with bulk ZnO (JCPDS Card No. 36-1451), which further confirmed that the prepared powders were crystalline in nature and had wurtzite phase. There was no other peak related to impurities in the spectrum within the detection limit of the XRD, which again confirmed that the synthesized powders were pure ZnO [7, 19, 20, 25].
Cytotoxicity results
MTT and NRU results
The results of cytotoxicity assessment have been summarized in Figs. 3 and 4. HepG2 cells were treated with ZnO-NPs in concentrations ranging from 1–100 μg/mL for 24 h. The cytotoxicity of ZnO-NPs was observed by MTT and NRU assays. These assays showed that ZnO-NPs did not produce significant cytotoxicity at concentrations of 10 μg/mL and lower. However, at concentrations of 25 μg/mL and above, ZnO-NPs induced cytotoxicity in a concentration-dependent manner, resulting in the reduction of HepG2 cell viability. Furthermore, ZnO-NPs, approximately 15–20 nm in size, were most cytotoxic, followed by ZnO-NPs (~ 6 ± 2 nm) and ZnO-NPs (~ 45–50 nm). ZnO-NPs (~ 100 nm) were found to be least cytotoxic to HepG2 cells. Cell viability, using MTT assay, was recorded at 5%, 6%, and 54% in ZnO-NPs (~ 15–20 nm); 12%, 16%, and 90% in ZnO-NPs (~ 45–50 nm); 9%, 11%, and 20% in ZnO-QDs (~ 6 ± 2 nm); and 50%, 63%, and 63% at 25, 50, and 100 mg/mL ZnO concentration, respectively (Fig. 3). As shown in Fig. 4, a similar trend of reduction in cell viability was recorded by the NRU assay. The cell viability by NRU assay was recorded as 12%, 15%, and 19% in ZnO-NPs (~ 15–20 nm); 20%, 21%, and 91% in ZnO-NPs (~ 45–50 nm); 29%, 32%, and 36% in ZnO-NPs (~ 6 ± 2 nm); and 49%, 68%, and 74% at 25, 50, and 100 μg/mL ZnO concentration, respectively (Fig. 4). The IC50 values obtained for (~ 6 ± 2 nm), (~ 15–20 nm), (~ 45–50 nm), and (~ 100 nm) ZnO-NPs were 15.8 μg/mL, 27.5 μg/mL, 30.08 μg/mL, and 101.2 μg/mL, respectively, by the MTT assay.
ZnO-NPs induced oxidative stress
ROS generation and GSH and LPO levels were examined to show the potential of ZnO-NPs to increase oxidative stress in HepG2 cells. The results revealed that HepG2 cells exposed to ZnO-NPs, had higher intracellular ROS generation (Fig. S2). Fluorescence microscopy results showed that ~ 6 ± 2 nm ZnO-QDs expressed more fluorescence intensity followed by ~ 15–20 nm, ~ 45–50 nm, and ~ 100 nm ZnO-NPs as compared to the untreated control (Fig. S2 graph). As shown in Fig. 5, the GSH level was considerably lower in HepG2 exposed to ZnO-NPs, however, the LPO level was higher (125, 148, and 174% was found in 6, 119, and 139 nm; 165% in 15–20, 110, and 122 nm; 147% in 50 nm and 100, 128, and 140% were found in 100 nm sized NPs, as compared with the control, which was 100% at different concentrations of NPs (10, 25, and 50 µg/mL), in HepG2 cells exposed to ZnO-NPs for 24 h (Fig. 6).
ZnO-NPs induced change in MMP level
MMP levels in HepG2 cells exposed to ZnO-NPs for 24 h at 25 μg/mL are presented in Fig. S3. The decrease in MMP levels was recorded in terms of fluorescence intensity of the mitochondria specific dye Rh 123. As shown in Fig. S3, ZnO-NPs decreased the fluorescence intensity of Rh 123. This reduction in fluorescence intensity in HepG2 cells treated with ZnO-NPs indicated a significant decrease in MMP levels with low to high range of NPs (54, 45, 36, and 23) compared to the control (100).
