Iron oxide nanoparticles (IONPs) are usually composed of magnetite (Fe3O4) and maghemite (γ-Fe2O3). They are highly adsorptive due to small size and large surface area-to-volume ratio and have magnetic properties, which make them useful in numerous applications such as biomedicine, environmental remediation, magnetic storage and recording media, catalysis, and magnetic fluids. They can be synthesised using various methods, including co-precipitation, thermal decomposition, sol-gel synthesis, and microemulsion techniques, which can tune IONP properties to specific application by changing their size, shape, surface chemistry, and crystalline structure during synthesis. Although they are characterised by low toxicity and cost, they may still be toxic and entail environmental risks, especially with biomedical and environmental applications (1,2,3,4,5,6,7,8,9).
Such concerns are well grounded due to their widespread use and potential release into the environment. IONPs can easily reach air, water, and soil thanks to small size and high surface area-to-volume ratio, which enhance their mobility and persistence in the environment, leading to potential long-term exposure and accumulation in various environmental compartments. One of the key environmental hazards associated with IONPs is their toxicity to aquatic organisms, including fish, algae, and other aquatic life, with adverse effects including impaired growth, reproduction, and survival of organisms exposed to high concentrations. Besides, they have the potential to bioaccumulate in aquatic organisms through ingestion or absorption and to biomagnify, which means that IONP concentrations increase as they move up the food chain, posing higher risks to higher trophic levels, including humans (4, 10,11,12,13,14,15). Moreover, IONPs may interact with other pollutants or environmental stressors, leading to synergistic or antagonistic effects on ecosystems (10, 16,17,18).
The profound effect of IONPs on haematology, ion regulation, and gill Na/K ATPase activity has been demonstrated in the Indian major carp (
Fish tissues contain a large amount of polyunsaturated fatty acids, which are highly vulnerable to oxidative stress, followed by tissue damage. Oxidative balance in cells or tissues is maintained by a well-equipped prooxidant/antioxidant defence system that scavenges free radicals, yet oxidative stress varies between tissues and may affect them differently.
Despite considerable research of IONP toxicity in fish, there are still knowledge gaps concerning their long-term adverse effects. Therefore, one aim of this study was to investigate the effects of IONPs on antioxidant defence and susceptibility to oxidative stress in the gill, liver, and brain tissues, and whether the nanoparticles get accumulated inside these tissues of the juvenile Mozambique tilapia (
For this study we used the juvenile Mozambique tilapia (
Optimal physico-chemical characteristics of the tap water were maintained and monitored in line with the standard methods published by the American Public Health Association (APHA) (24) and the OECD guideline on acidity and alkalinity (25) as follows: temperature 28±2 °C, pH 7.0±0.5, dissolved oxygen 8.6±0.6 mg/L, water hardness 48 mg/L calcium carbonate, total organic carbon 0.04 mg/L, non-ionised ammonia 0.01 mg/L, nitrate 10 mg/L, chlorine 4 mg/L, metallic impurities <1 mg/L, and chemical oxygen demand 3 mg/L. Water analyses were done to ensure that water did not affect the experimental outcomes.
Preparation and characterisation of IONPs used in this study has been described in detail in our previous publications (26, 27). Briefly, IONPs (Fe3O4-NPs; Cat. No. 637106) were obtained from Sigma (Darmstadt, Germany). X-ray diffraction (XRD; Rigaku Miniflex, Tokyo, Japan) and transmission electron microscopy (TEM; Jeol/JEM, Tokyo, Japan) were performed to confirm the size and purity of IONPs. IONPs were suspended in double-distilled water and sonicated in an ultrasonic bath (GT Sonic, Guangdong, China) at a frequency of 100 kHz for 30 min to ensure uniformity. All the other chemicals used were of analytical grade and purchased from Himedia (Thane, India).
The test concentration was selected according to IONP dispersion, as mentioned in our previous publication (27). Following the acclimatisation phase, 160 fish were randomly distributed into eight 40-litre glass tanks (30 cm width, 60 cm length, and 30 cm depth), each holding 20 fish. The control group was not exposed to IONPs. Treatment groups were exposed to IONPs at 15 mg/L for 1, 3, 4, 15, 30, and 60 days (IONP1, 3, 4, 15, 30, and 60, respectively). The depuration group was first exposed to IONPs (15 mg/L) for 60 days, and then followed up in IONP-free water for another 60 days.
