Abstract
Water bodies are highly pollution-prone areas in which mercury (Hg) is considered as a major menace to aquatic organisms. However, the information about the toxicity of mercuric chloride (HgCl2) in a vital organ such as the liver of fish is still inadequate. This study aimed to assess the impact of mercuric chloride (HgCl2) exposure on the liver of Channa punctata fish over 15, 30, and 45 days, at two different concentrations (0.039 mg/L and 0.078 mg/L). Mercury is known to be a significant threat to aquatic life, and yet, information regarding its effects on fish liver remains limited. The results of this study demonstrate that exposure to HgCl2 significantly increases oxidative stress markers, such as lipid peroxidation (LPO) and protein carbonyls (PC), as well as the levels of serum glutamic-oxaloacetic transaminase (SGOT) and serum glutamic pyruvic transaminase (SGPT) in the fish. Additionally, the transcriptional and protein analysis of specific genes and molecules associated with necroptosis and inflammation, such as ABCG2, TNF α, Caspase 3, RIPK 3, IL-1β, Caspase-1, IL-18, and RIPK1, confirm the occurrence of necroptosis and inflammation in the liver. Histopathological and ultrastructural examinations of the liver tissue further reveal a significant presence of liver steatosis. Interestingly, the upregulation of PPARα suggests that the fish's body is actively responding to counteract the effects of liver steatosis. This study provides a comprehensive analysis of oxidative stress, biochemical changes, gene expression, protein profiles, and histological findings in the liver tissue of fish exposed to mercury pollution in freshwater environments.
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Discover the latest articles, news and stories from top researchers in related subjects.Introduction
Heavy metal contamination is a widespread problem, with a particular emphasis on mercury, in aquatic ecosystems in India. Mercury pollution is a critical concern due to its adverse impacts on the environment and human health. India is a significant contributor to global mercury emissions, and various sources, such as industrial waste, compact fluorescent lamps (CFLs), and groundwater, have resulted in elevated mercury levels in both organisms and humans. The urgency of comprehending and addressing the repercussions of mercury pollution on aquatic ecosystems and public health is needed. Many studies highlight that mercury affects various organs and systems in aquatic organisms, emphasizing the need for environmental and health measures to mitigate contamination. The gravity of mercury pollution in India and its significant implications, emphasizing the importance of monitoring and regulating mercury emissions to protect both the environment and human well-being is largely obscure hitherto. In the list of the world's biggest sources of environmental mercury (Hg), India stands at number two with an approximate discharge of 144.7 tonnes of Hg/year1. Hg contamination in India is pointing towards lethal conditions due to the release of unwanted pollutants having a range of Hg from 0.058 to 0.268 mg/L. This is higher than the permissible Indian and WHO limits of 0.001 mg/L for drinking water and 0.01 mg/L for industrial effluents. Large numbers of mercury poisoning cases have been reported in the recent past, which are largely ignored. The leading anthropogenic and natural release of Hg exists as Mercuric (II) chloride (EPA, 2020).
Mercury enters in the aquatic regimes through various natural (geothermal springs and volcanic eruptions) and anthropogenic activities (coal-fired power plants and waste incineration).Once in the water, mercury undergoes various transformations. Inorganic mercury, such as HgCl2, can be converted into methyl mercury (MeHg), a highly toxic form that tends to bioaccumulate in aquatic organisms. Fish can absorb mercury through their gills, skin, and diet. Inorganic mercury is transformed into organic forms like methylmercury by bacteria in water, and this form is readily taken up by aquatic organisms. As fish consume contaminated prey or come into contact with contaminated water, mercury accumulates in their tissues, particularly in the liver and muscles.Mercuric chloride harms fishes by inducing oxidative stress, damaging cellular structures, particularly in the liver, and triggering inflammatory responses, ultimately compromising fish health and survival2. Additionally, mercury accumulates in fish tissues, disrupting physiological processes and posing risks to both aquatic ecosystems and human consumers. Since Hg is absorbed and bioaccumulated in fish, it harms aquatic regimes as well as human health through biomagnification. The elevated levels of Hg can lead to mortality of aquatic fauna, ultimately decline the number of species, majorly fish communities, and badly impact overall aquatic biodiversity3. Thus, the information on Hg toxicity in aquaculture has become very important in research. A large number of investigations have been performed on the effect of heavy metals on aquatic fauna4,5 but, despite being the imperative organ of xenobiotic metabolism in fish, there is not sufficient information available on the potential risk ofHgCl2pollution induced liver steatosis in fish.
