Abstract
The objective of this study was to detect the effects of acute aflatoxin B1 (AFB1) exposure in Nile tilapia (Oreochromis niloticus) and the effectiveness of Saccharomyces cerevisiae and silicate in reducing these effects. Two hundred and forty Nile tilapia fingerlings (16 ± 0.5 g) were randomly assigned to four experimental groups, each with 60 fish and three replicates. Control basal diet (Diet 1) and three test diets were formulated, where Diet 2 was supplemented with 200 ppb AFB1. Diets 3 and 4 were intoxicated with AFB1 (200 ppb) and supplemented with 0.5% S. cerevisiae or 0.5%, respectively. After 60 days, Diet 1 had considerably greater growth characteristics than the other groups (p < 0.05). Diet 2 revealed a reduced (p < 0.05) survival rate after 1 month of exposure. In addition, Diet 1 showed higher (p < 0.05) total protein and albumin levels than Diets 3 and 4. AFB1 residues were detected in the liver in fish-fed Diet 2, Diet 4, and Diet 3. Alanine aminotransferase, aspartate aminotransferase, creatinine, and urea levels increased (p < 0.05) in fish-fed Diet 2. The glutathione peroxidase, lysozyme, and catalase activity were decreased (p < 0.05) in the fish-fed Diet 2. The malondialdehyde level was significantly higher in fish given Diet 2 (p < 0.05) than in fish-fed Diets 3 and 4. Histopathological investigation of fish-fed Diet 2 revealed impaired liver and spleen; however, both treatments (Diets 3 and 4) successfully lowered inflammation and preserved liver and spleen integrities. In conclusion, AFB1 impaired growth performance and posed a severe health risk to Nile tilapia. Furthermore, S. cerevisiae alleviated the contamination of AFB1 effects more efficiently than silicate employed for toxin adsorption.
Similar content being viewed by others
Avoid common mistakes on your manuscript.
Introduction
Aquaculture is being expanded globally to offer food and nutritional security for the world’s rising population [1]. The initial step towards long-term aquaculture sustainability is a nutritionally balanced feed that is carefully manufactured and safe for nourishing aquatic species [1, 2]. Moreover, including plant protein components may pose significant concerns due to the possibility of fungal growth [3]. When certain physical, chemical, and biological conditions are present in uncontrolled storage conditions, fungi produce mycotoxins and toxic metabolites that accelerate the degradation of feed ingredients and feed [4]. To date, more than 300 distinct mycotoxins have been separated due to sophisticated methodologies and a growing interest in this field of research [5]. Aflatoxins (AF) constitute a significant class of mycotoxins, with aflatoxin B1 (AFB1) being the most toxic and displaying the most significant health risk [6]. AFB1 exposure may adversely affect aquatic animals’ health and performance [7]. Damage to the gills and intestines, failure of hepatorenal function, cytotoxicity, oxidative stress, neurotoxicity, and immunosuppression are the most obvious signs in aquatic animals fed diets contaminated with AFB1 [8, 9]. Accordingly, contaminated diets with AFB1 are the main reason for growth retardation in aquatic animals in fish farming. Thus, they result in high mortalities, reducing fish production and causing economic losses [9]. Fish suffering from aflatoxicosis B1 have pale gills, poor blood coagulation, slow growth, immunosuppression, and increased mortality [10]. Liver tumors are brought on by prolonged feeding of low quantities of AFB1, and they manifest as light-yellow lesions that can migrate to the kidney [10, 11].
Feeding Nile tilapia with diets polluted with aflatoxin in deficient concentrations can cause histopathological damage and disturb their physiological balance [12]. Residual aflatoxin levels in the liver and carcass of fish exposed to concentrations of aflatoxin higher than 350 µg kg−1 in the feed were previously detected, as well as exposure to 50 µg AFB1 kg−1 for 120 days in lambari (Astyanax altiparanae) fish which resulted in residual levels of AFB1 in the muscle tissue [13, 14]. Practically, destroying the contaminated feed is impossible; therefore, to avoid the effect of this toxic substance, improvement in animal immunity must be made. Various physical, chemical, and biological techniques are used to detoxify and decontaminate mycotoxin-containing animal diets. These techniques involve eliminating mycotoxins from contaminated feed ingredients, reducing the bioavailability of such mycotoxins in animal intestinal pathways, and directly destroying mycotoxins in the feed. Adsorbent-mediated AF degradation is a well-known and widely utilized approach for reducing the danger of mycotoxicoses in animals by integrating them into contaminated feed, thereby preventing and decreasing mycotoxicosis and transportation of mycotoxins into animal products [15,16,17,18]. Silica, or silicon dioxide (SiO2), is a primary binding agent in the food industry. It is also employed in the chemical sector as an adsorbent or glidant to allow powder to flow easily when producing tablets [19, 20]. Silica is not digested or absorbed in the intestinal tract, posing no toxicity risk. Moreover, silica is generally recognized as safe by the FDA [20].
Over the past 10 years, interest in the biological detoxification of AFB1 has grown significantly. According to several studies, lactic acid bacteria, bifidobacteria, and yeast can bind mycotoxins and minimize their toxicity [21,22,23,24]. Saccharomyces cerevisiae is the most effective probiotic for binding AFB1 in food and feed [25, 26]. Moreover, it is one of the biological biodegrading agents that can promote growth performance, immune activity, and carcass characteristics. The efficacy of S. cerevisiae cells, both intact and heat-inactivated, has been demonstrated as a toxin adsorbent [25, 27].