Effect of different sized ZnO-NPs on cell-cycle progression
Analysis of the effects of varying sizes of zinc oxide NPs on HepG2 cells indicated an increase in the apoptotic sub-G1 peak after 24 h of exposure (Fig. 7). With an average of 5.9% back ground level of apoptotic peaks in HepG2 control, ZnO-QDs (< 10 nm) at lower doses of 10 and 25 µg/mL did not show any changes in the normal cell cycle. At the higher concentration of 50 µg/mL, a significant increase of 24.4% in the sub-G1 apoptotic phase was recorded (Fig. 7). HepG2 cells exposed to low doses of ZnO-NPs (< 20 nm) exhibited a typical pattern of G2/M arrest. In comparison to 27.4% of the control cells in G2/M phase, 10 and 25 µg/mL of ZnO-NPs (< 20 nm) treatment showed 42.4% and 33.1% cells in G2/M phase, respectively. At the highest concentration of 50 µg/mL, ZnO-NPs (< 20 nm) exhibited transition of G2/M arrested cells (16.5%) in the apoptotic phase (16.0%) (Fig. 7). A similar pattern of G2/M arrest, along with an increase in apoptosis, was observed in ZnO-NPs-50 (< 50 nm)-treated HepG2 cells. Lower doses of 10 and 25 µg/mL exhibited 34.4% and 18.1% of cells arrested in G2/M phase, respectively, vis-à-vis untreated control, which showed only 23.7% cells, in G2/M phase. Nonetheless, bigger ZnO particles (~ 45–50 nm), at the highest concentration of 50 µg/mL, exhibited a substantial increase in apoptotic response with 27.2% cells in sub-G1 phase, as compared to 8.8% of apoptotic cells in the untreated control group (Fig. 7). In comparison to treatment with larger sized ZnO nanoparticles, such as 100 nm, ~ 45–50 nm, and 15 ± 20 nm, HepG2 exposed to ZnO particles of 6 ± 2 nm, exhibited stronger apoptotic response during cell-cycle progression. Lower dose (10 and 25 µg/mL) exposure of HepG2 cells exhibited 16.4% and 22.8% increase in apoptotic sub-G1 peak, respectively. At the highest concentration of 50 µg/mL, nearly 44% of cells underwent apoptosis (Fig. 7).
Analysis of mRNA level of apoptotic genes using quantitative real-time PCR
HepG2 cells were exposed to different sizes of ZnO-NPs for 24 h at a concentration of 50 μg/mL, and quantitative real-time PCR was performed to evaluate the mRNA level of apoptotic genes (p53, bax, casp3, and bcl-2). Different sized NPs significantly altered the regulation of apoptotic genes in HepG2 cells (p < 0.05 for each gene) (Fig. 8). The mRNA levels of the cell-cycle checkpoint or tumor suppressor gene p53 (Fig. 8) and the pro-apoptotic gene bax (Fig. 8) were upregulated. We also detected higher expression of the caspase-3(Fig. 8) gene in NP-treated cells. The expression of bcl-2 (Fig. 8), an anti-apoptotic gene, was downregulated in cells treated with different sized ZnO-NPs. Thus, ZnO-NPs of different sizes induced expression of apoptotic genes.