Several studies have documented that Hg imbalances ROS production and its removal by the antioxidant system, which is known as an oxidative stress response6. Oxidative stress plays a significant role in initiating heavy metal toxicity in fish7,8,9. Assessing the activity of lipid peroxidation, protein carbonyl, and biomarker enzymes in liver tissue reflects the expanse of oxidative stress10. There are an ample number of studies describing oxidative stress induced by heavy metals as responsible for necroptosis, inflammation, and apoptosis in different organisms11. Oxidative stress-mediated necroptosis and inflammation inducing liver steatosis in fish remain largely obscure hitherto under long-term exposure to HgCl2. To fill this research gap, the present study was conducted, which illustrates the above-mentioned parameters coupled with the transcriptional and translational profile of certain necroptosis and inflammation related genes in freshwater food fish Channa punctata. This is an empirical study to explore the effects of HgCl2 exposure on ultrastructural perturbations, enzymatic, biochemical, and molecular levels in the liver of fish, which will greatly extend our understanding of the pathways involved in systemic toxicity of HgCl2 in fish. The study is necessary due to the environmental urgency, public health concerns, data gaps, application of advanced research methods, the need for effective policy measures, and the importance of conserving aquatic biodiversity. It serves as a vital step in addressing the multifaceted challenges posed by mercury contamination in India and beyond. This study is innovative in deriving howHgCl2impacts Channa punctata, delving into oxidative stress, necroptosis, and inflammation pathways in the fish liver. By addressing gaps in understanding HgCl2-induced toxicity, it provides unique insights into molecular responses, gene expressions, and protein profiles, fostering a more comprehensive understanding of mercury's multifaceted effects on fish physiology. This enriches scientific literature in the field of aquatic toxicology.
Materials and methods
Test chemical
S.D Fine-chem. Ltd., Mumbai, India manufactured HgCl2 was procured from a scientific chemical dealer.
Chemicals used
Methane sulfonate, ethylenediaminetetraacetic acid, potassium per magnet, dimethyl sulfoxide, hydrochloric acid, 2,4-dinitrophenylhydrazine, trichloroacetic acid, ethanol, ethyl acetate, sodium hydroxide, guanidine hydrochloride, trizol, chloroform, isopropanol, DEPC water, thiobarbituric acid, acrylamide, bisacrylamide, tris base, sodium dodecyl sulphate, ammonium persulphate, Temed, sodium chloride, Tween20, bovine serum albumin, bromophenol blue, glycerol, mercapto ethanol, methanol, sodium carbonate, copper sulphate, potassium sodium tartarate, Folins reagent, acetone, glutaraldehyde, osmium tetraoxide, DPX, Bouins fluid, alcohol.
Determination of median lethal concentration of HgCl2
In order to determine the 96-h LC50 of HgCl2 for Channa punctata, standard protocols outlined in the American Public Health Association (APHA) 201712 and the Organization for Economic Co-operation and Development (OECD) guidelines for fish acute bioassays (OECD203, 92/69/EC, method C1) were followed. The study involved five aquaria, each containing four acclimatized fish with an average weight of 30 ± 3.0 g and length of 14.5 ± 1.0 cm. These fish were exposed to five concentrations of HgCl2 on a logarithmic scale (0.1, 1.0, 10, 100, and 1000 mg/L) for 96 h in a semi-static bioassay system, while maintaining a fish loading rate of 4 g/L of water13. The observed lethality range was noted to be between 0.1 and 1.0 mg/L of HgCl2. Subsequently, a logarithmic series of ten nominal concentrations (0, 0.2, 0.4, 0.6, 0.8, 1.0, 1.2, 1.4 mg/L) was employed to determine the LC50 value. The LC50 values for HgCl2 at 96 h were calculated using the probit analysis method14.
Sample size calculation
The sample size was calculated using the software GPower 3.115,16,17,18,19, based on ANOVA for repeated measures, effects between subjects, a significance level of 5%, a power of 90%, and an expected medium effect size (0.5), yielding 135 fishes.
Experimental design
Channa punctata (30 ± 5.0 g; 15 ± 1.0 cm) were collected from water bodies of Lucknow and its suburbs (26° 55′ N, 80° 59′ E), Uttar Pradesh, India. Specimens were brought to the laboratory and prophylactic treatment (0.05% KMNO4) was given for 3–5 min, to remove exterior contagions if any20. Acclimatization of 135 fish for 15 days was done in 160 L well aerated glass aquaria (100 × 40 × 40 cm3) filled with 100 L of 15 days aged tap water12. Fish were fed two times a day with commercial aquarium food pellets (Perfect Companion Group Company Limited, Thailand) at the rate of 3% of the body weight per day21. A day before the start of the experiment feeding was stopped22. The experimental design consisted of three groups, each replicated in triplicate, with 15 fish in each group. Group I served as the control, while Group II was exposed to a dose of 0.039 mg/L of HgCl2 (equivalent to 96 h-LC50/20). Group III received a dose of 0.078 mg/L of HgCl2 (equivalent to 96 h-LC50/10). These specific concentrations were selected to represent controlled conditions, a sub-lethal dose, and a higher but still sub-lethal dose, respectively, allowing for the assessment of potential effects on the fish over designated exposure period. No mortality was reported during the experiment but some behavioural changes were observed like hyper activeness, surfacing, gulping, and jumping in the fish. The aquaria were cleaned and water was renewed23 daily to prevent waste and debris24. On each sampling day (15, 30, and 45d), three fish from every replicate were anesthetized by using tricaine methane sulfonate (MS-222; 0.3 g/L Sigma Aldrich E10521)25, a heparinized syringe was used to withdraw blood from the caudal blood vessel and stored in vials coated with EDTA (1.8 mg/mL) for ROS examination. Fish were dissected longitudinally from the ventral side and its liver was excised for evaluation of oxidative stress, biochemical, molecular changes, and tissue histology. Samplings were done as per OECD 2019, guidelines. The study was carried out following the ARRIVE guidelines.