The present study aimed to study the effects of acute dietary AFB1 toxicity in Nile tilapia (Oreochromis niloticus) and to investigate the potential role of the probiotic yeast and silicate to ameliorate the health hazard effect of AFB1 in the diet of Nile tilapia. The growth performance, blood biochemistry, mortality rate, and bioaccumulation of aflatoxin residues were also highlighted.
Materials and Methods
Ethical Statement
The study protocol was approved by The Institutional Animal Care and Use Committee of Kafrelsheikh University’s ethical review board, Faculty of Agriculture, Kafrelsheikh University, Egypt.
Fish and Experimental Facilities
A private farm in Kafr El Sheikh, Egypt, provided 240 mono-sex Nile tilapia (O. niloticus) fingerlings with a total initial body weight of 16 ± 0.5 g/fish. The fish were exposed to experimental conditions for 15 days in three indoor circular fiberglass tanks prior to the trial (1 m3). Fish were fed a control diet (30% crude protein and 6.5% crude fat) throughout this time. The fish were acclimated before being randomly divided into 12 glass aquariums, each measuring 30 × 40 × 60 cm. These aquariums represented four different types of experiments (in triplicate). There were 20 fish stocked in each tank. Throughout the experiment, feces and uneaten feed were removed from the aquarium by siphoning two-thirds of the water and replacing it with clean, well-aerated water from a storage tank. This allowed for the maintenance of clear, healthy water throughout the trial. During the 60-day feeding trial, fish were fed the test diets up to satiation level. Water quality measures were recorded throughout the experiment for temperature, pH, oxygen, salinity, and total ammonia nitrogen as follows: 27 ± 0.2 °C, 7.1 ± 0.1, 5.8 ± 0.1 mg/L, 11.5 ppt, and 0.1 ± 0.02 mg/L, respectively.
Aflatoxin B1, Saccharomyces cerevisiae, and Silicate Sources
Aflatoxin was produced by growing Aspergillus parasiticus (standard toxigenic strain, NRRL 2999 culture, lyophilized strain, was kindly obtained from Vet. Med. Microbiology Dept., Iowa State University, USA) on rice fermentation. The moldy rice was steamed to kill the fungus, dried, milled, and analyzed for aflatoxin determination [28]. A Saccharomyces cerevisiae–based product (MiaMyco-Fit®: A product of MIAVIT GmbH Company, Germany) used in the study was added to the diet in a dose of 0.5 g/kg diet. Modified silicon dioxide (silicate) (Fylax®: A product of Selko Feed Additive) used in the study was added to the diet in a 0.5 g/kg diet.
Test Diet Preparation
The basal diet was formulated using the ingredients in Table 1 with 30.1% crude protein and 17.9 kJ/kg gross energy. The first diet was assigned as control without any additives. The second, third, and fourth basal diets were supplemented with 200 ppb standard toxigenic strain of aflatoxin B1 (AFB1) as sublethal doses. The third diet was supplemented with 0.5 g MiaMyco-Fit®/kg as S. cerevisiae–based biological detoxifier. The fourth diet was supplemented with 0.5 g Fylax®/kg as a silicate-based detoxifier.
Ingredients and proximate compositions of the experimental diets are presented in Table 1. All ingredients were finely ground, weighed, mixed manually for 5 min, and then transferred to a mixer for another 15 min. After mixing the dietary ingredients in a food mixer, they were pelleted via a 1.6–2.1 mm diameter die in a laboratory storage container. The four formulated diets were prepared biweekly to ensure the intended AFB1 level. The pellets were air-dried at room temperature before being stored in a freezer until needed.
Sample Collection
After 60 days, the fish was fasted for 24 h, and the following formulas were used to compute the growth parameters based on the body weight and length of each fish in each tank according to Bulut et al. [29]:
Weight gain (%) = (final weight-initial weight) × 100/initial weight.
Specific growth rate (SGR, %day−1) = [Ln (final weight) − Ln (initial weight)/duration] × 100.
Feed conversion efficiency (FCE) = live weight gain (g)/dry feed intake (g).
Protein efficiency ratio (PER) = live weight gain (g)/dry protein intake (g). Survival (%) = 100 × (final no. of fish/initial no. of fish).
Whole-Body Proximate Analysis
Three individual fish were collected randomly from each replicate and kept at − 20 °C for later examination. All diets and whole-body fish composition, including dry matter, crude protein, crude fat, and ash content, were determined using AOAC [30] methodology. Viscera and liver of Nile tilapia were dissected from the fish above, weighted individually to calculate the viscerosomatic index (VSI) and hepatosomatic index (HSI) using the following formulae:
VSI (%) = weight of viscera/weight of fish × 100.
HSI (%) = weight of liver/weight of fish × 100.
Biochemical Analysis
Blood samples were collected at the end of the experiment, and the serum was separated by centrifugation at 3000 rpm for 15 min at 4 °C. Serum samples were examined for the concentrations of total proteins and the major protein fractions in order to assess changes in the protein profile in Nile tilapia. To separate serum protein fractions, serum protein electrophoresis was carried out on agarose gel following the manufacturer’s application instructions using an automated electrophoresis machine and commercial diagnostic kits [28]. Zone electrophoresis was used on a buffered agarose gel with a pH of 8.7 to separate the various serum protein fractions.
The labeled sample wells on the agarose gel were filled with 10 µL of each serum sample. Each batch of samples contained control serum (Control Serum Human Normal, Sebia Corporate, France). The electrophoretic migration was carried out continuously for 15 min at 20 °C using 10 W, 40 mA, and 240 V. After migration, the gels were dyed in an amido black staining solution, then de-stained using acidic solutions and thoroughly dried. After the gels had been separated and stained, the staining intensity of each protein band was measured using a densitometer, the Epson Perfection V700 (Epson America Inc., CA, USA), together with the image analysis program Phoresis version 5.50 (Sebia Corporate, France).