IONP tissue accumulation was analysed in fish groups treated for four days (IONP4), 60 days (IONP60), and in the 60-day depuration group using a method described by Arslan et al. (28) with slight modifications. Fish from each group were captured with a small dip net to avoid additional stress, euthanised, and dissected. Gill, liver, and brain were excised and rinsed with cold saline before weighing. Wet tissue samples were weighed and digested with a mixture of concentrated nitric and hydrochloric acid (3:1) at 200 °C for 1 h, and the digested material was evaporated to remove any contaminants or residues that might interfere with analytical measurements. The remaining tissue was diluted with deionised water to a known volume. Total iron content, consisting of both iron nanoparticles and any other forms of iron within the samples, was quantified with inductively coupled plasma mass spectrometry (ICP-MS; Thermo Fisher, Waltham, MA, USA). The IONP content in total iron concentration was estimated based on the known molar mass of Fe3O4 and atomic mass, as follows:
This conversion allowed us to determine the number of nanoparticles corresponding to the measured mass, which was used to calculate the bioaccumulation factor (BAF), expressed as micrograms per gram of wet tissue weight.
At the end of every treatment, fish were captured as described above, weighed, euthanised, and dissected to remove the gill, liver, and brain. The tissues were then rinsed with cold saline and weighed. The hepatosomatic index (HSI) of the fish was calculated using the following equation:
Tissue homogenates (1 % w/v) were prepared separately in normal saline on ice using a motor-driven tissue homogeniser (Remi, Mumbai, India) and the homogenates centrifuged at 800
SOD activity was determined as described by Marklund and Marklund (30). The assay mixture contained tris-hydrochloric acid buffer (50 mmol/L, pH 7.6) consisting of 1 mmol/L EDTA, 0.2 mmol/L pyrogallol, and 100 µL of enzyme source. The increase in absorbance was measured at 420 nm against an enzyme-free blank at 10-second intervals over 3 min using an ultraviolet (UV)-visible spectrophotometer (Shimadzu, Kyoto, Japan). Enzyme activity is expressed as nmol of oxidised pyrogallol per min per mg of protein.
CAT activity was determined using the method described by Claiborne (31). A total mixture of 3 mL was composed of phosphate buffer (50 mmol/L, pH 7.0), hydrogen peroxide (19 mmol/L), and 50 µL of enzyme source. The decrease in absorbance was measured at 240 nm against an enzyme-free blank at 10-second intervals over 3 min using a UV-visible spectrophotometer (Shimadzu, Kyoto, Japan). Enzyme activity was expressed as mol of hydrogen peroxide consumed per min per mg of protein.
The activity of GR was assayed as described by Carlberg and Mannervik (32). The assay mixture comprised phosphate buffer (100 mmol/L, pH 7.6), NADPH (0.2 µmol/L), oxidised glutathione (2 mmol/L), EDTA (0.01 mol/L), and the enzyme source. The reduction of NADPH was monitored by measuring the decrease in absorbance at 340 nm against an enzyme-free blank at 10-second intervals over 3 min using a UV-visible spectrophotometer (Shimadzu). Enzyme activity is expressed as nmol of oxidised NADPH per min per mg of protein.
The activity of GPx was determined with the method described by Mohandas et al. (33) utilising hydrogen peroxide and NADPH as substrates. The assay mixture comprised phosphate buffer (100 mmol/L, pH 7.6), EDTA (0.01 mol/L), sodium azide, GR, reduced glutathione, and NADPH (0.2 µmol/L). Enzyme assay was added and NADPH reduction monitored by measuring the decrease in its absorbance at 340 nm against an enzyme-free blank at 10-second intervals over 3 min using a UV-visible spectrophotometer (Shimadzu). Enzyme activity is expressed as nmol of oxidised NADPH per min per mg of protein.
The levels of hydrogen peroxide were assessed following the method described by Pick and Keisari (34). The assay is based on the H2O2-mediated and horseradish peroxidase-dependent oxidation of phenol red to a product. The incubation mixture comprised phosphate buffer (50 mmol/L, pH 7.6), horseradish peroxidase (8.5 units), phenol red (0.28 nmol/L), dextrose (5.5 nmol/L), and enzyme source (100 µL). The reaction was carried out at room temperature for 30 min, after which it was terminated by adding 10 eq/L sodium hydroxide. The absorbance was measured at 610 nm against the blank. A standard curve was prepared using known concentrations of H2O2, and the results are expressed as nmol of generated hydrogen peroxide per mg of protein.