Evaluation of cell viability
Cell viability was assessed using the trypan blue exclusion assay at three time points: 15, 30, and 45 days. In this assay, 50 μL of the cell suspension was mixed with 0.4% trypan blue solution in 1:1 (v/v) ratio, and viable cells were quantified using a hemocytometer26,27. Samples with a cell viability exceeding 85% underwent additional analysis using the single-cell gel electrophoresis (SCGE) assay and ROS production. Viable cells, which expelled the dye and exhibited a round, shiny appearance, remained unstained, whereas non-viable cells retained the blue stain (Supplementary Fig. S3).
Percentage of viable cells were counted as follows
ROS production
A fluorescent dye 2′, 7′-dichlorodihydrofluorescein (20 µM, DCFH-DA; Sigma Aldrich, USA) was used to quantify ROS level in the blood of test fish2,28. The fluorescence intensity of stained blood cells depicts the amount of ROS generated. Image J software (version 1.50, USA) was used to measure the corrected total cell fluorescence.
DNA fragmentation assay
DNA fragmentation was measured by SCGE/comet assay27. The assay was conducted using a three-layer technique with minor adjustments. In summary, approximately 15 μL of cell suspension containing about 20,000 cells was mixed with 85 μL of 0.5% low melting-point agarose (LMPA) and layered onto a frosted glass slide pre-coated with 200 μL of 1% normal agarose. After solidification, a third layer of 100 μLLMPA was added. Slides were immersed in a lysing solution overnight at 4 °C. Subsequently, they were subjected to alkaline electrophoresis in fresh cold alkaline electrophoresis buffer for 20 min at 4 °C. Electrophoresis was performed at 15 V (0.8 V/cm) and 300 mA. Slides were neutralized with Tris buffer, stained with ethidium bromide, and comet images were analyzed using an image analyzer system to quantify DNA damage based on percent tail DNA (% tail DNA).
The activity of the liver biomarker enzymes
At 3000 rpm blood was centrifuged for 10 min to separate serum. In the serum, the activity level of SGOT and SGPT was analyzed by kinetic method using the commercial kit (Robonik India Pvt. Ltd, Navi Mumbai). Absorbance was measured using a Shimadzu UV-1700 pharma spec UV–VIS spectrophotometer. Due to the oxidation of NADH to NAD, there was a significant decrease in absorbance measured at 340 nm, which is directly proportional to the activity of SGOT and SGPT in the sample. Its activity is expressed in Units/L.
Estimation of LPO
The LPO in liver tissue was estimated by following the methodology of Buege and Aust, (1978)29. The breakdown of polyunsaturated fatty acids results in the formation of malondialdehyde, which serves as a convenient index for determining the extent of the peroxidation reaction.
Estimation of protein carbonyls in the liver
The method of Levine et al. (1990)30 was used to estimate the activity level of protein carbonyls. A protein-DNP hydrazone moiety is produced due to the reaction of dinitrophenylhydrazine (DNPH) with protein carbonyl groups, which was detected through a spectrophotometer.
Transcriptional analysis of targeted genes
TRIzol method31 was used to isolate total RNA from liver tissue.NanoDrop 2000/2000c (Thermo Scientific, USA) was used to ascertain the quality and quantity of the isolated RNA. cDNA synthesis was performed using Revert Aid H Minus Synthesis Kit (#K1632; Thermo Scientific, USA) as per manufacturer's lab manual, and alteration in the mRNA levels of ABCG2, TNF α, Caspase 3, RIPK 3, IL-1β, PPAR-α, Caspase-1, IL-18 and RIPK1 (Table 1) in response to HgCl2 treatment was quantified by a CFX96™ Real-Time PCR System (qRT-PCR) (C1000 Touch™ Thermal Cycler, Bio-Rad, USA) using SYBR Green Master mix (#A25742; Thermo Scientific, USA). The qRT-PCR data were analyzed using the relative gene expression 2−ΔΔCtmethod32 and the results were depicted as the fold change in mRNA transcripts standardized to the endogenous reference gene β-actin. Bands of amplified DNA were also pictured by 1% agarose gel electrophoresis (Bio-Rad, USA).