Serum aspartate aminotransferase (AST), alanine aminotransferase (ALT), creatinine, and urea were detected using ready-made kits, following the manufacturer’s instructions [31].
Aflatoxin Residue Analysis
Liver and muscle were collected from three fish per replicate, combined in triplicate, yielding three analytical samples per group, which were then transferred into individual microtubes for AFB1 identification and measurement. The tissues were ground and stored at − 20 °C until analysis. Michelin et al. [14] mentioned that aflatoxins were identified in liver and muscle samples using HPLC and immunoaffinity column cleanup.
Histopathological Analysis
Three fish from each replicate tank were used for the liver and spleen morphology study. The entire spleen and liver were removed and collected to prepare the histological sample. All tissues were thoroughly washed with PBS (pH = 7.4) and immediately fixed in Davidson’s solution (agitated for 5 min) for 8 h to remove intestinal content. After that, the fixed tissues were gradually dehydrated in ethanol (70 to 100%), cleaned twice with xylene (1 and 2 h), and embedded in paraffin. Sections of 5-µm thickness were collected and stained with hematoxylin and eosin. Two cross-sectional slices were prepared from each tissue. The tissue slices were stained with hematoxylin and eosin before being examined using a light microscope (Eclipse 50i; Nikon, Tokyo, Japan) and camera (Digital Sight DS2MV with a DS-L2 control unit, Nikon) by using SigmaScan Pro 5 software. For each tissue, ten measurements were obtained according to de los Santos et al. [32].
Measurement of Antioxidant Enzyme Activities
Using the thiobarbituric acid technique, malondialdehyde (MDA) levels were assessed [33]. The levels of GPx and catalase (CAT) in serum were assessed spectrophotometrically following the techniques used in other investigations [34] and [35], respectively. Lysozyme activity in serum was measured using turbidimetric assays [28]. The quantity of enzyme that resulted in a 0.001/min drop in absorbance was referred to as an enzyme activity unit.
Statistical Analysis
Using SPSS version 22 (SPSS Inc., IL, USA), one-way analysis of variance was performed on the collected data. The homogeneity and normality of the variance were evaluated using the Shapiro–Wilk and Levene tests. Duncan’s test was used as a post hoc test, and differences between the means were examined at the 5% probability level.
Results
Growth Performance
The results of the growth and survival rate of O. niloticus exposed to either 200 ppb AFB1 with or without anti-mycotoxin (biological or chemical) treatments for 30 and 60 days are presented in Table 2. In comparison to the control group, all growth performances as indicated by the final weight (FW), weight gain (WG), specific growth rate (SGR), feed conversion efficiency (FCE), protein efficiency ratio (PER), and survivability were deteriorated significantly after 1 month feeding on 200 ppb aflatoxin B1, followed by chemical (silicate-based product) treated group (Diet 4) than biological (S. cerevisiae–based product) treated one (Diet 3) (p < 0.05), respectively.
Whole-Body Proximate Analysis
The body composition and somatic indicators of Nile tilapia are shown in Table 3. Except for whole-body protein and hepatosomatic index (p > 0.05), investigated diets demonstrated non-significant (p > 0.05) effects on whole-body proximate analysis and somatic indices when compared to the control group. Diet 2-fed fish had the lowest whole-body crude protein content and HSI (p > 0.05).
Aflatoxin B1 Residues
Only the liver of Nile tilapia fish was substantially (p < 0.05) affected by the experimental treatments; the muscular tissues remained unaffected (Table 4). Aflatoxin accumulation in the liver of fish given 200 ppb aflatoxin B1–contaminated diet (AFB1) (Diet 2) rose considerably (p < 0.05). However, after supplementation with chemical (silicate-based product) or biological (S. cerevisiae–based product) treatments considerably (p < 0.05) lowered the concentration of aflatoxin residues, with an advantage towards the biological treated group (S. cerevisiae–based product) (Diet 3). Furthermore, no residues were discovered in fish muscle in all fish groups fed on the experimental diets for 60 days.
Liver and Spleen Histopathological Analysis
The most visible pathologic lesions were found in fish livers given a 200 ppb AFB1-contaminated diet (Diet 2). The livers had significant vacuolation, hepatocyte degradation, and necrotic alterations in the hepatopancreas. There were several preneoplastic foci as eosinophilic and clear foci types and significant nodular pancreatic proliferation (Fig. 1B). The liver of the control fish showed both normal hepatocytes and hepatopancreas. The liver of fish supplied with AFB1 and treated with S. cerevisiae–based product was within the normal limits (Fig. 1C): The liver supplied with AFB1 and treated with silicate showed liver degeneration signs and loss of hepatocytes regular structure (Fig. 1D). The spleen of fish given an AFB1-contaminated diet (200 ppb) without any treatment showed considerable lymphoid hypoplasia, severe atrophy of the melano-macrophage centers, and red pulp congestion (Fig. 1F). Spleens in the group given AFB1-contaminated diet but treated with silicate feed additive showed lymphoid hypoplasia with somewhat less exaggeration where lymphocytes occurred in lymphoid follicles; however, spleen of fishes fed on AFB1-contaminated diet and treated with S. cerevisiae–based product showed marked lymphocytes within the white pulp and normally scattered melano-macrophages centers (Fig. 1G, H).
Blood Serum Protein
Figure 2 reveals a photograph of SDS-PAGE of the protein fractions in the serum of Nile tilapia. Figure 3 demonstrates the electrophoretograms of the protein fractions and changes in their proportion in all tested groups. Following the addition of 200 ppb AFB1 to the Nile tilapia diet (Diet 2), total protein and albumin were considerably (p < 0.05) decreased, while gamma one globulin levels were markedly increased (Table 5 and Figs. 2 and 3). Furthermore, when compared to the (Diet 2) group, the chemical and biological treatments significantly (p < 0.05) increased the levels of total protein and albumin and reduced gamma one globulin level to mimic the values in the control.