LPO was measured using thiobarbituric acid as outlined by Ohkawa et al. (35). A working solution was prepared by combining 15 % w/v trichloroacetic acid, 0.37 % 2-thiobarbituric acid, and 0.25 eq/L hydrochloric acid in a 1:1:1 ratio. The enzyme source was added to the working solution at a ratio of 1:2 and incubated in a boiling water bath for 10 min. Followed the measurement of absorbance at 535 nm against the blank. Malondialdehyde (MDA) solution served as the standard, and the results are expressed as nmol of MDA per mg of protein.
The activity of ALP in gill and liver tissues was determined following the method described by Bessey et al. (36). Pre-incubation involved
The activity of AChE in the brain tissue was determined as described by Ellman et al. (37) by monitoring the increase in yellow colour resulting from the reaction between thiocholine and dithiobisnitrobenzoate (DTNB; 0.01 mol/L). Brain tissue was homogenised and dissolved in phosphate buffer (0.1 mol/L, pH 8.0), 15 mg of sodium bicarbonate, and DTNB. Enzyme activity is expressed as nmol of hydrolysed acetylthiocholine per min per mg of protein.
Statistical analyses were run on the IBM SPSS Statistics version 21.0 for Windows (SPSS Inc., Chicago, MI, USA). Differences between the means were determined with one-way analysis of variance (ANOVA), followed by Duncan’s multiple range
The XRD results confirmed that IONPs used in our study were free from impurities. TEM analysis revealed a crystalline structure, with irregular and roughly symmetrical morphology, ranging in size from 1 to 100 nm. The average crystallite size calculated with the Scherrer equation was 15.65 nm. These results corroborate the manufacturer’s specifications (Figure 1).
X-ray diffraction (XRD) image showing XRD peaks corresponding to IONPs with a particle size of 15.65 nm (A) and the transmission electron microscopy (TEM) image showing the morphology of IONP aggregates dispersed in double distilled water. Scale bar = 100 nm
Fish exposed to IONPs did not exhibit significant changes in body weight. However, gill weight increased while the hepatosomatic index decreased significantly (P<0.05) after 30 and 60 days of exposure (Table 1). Brain weight remained unchanged throughout the experiment. The hepatosomatic index returned to control levels in the depuration group, while body and organ weights remained unchanged (Table 1).
The Effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) body and tissue weights of the fish Mozambique tilapia (
6.71±0.09 | 6.25±0.40 | 6.31±0.35 | 6.51±0.26 | 6.59±0.38 | 6.47±0.38 | 6.63±0.40 | 6.99±0.13 | |
143±11.9 | 146±3.25 | 152±3.88 | 152±1.19 | 159±3.20 | ||||
13.53±1.86 | 13.78±1.75 | 13.22±1.06 | 12.06±1.42 | 11.98±1.53 | 13.22±0.48 | |||
16.5±1.81 | 16.6±2.23 | 16.3±3.56 | 15.2±1.61 | 15.1±0.90 | 15.3±2.83 | 15.0±1.66 | 19.5±1.08 |
P<0.05 compared to the control group
The ICP-MS analysis confirms the presence of IONPs in the gill, liver, and brain tissues of the fish after 4 and 60 days of exposure (Table 2). The gill tissue exhibited the highest bioaccumulation factor, followed by the liver and brain. The 60-day depuration failed to restore IONP levels to control.