Protein expression
Protein expression was assessed by western blotting method for TNF α, Caspase 3, RIPK1, and β-Actin in liver tissue of control and 15, 30, and 45 days of HgCl2 treated (Group II and III) C. punctata. TNF α, Caspase 3, RIPK1, and β-Actin proteins were identified and expressions were evaluated, total protein extricated from hepatic tissue of fish was lysed in RIPA buffer having 1X protease inhibitor, followed by estimation of protein concentrations by the method of Lowry et al., (1951)33. About 20–50 μg of protein was loaded in each lane and allowed for separation by 15% SDS-PAGE and from gel it was transferred to a polyvinylidene difluoride (PVDF) membrane (Bio-Rad Cat. #162-0177). After being blocked with 3% BSA in 1× Tris-buffered saline Tween (TBST) buffer, the membrane was blotted overnight with the primary antibodies at 4 °C and then incubated with the horseradish peroxidase-conjugated secondary antibody (1:5000, Elabscience E-AB-1003) for 1 h at 37 °C. The proteins were distinguished using the Clarity™ Western ECL Substrate (Bio-Rad Cat. # 170-5061), and digital photographs were obtained using a gel-imaging system (Molecular ImagerRChemiDoc™ XRS + with Image Lab™ Software Bio-Rad). The antibodies used for the experiments were: anti-RIPK1 (1:2000, E-AB-18284), anti- TNF α (1:2000, E-AB-33121), anti- Caspase-3 (1:2000, E-AB-66940) and anti- β actin (1: 4000, E-AB-30422).
Histopathology of the liver
For histological observation, Graff et al., 202234 were followed, the liver tissue was cleaned with normal saline solution and kept for 48 h in Bouin’s fluid for fixation then washed with 70% ethyl alcohol repeatedly for 4–5 days to get rid of extra Bouin’s fluid. Tissue was gradually dehydrated in 50%, 70%, 90%, and 100% ethanol, then embedded in paraffin wax. For tissue sectioning Yorco Precision Rotary Microtome, India (YSI062) was used. Finally, sections were stained with hematoxylin and counterstained with eosin for 2 min (Ratn et al., 201835) and examined under an oil immersion microscope (Nikon Corporation K 12432) with 10/40× magnification of the objective lens. Images were analyzed using ImageJ software; version ImageJ bundled with 64-bit Java 1.8.0_172.
Ultra-structural analysis
For scanning electron microscopic (SEM) study tissue was fixed in 2.5% glutaraldehyde solution for a day at 4 °C, and post fixing tissue was kept in 1% osmium tetroxide solution for two hours at 4 °C. Dehydration was performed through a graded series of acetone (50%, 70%, 90%, and 100%) after fixation. Tissue was dried with a critical point drier and then fixed on a metal stub and sputter-with gold plating (about 20 nm thick) and observed under the SEM (JSM 6490). Histopathological observations were analyzed by following Farrel et al., 200836.
Statistical analysis
The triplicate of each group was carried out and data were depicted as mean ± standard error mean (S.E.M.). SPSS software (version 20.0, SPSS Company, Chicago, USA) was used to evaluate the data. The significance (p < 0.05) of data was evaluated using one-way ANOVA with Tukey's post hoc test. Regression and correlation analysis were also performed among various physiological parameters.
Ethical statement
Experimentation was permitted by the Committee for Control and Supervision of Experiments on Animals (CCSEA), Ministry of Environment and Forests, Government of India under registration no.1861/GO/Re/S/16/CCSEA, and approved by the institutional ethical committee of University of Lucknow, Lucknow, India. All methods were performed according to the relevant guidelines and regulations.
Results and discussion
The 96 h-LC50 value of HgCl2 for Channa punctata was 0.783 mg/L with a 95% confidence limit of 0.724 mg/L (Lower) and 0.853 mg/L (Upper). Fish were exposed to two sub-lethal concentrations for chronic study (96 h-LC50/20) and (96 h-LC50/10) of HgCl2. Physicochemical parameters of water such as the potential of hydrogen (pH), the concentration of dissolved oxygen, hardness, temperature, and alkalinity were within the prescribed limits for the endurance of the fish (APHA, 2017)11, and no major variations among these parameters were observed (Table 2).