Serum Biochemical Evaluations
Compared to the control group (group 1), Nile tilapia exposed to 200 ppb AFB1 (Diet 2) had substantially higher serum AST and ALT hepatic enzyme activity, as shown in Table 6. These levels were also markedly reduced within the chemical or biological treated groups (Diet 3 and Diet 4). With increasing exposure period, from 30 to 60 days, these values within each group also considerably rose.
After 30 days of the trial, exposure to AFB1 (Diet 2) significantly increased serum creatinine and urea levels (Table 7). The effect of 200 ppb AFB1 (Diet 2) on Nile tilapia’s serum creatinine and urea levels was interestingly and significantly reduced by biological and chemical treatments (Diets 3 and 4, respectively). Furthermore, the biological treatment (Diet 3) revealed higher efficacy in decreasing the creatinine and urea levels, similar to the control group after 60 days of the trial.
Antioxidative‐Related Biomarkers
Figures 4, 5, 6, and 7 demonstrate the antioxidative and immune parameters in tested fish. The serum MDA activity increased significantly (p < 0.05) in fish fed 200 ppb AFB1 (Diet 2) compared to other tested groups. Moreover, it showed significantly declined serum catalase, glutathione peroxidase, and lysozyme activities compared to the control group (p < 0.05; Figs. 5, 6, and 7). S. cerevisiae–based product (MiaMyco-Fit) enhanced all antioxidant and immune parameters more efficiently than the silicate-fed group.
Discussion
As a result of the growing usage of plant-based additives in aquaculture feeds, aquatic animals became more sensitive to the effects of mycotoxins [28, 36]. Aflatoxin is a prevalent mycotoxin that has a deleterious impact on the health and development of aquatic animals. Aflatoxin B1 (AFB1) is a biological toxin generated by Aspergillus flavus and Aspergillus parasiticus when environmental conditions are appropriate [37]. These toxic substances can impact animal health and production, as well as cause harm to human beings if they are ingested [28, 36, 37]. The present study employed acute AFB1 toxication (200 ppb) for Nile tilapia with or without medications. Exposure of Nile tilapia to AFB1 at 200 ppb for 8 weeks has significantly reduced growth performance, including total weight gain, specific growth rate, protein efficiency ratio, and survivability, compared to control. These results were consistent with previous findings revealing similar growth performance retarding effects of aflatoxin in Nile tilapia, thinlip grey mullet (Liza ramada), and rainbow trout (Oncorhynchus mykiss) [9, 38,39,40,41]. The reduction of survivability of tilapia by AFB1 that has been reported is similar to what previously demonstrated in a 200 ppb/kg AFB1 in diet, fed for 10 weeks or 16 weeks, showed 34.34% and 30% mortality rate in Nile tilapia, respectively [28, 42]. The observed decrease in growth performance and fish survival might be related to protein synthesis impairment, poor hepatic metabolism, suppressed appetite, and nutritional malabsorption [38, 43].
Administration of yeast and silicate attenuated the detrimental effects of mycotoxins on weight gain and FCR of fish as suggested by the previous studies [42, 44,45,46]. In this study, the addition of Saccharomyces cerevisiae–based diet significantly counteracted the growth-suppressing effects of AFB1. At the same time, supplementation of Nile tilapia with silicate did not succeed in similar growth improvement. The success of yeast in boosting the growth and survivability of Nile tilapia may be related to its supportive effects on internal organs, particularly liver integrity, which is the first organ to be harmed by AFB1 [44, 47]. Similarly, Rahman et al. [48] reported that S. cerevisiae relieved the negative impacts of AFB1 exposure and enhanced the growth performance of Nile tilapia. In addition, Yang et al. [49] reported that turbot (Scophthalmus maximus) intoxicated with AFB1 and treated with yeast cell wall extract showed enhanced growth performance and feed efficiency. Yang et al. [49] related the mitigation role of yeast cell wall extract on AFB1 toxicity with the promoted intestinal microbiota diversity and reduced abundance of harmful pathogens. The liver is the main organ for silicate metabolism [50]; therefore, the lower growth value of the silicate-based product in this trial may be due to the aflatoxin-degenerative effect on the fish liver. HSI fish morphological indicator provided information on the physiological state and nutritional health of the fish. The loss of vacuolation and fat in the liver probably caused the significant decline in HSI in fish-fed Diet 2.
Mycotoxins present in fish directly endanger human health, primarily because of their toxic effects. Since there is currently no safe level for mycotoxin residues in fish, detecting mycotoxins in fish organs and tissues is crucial for determining the danger to public health and the amounts of mycotoxins in various fish tissues. AFB1 accumulation in the hepatic and muscular tissue was demonstrated in several studies [51,52,53,54,55]. In most of these trials, the residual AFB1 level in the liver is more significant than in the muscle. In this investigation, the AFB1 residue was discovered only in the liver of Nile tilapia fed on tested diets but not in the edible flesh. The most likely reason for that is the presence of a variety of P450 enzymes in the liver that play an essential role in the AFB1 metabolism and detoxification process, in which AFB1 is activated to the toxic form (AFBO) or converted to be less toxic as AFM1, AFP1, and AFQ1 [56]. This finding lines up with previous tilapia research, indicating that it is probably safe to ingest just the edible flesh of tilapia even when fed diets contaminated with a somewhat high AFB1 level [57, 58]. Supplementation with a S. cerevisiae–based product significantly reduced AFB1 accumulation in the liver, while silicate did not as compared to the AFB1-intoxicated group. This might be related to yeast’s involvement in improving liver function and maintaining hepatic cell integrity, which enhances AFB1 metabolism in liver tissue [47]. For the protection of human beings, detailed knowledge of the bioaccumulation of aflatoxins and their metabolites in aquatic species is required. Consequently, there is a need for scientific studies linking the amounts of AFB1 in the diet to the quantities of fish tissue intended for human consumption.