Discussion
QDs and NPs of ZnO have wide industrial and biomedical applications, such as in cancer, drug delivery, DNA damage, and cytotoxicity, due to their high surface area and catalytic properties [7, 19, 20, 25]. In this study, QDs and different sized NPs were prepared by soft chemical solution and annealing process using zinc acetate dihydrate with different reducing salts, such as octadecylamine and thiourea, at different processing parameters. The NP solutions were calibrated with acid (HCl) and base (NaOH) at desired concentrations [7, 19, 20, 25]. The QDs and NPs were characterized in terms of their crystalline and morphological properties with sophisticated instruments. Techniques such as XRD, FESEM, and TEM were used to check the crystallinity of the synthesized QDs and NPs. The FESEM and TEM results showed that the prepared nanostructures had diverse shapes, with a nearly smooth surface and an average diameter of 6–100 nm, for both QDs and NPs. High-resolution TEM (HR-TEM) confirmed that the structures had lattice spacing (~ 0.256 nm), were crystalline, and equal to pure wurtzite phase ZnO [5]. The nanostructures of ZnO were optically active materials, which exhibited similar band gap to the commercial zinc oxide powder (3.37 eV) [5]. In addition to the detailed characterization of ZnO-NPs, the aim of this study was to also investigate the cytotoxic responses of different sized NPs on liver cancer (HepG2) cells. The MTT and NRU assays were used to check the cytotoxicity of different sized NPs on the cells after a 24-h incubation period. HepG2 cells exposed to 1–100 μg/mL doses of ZnO-NPs significantly decreased cell viability in a concentration-dependent manner. The results are in accordance with those published previously on cytotoxic activity of NPs, within the same range [49]. Cytotoxicity of these NPs on cancer cells is due to their morphological organization, and their characteristic differences and functions are responsible for cell death [50]. In addition to assessing the cytotoxicity of HepG2 cells caused by NPs and investigating its mechanism, we also evaluated ROS generation and mitochondrial membrane potential (MMP), which played a key role in the cytotoxicity of HepG2 exposed to ZnO-NPs for 24 h. ROS can disturb cellular function by acting directly on DNA, protein, and lipids, destroying their structure and leading to cell death [51]. In the present study, we showed that NPs induced ROS damage in a concentration-dependent manner in HepG2 cells. Our results are in agreement with those reported previously, where various types of NPs have been shown to induce ROS generation, oxidative stress, and cellular cytotoxicity [51,52,53]. Furthermore, we checked MMP levels in HepG2 cells exposed to differently shaped NPs, and observed that the NPs were responsible in decreasing the level of MMP, in terms of reduction in fluorescence intensity of Rh 123. The mitochondria is directly involved in apoptosis and a reduction in MMPs, which can trigger the release of apoptogenic factors from the mitochondria into the cytosol, leading to cell death [54, 55]. Thus, cell death was induced with interaction/exposure of different sized NPs resulting in an increase in ROS generation and a decrease in MMPs, when treated with ZnO-NPs.
To evaluate the size-dependent toxicity of ZnO-NPs, we studied cell death in HepG2 cells. A comparative analysis suggested that smaller sized ZnO particles (ZnO, ~ 6 ± 2 nm) directly induced apoptosis in HepG2 at the higher concentration of 50 µg/mL. Although ZnO particles of size ~ 15–20 and ~ 45–50 nm also induced apoptosis at a higher concentration of 50 µg/mL, a strong connection with G2/M arrest was also revealed, indicating detrimental effects on DNA and cellular repair machinery. In contrast, we observed a low dose-dependent augmentation of apoptosis in HepG2 cells, treated with smaller size QDs (ZnO, ~ 6 ± 2 nm). The appearance of sub-G1 peak in cell-cycle analysis at increasing concentrations of ZnO-NPs suggested the possible involvement of early and late apoptotic/necrotic pathway genes, which might be triggered by alteration in mitochondrial and lysosomal functions [56, 57]. Moreover, HepG2 cells exhibited concentration-dependent G2/M arrest with ZnO-NPs-20, ZnO-NPs-50, and ZnO-NPs-100, suggesting heavy DNA damage and failure of DNA repair machinery. Cellular DNA repair mechanisms are highly conserved [58], and extensive DNA damage may lead to cell-cycle arrest and cell death [59, 60]. Overall, our flow cytometry data clearly exhibited a size-based hierarchy of toxicity, where ZnO 100 > ZnO 50 > ZnO 20 > ZnO 6. Based on the physical (XRD, SEM, and TEM) and biological results (MTT and NRU assay, MMP levels, RT-PCR, and flow cytometry), we presented a schematic detail of the interaction of QDs/NPs with cells, production of ROS, and cells’ death caused by nanostructures in a dose-dependent manner (Fig. 9).