ROS production was significantly (p < 0.05) augmented following an increase in the concentration of HgCl2 with respect to control (Fig. 1b). An increment in ROS level was recorded in both the HgCl2intoxicated groups in a time-dependent manner. The ROS generation was maximum in group III after 45 d of the exposure period (Fig. 1a).Furthermore, the percentage of tail DNA, indicating DNA damage, was assessed in blood cells from both control and exposed groups (Fig. 2a). Figure 2b illustrates the DNA strand breaks resulting from exposure to HgCl2 in C. punctata fish. Group III exhibited the highest DNA damage on day 45 compared to the control group. Fish exposed to HgCl2 in groups II and III showed significantly elevated DNA damage levels compared to the control group.
In general, the activity of lipid peroxidation (TBARS), protein carbonyls, and liver marker enzymes (SGOT and SGPT) were increased significantly (p < 0.05) in all groups treated with sublethal concentrations of HgCl2 (Fig. 3a–d). Lipid peroxidation was the highest (2.72 ± 0.009) in exposed group III (maximum concentration of HgCl2) as compared to the control (1.90 ± 0.05) after 45 days of the exposure period. In group III the level of protein carbonyls was 81.0 ± 0.87 nmol carbonyls/mg protein which was significantly higher than the control group, where it was 60.8 ± 0.14 nmol carbonyls/mg protein. All the treated groups (groups II and III) show significant (p < 0.05) differences in the level of protein carbonyl as compared to the control group in a time-dependent manner. The activity level of SGOT and SGPT was significantly (p < 0.05) altered after every exposure period in treated groups as compared to the control group. The highest increment in SGOT (32.5 ± 0.00) and SGPT (0.023 ± 0.00) was found in group III as compared to the control 18.5 ± 0.001 and 0.018 ± 0.001 respectively after 45 days.
The metabolism of heavy metals often leads to the formation of reactive intermediates like ROS, which possess high toxicity and can directly cause DNA breakage or hinder the repair of oxidized DNA bases37. While organisms possess antioxidant defence systems to safeguard tissues against oxidative damage, excessive ROS production beyond the capacity of these defence mechanisms can result in cellular and DNA breakage. Oxidative damage to DNA, triggered by ROS production during processes like respiration, has been identified as a significant factor contributing to the extensive and varying levels of DNA damage observed in the gill cells of C. punctata5. Exposure to mercuric chloride in aquatic environments makes fish species like trout, salmon, and tilapia especially vulnerable38. In this study mercuric chloride can induce oxidative stress mediated DNA strand breaks which causes genotoxicity in fish Channa punctata. Similarly, Trivedi et al., 20222 have reported that mercuric chloride can cause genotoxicity in targeted fish. The resulting oxidative damage disrupts cellular functions, initiating lipid peroxidation in biomolecules like lipids and proteins. LPO, along with protein carbonyls serves as a marker for oxidative stress, indicating potential cell death pathways. LPO is a method in which electrons are removed from lipids by free radicals and later produce reactive species. The LPO acts as a cell death signal to induce different cell death pathways and is also capable of damaging phospholipids directly39. Cell damage can be induced by the oxidation of lipids and proteins. So, the LPO and PCs have been identified as markers for lipid and protein oxidation in various organs of the body40. PC groups have been used as biomarkers of oxidative stress41. Increased LPO and PCs in fish liver and kidney can lead to impaired organ function, inflammation, and potential ecological and health risks42. This study is in harmony with Sharma, (2017)43 who has documented similar results and evaluated the lead toxicity in the muscle of fish C. punctata. Furthermore, increased ROS and oxidative stress in fish liver initiates detrimental effects on cellular functions. This disturbance between ROS and antioxidant defences is reflected by elevated activities of enzymes like SGOT and SGPT in this study. The increased SGOT and SGPT levels serve as indicators of disrupted cellular processes, potentially reflecting instabilities in amino acid synthesis and transamination. These enzymatic changes underscore the physiological impact of oxidative stress on fish health, emphasizing the interconnected relationship between ROS-induced damage and the enzymatic responses observed in SGOT and SGPT activities. In this study, increased activity of SGOT and SGPT was observed at sub-lethal exposure of HgCl2.The elevated level of either SGOT or SGPT suggests an increased synthesis of amino acids or an increased transamination process from fatty acids or glucose during HgCl2 intoxication. InC. punctata sub-lethal concentrations of chromium and copper increased the level of SGOT and SGPT activity 37,38. In fish, increased SGOT and SGPT activities can be indicative of liver and kidney diseases. These conditions can affect the overall health and survival of the fish, potentially leading to impaired growth, reproduction, and increased susceptibility to other illnesses.