Mean (±SD) Bioaccumulation of iron oxide nanoparticles (IONPs; 15 mg/L) in the gill, liver, and brain tissues of the fish Mozambique tilapia (
60 days | Gill, liver, and brain | Below detection limit | Below detection limit | |
4 days | Gill | 0.53±.017 | 0.04 | |
Liver | 0.19±0.01 | 0.01 | ||
Brain | 0.15±0.01 | 0.01 | ||
60 days | Gill | 7.87±0.26 | 0.53 | |
Liver | 6.25±0.13 | 0.42 | ||
Brain | 1.86±0.10 | 0.13 | ||
Depuration (60 days) | Gill | 2.20±0.08 | 0.15 | |
Liver | 1.90±0.08 | 0.13 | ||
Brain | 0.92±0.13 | 0.06 |
BAF – bioaccumulation factor
The activities of SOD (Figure 2), CAT (Figure 3), GR (Figure 4), and GPx (Figure 5) showed a significant (P<0.05) decrease in the gill, liver, and brain in a time-dependent manner compared to respective controls. Conversely, the levels of hydrogen peroxide (Figure 6) and LPO (Figure 7) increased significantly (P<0.05) in all tissues in a time-dependent manner. Upon 60-day depuration, these levels did not return to control (Figures 2–7).
The effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) activity of superoxide dismutase (SOD) in the fish Mozambique tilapia (
The effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) activity of catalase (CAT) in the fish Mozambique tilapia (
The effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) activity of glutathione reductase (GR) in the fish Mozambique tilapia (
The effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) activity of glutathione peroxidase (GPO) in the fish Mozambique tilapia (
The effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) mean (±SD) hydrogen peroxide levels in the fish Mozambique tilapia (
The effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) lipid peroxidation (LPO) in the fish Mozambique tilapia (
In both gill and liver, ALP activity dropped significantly (P<0.05) in a time-dependent manner. A similar significant and time-dependent drop was observed for brain tissue AChE activity. Again, 60-day depuration did not reverse the activities of these enzymes (Figure 8).
The effect of iron oxide nanoparticles (IONPs; 15 mg/L) on mean (±SD) activity of alkaline phosphatase (ALP) in the fish Mozambique tilapia (
The accumulation of the IONPs in the gill, liver, and brain tissues of
Like all aerobic organisms, fish have well-defined and functional prooxidant/antioxidant systems to counter oxidative stress and the formation of reactive oxygen species (ROS) (42). In our study, exposure to IONPs resulted in depletion of antioxidant enzymes such as SOD, CAT, GR, and GPx in all tissues. This depletion resulted in the accumulation of free radicals, as evidenced by increased levels of hydrogen peroxide. Similar results have been observed in the gill and liver tissues of freshwater orange chromide (
Nanoparticle toxicity is owed to oxygen depletion and accumulation of free radicals (48, 49). Lipids, polyunsaturated fatty acids (PUFA) in particular, possess several double bonds and are highly susceptible to free radical attacks. Exposure to IONPs for 60 days resulted in a significant rise in LPO levels in all three tissues of our test organism, which suggests that gill, liver, and brain are equally targeted by oxidative stress and corroborates our earlier findings of elevated LPO levels in the liver of the same species (50).
Considering that ALP is involved in the hydrolysis of exogenous materials, transphosphorylation, and membrane transport (51), its decreased activity in the gill and liver tissues points to impaired membrane transport and cellular toxicity (50).
The activity of the brain tissue marker, AChE, the key enzyme involved in the breakdown of the neurotransmitter acetylcholine to terminate synaptic neurotransmission (51), dropped in a time-dependent manner, indicating the neurotoxic effects of IONPs. The activities of these marker enzymes remained depleted throughout the depuration period, which corroborates long-term nanotoxic effects.
Clearly, oxidative stress plays a major role in nanoparticle-induced toxicity, and nanoparticles execute it through different mechanisms like generating ROS, disrupting cellular antioxidant defence system, interacting and damaging biomolecules like proteins, lipids, and DNA, as well as by disrupting membrane integrity (52,53,54,55). Our findings well illustrate the cascade of events and the relation between different mechanisms that could lead to oxidative stress. IONP accumulation in the gill, liver, and even brain tissue confirms their internalisation by fish and also the ability to cross the blood-brain barrier and induce neurotoxicity. Accumulation of IONPs inside vital organs disrupted the antioxidant defence system by depleting antioxidant enzymes, resulting in redox imbalance, which in turn induced LPO and likely impaired cell membrane integrity.
Our study also highlights the persistence of IONPs and their toxic effects in the fish even after the depuration period. We therefore need to consider long-term exposure to IONPs and their exacerbating toxicity over time, as it has various biological implications for humans. Even though human health risks resulting from occupational and environmental exposure to IONPs are negligible,
Furthermore, our findings highlight the need for further investigations into the potential risks associated with nanoparticle exposure in aquatic environments.