Conclusion
In summary, we successfully synthesized different sized nanoparticles, such as QDs and NPs, using various chemical approaches under different conditions. The results from XRD showed that synthesized ZnO-NPs were pure and highly crystalline in character. The morphological investigations revealed that the prepared structures retained a wurtzite hexagonal phase. In this context, the obtained FESEM images showed sequential data of QDs and NPs from 6 to 100 nm in spherical shape and was consistent with TEM observations. To characterize the prepared materials, different sized NPs were incubated with liver cancer cells (HEPG2). The viability of cells was measured via the MTT and NRU assays, which clearly showed that the small nanoparticles (QDs) were more potent as compared to the bigger sized NPs. The results showed that ~ 15–20 nm ZnO-NPs had high cytotoxicity, followed by ~ 6 ± 2 nm NPs, and ~ 45–50 nm NPs. Moreover, the larger NPs (~ 100 nm) were found to be less cytotoxic to HepG2 cells, which may be due to the settling of high-density NPs at the bottom of the culture medium, resulting in their reacting slowly with cancer cells. Similar observations were made with the NRU data, which showed that the reduction in cell viability was affected by the size of the NPs. Smaller particles could enter the cells easily, owing to low density, and damage intracellular organelles, whereas larger particles, with higher density, exhibited lower reactivity. Thus, cell death was influenced by the concentration and size of ZnO-NPs. In this context, ROS production in cells was examined and smaller (6 nm) particles were shown to express a higher intensity (166) in terms of % change in green fluorescence of DCF, as compared to particles of other sizes (152, 143, and 112) and untreated control (100). Additionally, the level of the antioxidant GSH was also considerably lower in HepG2 cells, incubated with different sized NPs—84, 65, and 48% was found in 6 nm; 88, 69, and 54% in 15–20 nm; 92, 74, and 60% in 50 nm and 98, 79, and 65% in 100 nm sized NPs, while the lipid peroxidation level was found to increase (125, 148, and 174% for 6 nm; 119, 139, and 165% for 15–20 nm; 110, 122, and 147% for 50 nm; and 100, 128, and 140% for 100 nm sized NPs, as compared to 100% for control, with different concentration of NPs) in HepG2 cells exposed to ZnO-NPs for 24 h. The reduction in MMP level in cancer cells with NPs again showed the significance of nanostructures. In addition, flow cytometry results showed that at the highest concentration of 50 µg/mL, almost 44% of cells had undergone apoptosis.
Several approaches, such as chemotherapy and radiotherapy, have been used for cancer treatment, but the results have been unsatisfactory. To date, the surgical procedure is very costly and tedious for the patients and the recovery is painful and time consuming. Extensive work is still needed to establish a successful therapy that might be able to cure cancer efficiently, effectively, and economically. Recent advances in nanotechnology have contributed in various areas of science and technology in cost-effective ways. The biological application of nanostructured materials could provide significant improvement to the existing technologies with no harmful side-effects due to their biocompatibility. Moreover, the small dimensions of NPs enable them to be delivered directly and quickly to cells and proteins as compared to other available drugs.
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The authors are grateful to the Deanship of Scientific Research, King Saud University for funding through Vice Deanship of Scientific Research Chairs.
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Ahmad, J., Wahab, R., Siddiqui, M.A. et al. Cytotoxicity and cell death induced by engineered nanostructures (quantum dots and nanoparticles) in human cell lines. J Biol Inorg Chem 25, 325–338 (2020). https://doi.org/10.1007/s00775-020-01764-5
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DOI: https://doi.org/10.1007/s00775-020-01764-5