After 45 days of exposure to HgCl2, the mRNA expression of target genes in fish of all three groups was calculated by qRT-PCR with the 2−∆∆CT method (Fig. 4a). This study promulgates that expression of most of the studied genes (TNF α, Caspase 3, RIPK 3, IL-1β, PPAR-α, Caspase-1, IL-18, and RIPK1)excluding ABCG2 were increased in a time-dependent manner in HgCl2exposed fish in comparison to unexposed fish. In the liver of HgCl2treated fish, the mRNA transcripts of genes TNF α, Caspase 3, RIPK 3, IL-1β, PPAR-α, Caspase-1, IL-18, and RIPK1 were significantly (p < 0.05) induced, and the highest fold change in expressions of all the above-mentioned genes were found as 13.44, 15.7, 6.4, 14.2, 56.5, 26.5, 14.1and 14.14respectively in the liver tissue of 45 days exposed fish of group III in comparison to control. Moreover, ABCG2 mRNA level was significantly (p < 0.05) downregulated in the group III fish in comparison to the group I. However, PCR products separated by agarose gel electrophoresis exhibit changes in band intensities of genes TNF α, Caspase 3, RIPK 3, IL-1β, PPAR-α, Caspase-1, IL-18, and RIPK1 involved inHgCl2induced necroptosis and inflammation (Fig. 4b). For the normalization of data of genes, the β-actin gene was used as an internal control.
Immunoblot study showed that group III had the highest concentration of RIPK1, TNF α, and caspase-3 protein in the liver (Fig. 5a). In each of the treated groups, except the control group, HgCl2 caused an increase in RIPK1, caspase-3, and TNF α protein. The HgCl2-induced increment in aforesaid mentioned protein level was the highest in group III exposed with the highest concentration of HgCl2. The distribution of TNF α, RIPK1, and caspase 3 proteins are shown in Fig. 5a, b for both control and treated groups.
This study also evaluated HgCl2 exposure induced necroptosis and inflammation in the liver tissue, associated with oxidative stress. There is very little information present on oxidative stress induced necroptosis and inflammation in the fish liver due to exposure to mercuric chloride. This study tries to fill this gap and evaluate the oxidative potential of HgCl2.The protein profile, and mRNA expressions of genes involved in necroptosis (TNF α, Caspase 3, RIPK 3, and RIPK1) and inflammation (IL-1β, Caspase-1, and IL-18) were measured in liver tissue of C. punctata, treated with different concentrations of HgCl2to analyze the effects of potential oxidative stress inducers on necroptosis and inflammation. Overall protein profile and mRNA expressions were increased in the liver and revealed that the increased oxidative stress may lead to damage to the cell and its protein in test fish. In an aquatic ecosystem, fish often play important roles in nutrient cycling and as prey for other organisms. Liver damage and increased inflammation in fish can have cascading effects on the ecosystem by disrupting these ecological interactions44.
The onset of oxidative stress, triggered by mercuric chloride exposure in fish Channa punctata, initiates a cascade of molecular responses. This study delves into the intricate connection between oxidative stress and the gene expression of necroptosis and inflammation-related genes. As ROS disrupt cellular homeostasis, the upregulation of genes associated with necroptosis (such as RIPK1 and RIPK3) and inflammation (including TNF α, Caspase-3, IL-1β, and IL-18) signifies molecular pathway activation. This interplay sheds light on the intricate molecular mechanisms underlying the impact of oxidative stress on the transcriptional profile, providing valuable insights into the fish's cellular responses to environmental mercury contamination. One of the largest families of membrane proteins comprises ATP-binding cassette (ABC) transporters that translocate numerous substrates and heavy metals across the plasma membrane. Amongst the ABC transporters, ABCG2 is recognized as an active transporter for heavy metals. ABCG2 gene can transport HgCl2 in the cells45 and the downregulation of ABCG2 in this study is responsible for the efflux of HgCl2 in the liver, Similarly, Liu et al., (2016)46 documented that decrement in the mRNA expression of ABCG2 transporters may control Cd transport across the placenta. It is well established that inflammation is responsible for enhancing ROS generation resulting in oxidative stress and is thought to be responsible for HgCl2-induced liver toxicity. In this study, the intoxication of HgCl2 significantly (p < 0.05) increased protein levels and mRNA transcripts of TNF-α, IL-1β, Caspase-1, and IL-18 levels, reflecting inflammatory responses. Similarly, HgCl2 induced hepatic damage in rats by interfering with oxidative stress and inflammation47. Some ligands when attached to TNF family death domain receptors can activate necroptosis. In this study, HgCl2 often triggers downstream key proteins, including RIPK1 and RIPK3. Specifically, RIPK1activates RIPK3 then phosphorylation of Mixed Lineage Kinase Domain-Like Pseudokinase (MLKL) takes place and is translocated to the cell membrane where it induces pore opening and necroptosis48. Similarly, Zhang et al., (2017)49 documented mitochondria derived ROS promoted oxidative stress induced automatic addition of phosphorus groups to RIPK1, this instigates RIPK1 to form necrosome with the help of RIPK3, resulting in the start of TNFα-mediated necroptosis in colon cancer cells. Numerous studies testified that heavy metals could induce cell death pathways in hepatocytes20,28,31,35,50,51. The cell death induced by mercuric chloride can provoke an inflammatory response, contributing to further damage and impairing liver function. Fish play integral roles in aquatic ecosystems, and liver damage can disrupt these ecosystems by affecting nutrient cycling and the food web52. However, it is still arcane whether HgCl2 can induce necroptosis in the liver of fish or not and its mechanisms involved in oxidative stress mediated necroptosis and inflammation remain to be clarified. Also, this is the first study in fish C. punctata that documents the role of PPARα against HgCl2-induced oxidative stress mediated necroptosis and inflammation. PPARαis highly expressed in vital organs such as the liver53. The expression of PPARα is closely related to oxidative stress and LPO. Therefore, the significant (p < 0.05) upregulation of PPARα in this study may reduce the overload of oxidative stress and also suggest an increase in oxidized fatty acids54. PPARα nuclear receptors regulate the expression of enzymes and proteins involved in inflammation. So, once PPARα gets activated it prevents inflammation in the liver tissue of fish. There is an ample number of data on the alleviating capacity of PPAR-α against oxidative stress induced inflammation53,55,56 but still a lot more has to be done for the aquatic organism.