Serum protein concentrations in fish vary based on the species, age, and health of the fish. Healthy fish have greater blood protein concentrations than unhealthy fish [59]. Stressful environmental factors, such as high temperatures or low oxygen levels, can also alter blood protein concentrations in fish [60]. The gamma area, mostly made up of antibodies of the IgG type, is the region that receives the most attention in the development of serum protein ionophoresis [61]. Many conditions, such as connective tissue disorders, liver cirrhosis, and chronic infections (granulomatous diseases), may cause an increase in the gamma-globulin zone [62]. In this study, AFB1 poisoning reduced total blood protein and albumin levels while increasing gamma globulin levels (Table 4, Figs. 2 and 3), indicating liver tissue injury [63]. Normal levels of total protein, albumin, and even globulin fractions were found in yeast and silicate-supplemented groups, indicating a positive impact on the liver tissue, health, and its function.
Liver enzyme activity (AST and ALT) was markedly increased in the case of the AFB1-supplemented group and returned to normal levels with yeast supplementation. Expectedly, previously mentioned proof of liver injury revealed after AFB1 exposure might contribute to releasing hepatic enzymes (AST, ALT, and ALP) in the blood circulation, raising their serum levels. Similarly, Nile tilapia [57], sea bass (Dicentrarchus labrax) [53], turbot [49], and gibel carp [54] intoxicated with AFB1 revealed deteriorated secretion of AST and ALT. Further, Eraslan et al. [64] showed considerable hepatocellular deterioration together with elevated hepatic enzyme activity, demonstrating a severe impairment of liver function following AFB1 intoxication in adult Wistar albino rats. In this study, the normal levels of liver enzyme activity demonstrated in the case of the yeast supplementation group may be due to the impact of yeast and its different components (mannan-oligosaccharide and β-glucan) on hepatocytes integrity and health. This supports earlier studies that found dietary S. cerevisiae dramatically improved liver health and function [65,66,67]. Dietary AFB1 was demonstrated to cause renal damage, which may entail inflammation, cell necrosis, and toxicosis based on the biochemical measures in this study that showed higher serum creatinine and urea concentrations.
Together with those mentioned above, the current findings highlighted the adverse effects of AFB1 on liver and spleen histomorphology of Nile tilapia, showing clear cell type preneoplastic foci, loss of regular structure of hepatic cells, and depleted lymphocytes and lacked a melano-macrophage core in their spleen [28]. After S. cerevisiae supplementation, these adverse effects were successfully alleviated, confirming the S. cerevisiae’s positive benefits on the health of the liver’s tissues, hepatocytes, and fish spleen. This histologically positive yeast effect on liver and spleen histomorphology is a marker of improved antioxidative status of Nile tilapia following supplementation with S. cerevisiae–based product (MiaMyco-Fit) as narrated by previous studies [28, 68,69,70,71,72]. In this regard, Pinheiro et al. [73] also reported that tambaqui (Colossoma macropomum) intoxicated with AFB1 exhibited deteriorated liver histological features; however, dietary S. cerevisiae relieved the negative impacts of AFB1 on the liver tissue. AFB1 is metabolized, detoxified, and/or conjugated with nucleic acids and proteins in the liver, which is its target organ [74]. The liver, muscle, and other edible animal tissues have a certain amount of aflatoxin that may accumulate over time without causing any alterations [75]. Numerous studies have shown that animals exposed to AFB1 have residues in their tissues that induce negative health consequences when consumed [28, 53, 76]. In the current study, there were no measurable residual amounts of AFB1 in the muscles of any group. It was shown that Nile tilapia fed diets containing AFB1 alone, without treatment, had significant residual quantities of the toxin in their livers. This finding is consistent with other studies on tilapia exposed to long-term dietary aflatoxin [57]. However, adding S. cerevisiae significantly reduced those levels, whereas silicate did not. This result is similar to previous research that gave broiler chicken liver diets containing AFB1 (100 g/kg) and the yeast Pichia kudriavzevii (0.1%); there was a drop in the residual levels of AFB1 [44].
Oxidative stress is a potential danger factor for livestock development because it can produce large amounts of reactive oxygen species (ROS), resulting in oxidant activity that surpasses antioxidant neutralization capacities and impaired antioxidant system effectiveness [77, 78]. Malondialdehyde (MDA), lysozyme, glutathione peroxidase (GPX), and catalase activity (CAT) in Nile tilapia serum were examined in the current study using ELISA. It was discovered that MDA was considerably higher and that lysozyme, GPX, and CAT were significantly reduced in the group that had received AFB1 without treatments. MDA is a byproduct of the peroxidation of polyunsaturated fatty acids. It has been employed as a biomarker to assess oxidative stress [79, 80]. The increased MDA activity indicates that Nile tilapia given AFB1-contaminated feed are under considerable oxidative stress [81]. Furthermore, given an aflatoxicated diet with yeast and silicate administration, Nile tilapia had lower MDA levels that were substantially identical to the control group. Many studies have demonstrated that S. cerevisiae is a practical, viable, and low-cost tool for minimizing oxidative stress, is one of the potential approaches to lowering the risk associated with the presence of mycotoxins in feedstuffs, and can be regarded as a biological detoxifier [22, 25, 82,83,84].