Scanning electron microscope images and stained microphotographs of control as well as treated fish tissue are depicted in Fig. 6a, b. Liver tissue of control fish displayed normal histology and morphology, whereas micro steatosis and macro steatosis were prominent in group II and group III, treated with HgCl2. The uneven fat deposition was recorded among the allHgCl2 treated groups; defined foci of micro steatosis were most prominent in areas of the hepatic lobule of group II fish liver tissue. However, macro steatosis appeared to be a more common feature among the fish treated with the highest concentration of HgCl2. The100× images display representative foci of inflammatory cells scattered among regions of micro- and macro-steatosis present in HgCl2 treated groups. The SEM facilitated the observation of micro steatosis and macro steatosis in the HgCl2 treated liver (Group II and III).
The augmented expression of necroptosis and inflammation-related genes in response to mercuric chloride exposure, as observed in this study, establishes a noteworthy link to the development of liver steatosis in fish. The upregulation of genes such as RIPK1, RIPK3, TNF α, Caspase-3, IL-1β, and IL-18 signifies a molecular orchestration that contributes to the observed pathological changes. This study unveils a direct correlation between heightened gene expression and the manifestation of liver steatosis, providing a comprehensive understanding of the molecular mechanisms underpinning the adverse effects of mercury contamination on fish liver health. Liver injury and its severity are directly proportional to regulated cell death. Hepatocyte death is a critical event in the progression of liver disease, ultimately leading to fibrosis due to the resultant inflammation. The pathogenesis of various liver disorders is a consequence of apoptosis, necrosis, necroptosis, steatosis, autophagy, pyroptosis, and ferroptosis. In this study, HgCl2 increases the accumulation of lipids leading to liver steatosis. Similarly, an increase in severe liver lesions/damage was reported due to enhanced hepatic steatosis in animals exposed to Cd57. Moreover, it is well established that Hg exposure increases the susceptibility of the liver to oxidative stress mediated steatosis in zebrafish58. Fish with liver steatosis may suffer from poor growth, weakened immune responses, and increased susceptibility to other diseases and stressors. Moreover, Liver steatosis can affect reproductive capabilities, potentially leading to decreased fish population size59. Liver steatosis induced by heavy metals in fish can disrupt nutrient cycling within aquatic ecosystems, affecting the availability of essential nutrients for other organisms53,60. Changes in fish populations and their health can have cascading effects throughout the food web, potentially leading to imbalances and reduced biodiversity.
Evaluation by correlation among targeted parameters exhibited a strong connotation of physiological and molecular perturbations with higher correlation coefficient (R) values in the liver tissue of HgCl2 exposed fish. Precisely, the increased generation of ROS causes oxidative stress which is evident by an enhancement in lipid peroxidation and protein carbonyl activity in hepatic tissue. Therefore, a strong positive correlation was detected amid ROS and LPO, protein carbonyl, SGOT, and SGPT in the liver of fish treated with HgCl2 (Supplementary Table 1). Furthermore, a strong positive correlation between ROS and LPO, TNF α, Caspase 3, RIPK 3, IL-1β, PPAR-α, Caspase-1, IL-18, and RIPK1 was found in the liver treated with HgCl2. The relationship between ROS, LPO, and protein levels of TNF α, caspase-3, and RIPK1 was analyzed to examine the relationship between oxidative stress, necroptosis, and inflammation in the test fish. The correlation between transcripts of mRNA and the protein level of targeted genes of necroptosis and inflammation showed a strong positive correlation in the HgCl2 intoxicated fish, Channa punctata (Supplementary Table 2).
This study provides crucial insights into the physiological and molecular responses associated with oxidative stress, necroptosis, and inflammation in the liver of a freshwater food fish. The findings reveal significant alterations in ROS production, lipid peroxidation, liver marker enzymes, and the expression of genes related to necroptosis and inflammation, shedding light on the intricate mechanisms of mercury-induced toxicity. The study's application lies in addressing the urgent environmental and public health concerns related to mercury contamination in aquatic ecosystems, particularly in India. By elucidating the pathways involved in liver steatosis and the molecular responses triggered by HgCl2, this research contributes valuable information for formulating effective policies to mitigate mercury pollution, safeguarding fish populations, and ultimately preserving the ecological balance of aquatic ecosystems. The documented correlations between oxidative stress, necroptosis, and inflammation underscore the interconnectedness of these processes, emphasizing the need for comprehensive approaches in addressing the multifaceted challenges posed by mercury contamination.
Conclusion
The findings of the study were analyzed and interpreted in the context of the research gaps. The authors highlighted the significant increase in oxidative stress markers, the presence of necroptosis and inflammation, and the occurrence of liver steatosis as a result of HgCl2 exposure. The upregulation of PPARα was interpreted as the fish's response to counteract the effects of liver steatosis. The findings of the study reveal that HgCl2 exposure induced oxidative stress, lead tonecroptosis and inflammation in the liver of fish C. punctata through the regulation of TNF α/ RIPK1/RIPK3/Caspase 3/ Caspase 1/ IL1-β/IL18 signaling (Fig. 7). This study establishes a link between various consequences of HgCl2 exposure in the fish liver, emphasizing the role of oxidative stress in hepatotoxicity. Further research is needed to fully understand the mechanism of PPARα in mitigating heavy metal toxicity. The study holds practical applications in environmental protection, public health, fisheries management, and policy development, addressing the critical issue of mercury contamination in aquatic ecosystems and its implications for human health.
Data availability
All data generated or analyzed during this study are included in this manuscript (and its Supplementary Information files).
Abbreviations
- HgCl2 :
-
Mercuric chloride
- ROS:
-
Reactive oxygen species
- LPO:
-
Lipid peroxidation
- PC:
-
Protein carbonyls
- SGOT:
-
Serum glutamic-oxaloacetic transaminase
- SGPT:
-
Serum glutamic pyruvic transaminase
- ABCG2:
-
ATP-binding cassette subfamily G member 2
- TNF α:
-
Tumour necrosis factor-alpha
- RIPK 3:
-
Receptor-interacting protein kinase 3
- Cas-3:
-
Caspase-3
- IL-1β:
-
Interleukin-1β
- IL-18:
-
Interleukin-18
- Cas-1:
-
Caspase-1
- RIPK1:
-
Receptor-interacting protein kinase 1
- PPAR α:
-
Peroxisome proliferator-activated receptor alpha
- LC:
-
Lethal concentration
- KMNO4 :
-
Potassium per magnet
- APHA:
-
American Public Health Association
- OECD:
-
Organization for Economic Co-operation and Development
- EDTA:
-
Ethylenediaminetetraacetic acid
- NADH:
-
Nicotinamide adenine dinucleotide (NAD) + hydrogen (H)
- NAD:
-
Nicotinamide adenine dinucleotide
- RNA:
-
Ribonucleic acid
- cDNA:
-
Complementary deoxyribonucleic acid
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Acknowledgements
We are thankful to the Head, Department of Zoology, University of Lucknow, Lucknow (226007) for providing laboratory facilities. We also record our sincere thanks to the University's sophisticated instrumentation center, Babasaheb Bhimrao Ambedkar University, Lucknow for providing a scanning electron microscope facility.
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Ms. Shefalee Singh: Raw data collection and writing the first draft of the manuscript. Ms. Shikha Dwivedi: Experimental setup and maintenance. Mr. Adeel Ahmad Khan: Transcriptional analysis. Ms. Anamika Jain: Sampling and maintenance of fish specimens in the wet lab. Dr. Shraddha Dwivedi: Statistical analysis of the data. Dr. Kamlesh Kumar Yadav: Analysis of biochemical indices. Dr. Indrani Dubey: Analysis and interpretation of data and management of the references. Dr. Abha Trivedi: Histopathological investigation and analysis. Dr. Sunil P. Trivedi: Supervision, Validation of Methodologies. Dr. Manoj Kumar: Conceptualization, designing of experiment, review, and editing of the manuscript.
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Singh, S., Dwivedi, S., Khan, A.A. et al. Oxidative stress, inflammation, and steatosis elucidate the complex dynamics of HgCl2 induced liver damage in Channa punctata. Sci Rep 14, 9161 (2024). https://doi.org/10.1038/s41598-024-59917-4
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DOI: https://doi.org/10.1038/s41598-024-59917-4
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