Catalase is an essential antioxidant enzyme that plays a vital role in the H2O2 scavenging process by converting H2O2 to H2O and O2 [85]. The reduced CAT level in the AFB1-fed group without treatments indicates the negative impact of AFB1 on the antioxidant defense system. Nile tilapia–fed AFB1 supplemented diet with S. cerevisiae–based product succeeded in relieving the reduced effect on CAT activity even more than the silicate group. In order to diminish the hydrogen peroxide’s adverse effects, the intracellular antioxidant enzyme glutathione peroxidase-1 (GPx-1) transforms superoxide anion radicals to hydrogen peroxide, protecting cells from oxidative damage [86]. Similarly, AFB1 resulted in a lower activity of GPX in Nile tilapia. In contrast, S. cerevisiae and silicate have improved GPX levels, indicating the positive effects of biological and chemical detoxifiers used in this study on the Nile tilapia antioxidant system. In line with the present study, AFB1 exposure induced oxidative damage in Nile tilapia [87], northern snakehead (Channa argus) [88], and thinlip grey mullet [38], while supplementary lipopolysaccharides and probiotics mitigated AFB1-negative impacts on the antioxidative capacity in Nile tilapia [87] and thinlip grey mullet [38].
Lysozyme is a vital enzyme of leucocytic origin that is a crucial component of the innate immune system’s defense against microbial invasion (bacteria, viruses, and fungi) [89]. Hereby, AFB1 demonstrated a reduction in the lysozyme secretion, which directly impacts Nile tilapia’s immune status. This negative impact was relieved significantly after supplementation with S. cerevisiae and silicate-based products. The improved antioxidative and immune status previously mentioned in the case of yeast administration might be related to the cell components of S. cerevisiae since the cell wall is mainly made up of an inner layer of β-glucans and chitin and an outer layer of highly glycosylated mannoproteins, which have a substantial influence on toxin adsorption efficacy in S. cerevisiae [82]. In addition, silicate has been recorded as a potent toxin adsorbent in several investigations, and the favorable impacts displayed on antioxidation, and immunological boosting mechanisms are because of the silicate capacity in the mycotoxin adsorption process [90,91,92,93,94,95].
Conclusion
In the present study, the effect of aflatoxin on Nile tilapia was investigated. Further, the protective influence of the biological and chemical treatments against the toxic action of AFB1 was also estimated. The AFB1 drastic effects on growth, survivability, and immunity of Nile tilapia were demonstrated. The biological treatment (S. cerevisiae) has significantly decreased the adverse effects of AFB1 on Nile tilapia throughout, supporting the hepatocytes integrity more than the silicate-treated group.
Availability of Data and Materials
The authors confirm that the data supporting the findings of this work are available within the article. Raw data that supports the findings are available upon reasonable request.
References
Dawood MAO et al (2016) Probiotics as an environment-friendly approach to enhance red sea bream, Pagrus major growth, immune response and oxidative status. Fish Shellfish Immunol 57:170–178
Tacon AG, Metian M (2013) Fish matters: importance of aquatic foods in human nutrition and global food supply. Rev Fish Sci 21(1):22–38
Ludwig A, Boller T (1990) A method for the study of fungal growth inhibition by plant proteins. FEMS Microbiol Lett 69(1–2):61–66
Schrödter R (2004) Influence of harvest and storage conditions on trichothecenes levels in various cereals. Toxicol Lett 153(1):47–49
Alshannaq A, Yu J-H (2017) Occurrence, toxicity, and analysis of major mycotoxins in food. Int J Environ Res Public Health 14(6):632
Marchese S et al (2018) Aflatoxin B1 and M1: biological properties and their involvement in cancer development. Toxins 10(6):214
Rodríguez-Cervantes C et al (2010) Aflatoxin B1 and its toxic effects on immune response of teleost fishes: a review. World Mycotoxin J 3(2):193–199
Fallah A et al (2014) Mycoflora, aflatoxigenic strains of Aspergillus section Flavi and aflatoxins in fish feed. Quality Assurance and Safety of Crops & Foods 6(4):419–424
Ayyat MS et al (2018) Effect of some safe feed additives on growth performance, blood biochemistry, and bioaccumulation of aflatoxin residues of Nile tilapia fed aflatoxin-B1 contaminated diet. Aquac 495:27–34
Oliveira M, Vasconcelos V (2020) Occurrence of mycotoxins in fish feed and its effects: a review. Toxins 12(3):160
Zhou R et al (2019) Clinical features of aflatoxin B1-exposed patients with liver cancer and the molecular mechanism of aflatoxin B1 on liver cancer cells. Environ Toxicol Pharmacol 71:103225
Eberl G, Lochner M (2009) The development of intestinal lymphoid tissues at the interface of self and microbiota. Mucosal Immunol 2(6):478–485
Bedoya-Serna CM et al (2018) Effects of dietary aflatoxin B1 on accumulation and performance in matrinxã fish (Brycon cephalus). PLoS ONE 13(8):e0201812
Michelin EC et al (2017) Carryover of aflatoxins from feed to lambari fish (Astyanax altiparanae) tissues. Food Additives & Contaminants: Part A 34(2):265–272
Jard G et al (2011) Review of mycotoxin reduction in food and feed: from prevention in the field to detoxification by adsorption or transformation. Food Additives & Contaminants: Part A 28(11):1590–1609
He J, Zhou T (2010) Patented techniques for detoxification of mycotoxins in feeds and food matrices. Recent Pat Food Nutr Agric 2(2):96–104
Ji C, Fan Y, Zhao L (2016) Review on biological degradation of mycotoxins. Anim Nutr 2(3):127–133
Zhu Y et al (2017) Strategies and methodologies for developing microbial detoxification systems to mitigate mycotoxins. Toxins 9(4):130
Essa SS et al (2017) Modulating effect of MgO-SiO2 nanoparticles on immunological and histopathological alterations induced by aflatoxicosis in rats. Toxicon 140:94–104
Younes M et al (2018) Re-evaluation of silicon dioxide (E 551) as a food additive. Efsa j 16(1):e05088
Huang W et al (2019) Effect of compound probiotics and mycotoxin degradation enzymes on alleviating cytotoxicity of swine jejunal epithelial cells induced by aflatoxin B1 and zearalenone. Toxins (Basel) 11(1)
Liu L, Xie M, Wei D (2022) Biological detoxification of mycotoxins: current status and future advances. Int J Mol Sci 23(3)
Guan Y et al (2021) Aflatoxin detoxification using microorganisms and enzymes. Toxins 13(1):46
Luo Y et al (2020) Complicated interactions between bio-adsorbents and mycotoxins during mycotoxin adsorption: current research and future prospects. Trends Food Sci Technol 96:127–134
Shetty PH, Jespersen L (2006) Saccharomyces cerevisiae and lactic acid bacteria as potential mycotoxin decontaminating agents. Trends Food Sci Technol 17(2):48–55
Pizzolitto RP et al (2013) Evaluation of Saccharomyces cerevisiae as an antiaflatoxicogenic agent in broiler feedstuffs. Poult Sci 92(6):1655–1663
Zhang Z et al (2019) Physical adsorption of patulin by Saccharomyces cerevisiae during fermentation. J Food Sci Technol 56(4):2326–2331
Mahfouz ME, Sherif AH (2015) A multiparameter investigation into adverse effects of aflatoxin on Oreochromis niloticus health status. J basic appl zool 71:48–59
Bulut M et al (2014) Evaluation of dietary protein and lipid requirements of two-banded seabream (Diplodus vulgaris) cultured in a recirculating aquaculture system. Aquacult Int 22(3):965–973
AOAC (2007) Method 2007–04. Association of Official Analytical Chemists. Association of Official Analytical Chemists.Washington, DC
Reitman S, Frankel S (1957) A colorimetric method for the determination of serum glutamic oxalacetic and glutamic pyruvic transaminases. Am J Clin Pathol 28(1):56–63
de los Santos FS et al (2007) Gastrointestinal maturation is accelerated in Turkey poults supplemented with a mannan-oligosaccharide yeast extract (Alphamune)1. Poult Sci 86(5):921–930
Ohkawa H, Ohishi N, Yagi K (1979) Assay for lipid peroxides in animal tissues by thiobarbituric acid reaction. Anal Biochem 95(2):351–358
Paglia DE, Valentine WN (1967) Studies on the quantitative and qualitative characterization of erythrocyte glutathione peroxidase. J Lab Clin Med 70(1):158–169
Aebi H (1984) Catalase in vitro. Methods Enzymol 105:121–126
Vardali S et al (2023) Recent advances in mycotoxin determination in fish feed ingredients. Molecules 28(6):2519
Kumar P et al (2007) Aflatoxins: a global concern for food safety, human health and their management. Front Microbiol 7
Khalafalla MM et al (2022) Dietary lactobacillus acidophilus ATCC 4356 relieves the impacts of aflatoxin B1 toxicity on the growth performance, hepatorenal functions, and antioxidative capacity of thinlip grey mullet (Liza ramada)(Risso 1826). Probiotics and Antimicrobial Proteins 14(1):189–203
Gonçalves RA et al (2018) Aflatoxin B 1 (AFB 1) reduces growth performance, physiological response, and disease resistance in Tra catfish (Pangasius hypophthalmus). Aquacult Int 26:921–936
Ghafarifarsani H, Kachuei R, Imani A (2021) Dietary supplementation of garden thyme essential oil ameliorated the deteriorative effects of aflatoxin B1 on growth performance and intestinal inflammatory status of rainbow trout (Oncorhynchus mykiss). Aquac 531
Alinezhad S et al (2017) Effects of nanostructured zeolite and aflatoxin B1 in growth performance, immune parameters and pathological conditions of rainbow trout Oncorhynchus mykiss. Fish Shellfish Immunol 70:648–655
Selim KM, El-hofy H, Khalil RH (2014) The efficacy of three mycotoxin adsorbents to alleviate aflatoxin B 1-induced toxicity in Oreochromis niloticus. Aquacult Int 22:523–540
Zeng Z-Z et al (2019) Dietary aflatoxin B1 decreases growth performance and damages the structural integrity of immune organs in juvenile grass carp (Ctenopharyngodon idella). Aquac 500:1–17
Magnoli AP et al (2017) Use of yeast (Pichia kudriavzevii) as a novel feed additive to ameliorate the effects of aflatoxin B1 on broiler chicken performance. Mycotoxin Res 33:273–283
Patil R, Degloorkar N, Pawar P (2017) Ameliorating effects of Bantox® on clinical manifestation and growth performance of broiler chicken fed with ochratoxin A. J poult sc technol 5(3):22–27
Fadl SE et al (2020) Trial for reduction of ochratoxin A residues in fish feed by using nano particles of hydrated sodium aluminum silicates (NPsHSCAS) and copper oxide. Toxicon 184:1–9
Lin Z et al (2023) Protective effects of yeast extract against alcohol-induced liver injury in rats. Front Microbiol 14:1217449
Rahman AN, Abdellatief SA, Mahboub HH (2017) Protection of Nile tilapia, Oreochromis niloticus from aflatoxin B1 toxicity by dietary supplementation with Fennel essential oil and Saccharomyces cerevisiae. Egypt J Aquat Res 43(3):235–240
Yang J et al (2020) The assessment of diet contaminated with aflatoxin B1 in juvenile turbot (Scophthalmus maximus) and the evaluation of the efficacy of mitigation of a yeast cell wall extract. Toxins 12. https://doi.org/10.3390/toxins12090597
Sue P, Michon R, Meeinis J (1956) Metabolism of silica and silicates injected intravenously into animals, traced by weans of 31Si. Compte Rendu de l’Academie des Sciences 243(22):1809–1811
Plakas SM et al (1991) Tissue disposition and excretion of 14C-labelled aflatoxin B1 after oral administration in channel catfish. Food Chem Toxicol 29(12):805–808
Hussain M et al (1993) Effect of aflatoxin-contaminated feed on morbidity and residues in walleye fish. Vet Hum Toxicol 35(5):396–398
El-Sayed YS, Khalil RH (2009) Toxicity, biochemical effects and residue of aflatoxin B1 in marine water-reared sea bass (Dicentrarchus labrax L.). Food Chem Toxicol 47(7):1606–1609
Huang Y et al (2011) Response and recovery of gibel carp from subchronic oral administration of aflatoxin B1. Aquac 319(1):89–97
Huang Y et al (2014) Effect of dietary aflatoxin B1 on growth, fecundity and tissue accumulation in gibel carp during the stage of gonad development. Aquac 428–429:236–242
Guengerich FP et al (1998) Activation and detoxication of aflatoxin B1. Mutation Research/Fundamental and Molecular Mechanisms of Mutagenesis 402(1–2):121–128
Deng, S-X et al (2010) Toxic effects and residue of aflatoxin B1 in tilapia (Oreochromis niloticus×O. aureus) during long-term dietary exposure. Aquac 307(3):233–240
Lim H-A et al (2001) Contamination of palm kernel meal with Aspergillus flavus affects its nutritive value in pelleted feed for tilapia. Oreochromis mossambicus Aquac Res 32(11):895–905
Nabi N, Ahmed I, Wani GB (2022) Hematological and serum biochemical reference intervals of rainbow trout, Oncorhynchus mykiss cultured in Himalayan aquaculture: Morphology, morphometrics and quantification of peripheral blood cells. Saudi J Biol Sci 29(4):2942–2957
Esmaeili M (2021) Blood performance: a new formula for fish growth and health. Biology (Basel) 10(12)
Tripathy S (2012) The role of serum protein electrophoresis in the detection of multiple myeloma: an experience of a corporate hospital. J Clin Diagn Res 6(9):1458–1461
Kyle RA (1999) Sequence of testing for monoclonal gammopathies. Arch Pathol Lab Med 123(2):114–118
George ED, Sadovsky R (1999) Multiple myeloma: recognition and management. Am Fam Physician 59(7):1885–1892
Eraslan G et al (2017) The effects of diosmin on aflatoxin-induced liver and kidney damage. Environ Sci Pollut Res Int 24(36):27931–27941
Xia R et al (2022) Effects of dietary Saccharomyces cerevisiae on growth, intestinal and liver health, intestinal microbiota and disease resistance of channel catfish (Ictalurus punctatus). Aquac Rep 24
Feng Z et al (2022) Yeast culture improved the growth performance, liver function, intestinal barrier and microbiota of juvenile largemouth bass (Micropterus salmoides) fed high-starch diet. Fish Shellfish Immunol 120:706–715
Engstad RE, Robertsen B, Frivold E (1992) Yeast glucan induces increase in lysozyme and complement-mediated haemolytic activity in Atlantic salmon blood. Fish Shellfish Immunol 2(4):287–297
Mohammady EY et al (2023) Appraisal of fermented wheat bran by Saccharomyces cerevisiae on growth, feed utilization, blood indices, intestinal and liver histology of Nile tilapia. Oreochromis niloticus, Aquaculture, p 739755
Sönmez AY (2017) Evaluating two different additive levels of fully autolyzed yeast, Saccharomyces cerevisiae, on rainbow trout (Oncorhynchus mykiss) growth performance, liver histology and fatty acid composition. Turk J Fish Aquat Sci 17(2):379–385
Chen X-Q et al (2019) Effects of dietary hydrolyzed yeast (Rhodotorula mucilaginosa) on growth performance, immune response, antioxidant capacity and histomorphology of juvenile Nile tilapia (Oreochromis niloticus). Fish Shellfish Immunol 90:30–39
Zaineldin AI et al (2021) Singular effects of Bacillus subtilis C-3102 or Saccharomyces cerevisiae type 1 on the growth, gut morphology, immunity, and stress resistance of red sea bream (Pagrus major).
Espinosa C, Esteban MÁ (2020) Effect of dietary supplementation with yeast Saccharomyces cerevisiae on skin, serum and liver of gilthead seabream (Sparus aurata L). J Fish Biol 97(3):869–881
Pinheiro R et al (2021) Effect of Saccharomyces cerevisiae addition to feed contaminated with aflatoxin B1 on the health and performance indices of tambaqui (Colossoma macropomum) fingerlings. World Mycotoxin J 14(3):389–400
Liew WP, Mohd-Redzwan S (2018) Mycotoxin: its impact on gut health and microbiota. Front Cell Infect Microbiol 8:60
Magnoli AP et al (2011) Effect of low levels of aflatoxin B on performance, biochemical parameters, and aflatoxin B in broiler liver tissues in the presence of monensin and sodium bentonite. Poult Sci 90(1):48–58
Naiel MAE, Ismael NEM, Shehata SA (2019) Ameliorative effect of diets supplemented with rosemary (Rosmarinus officinalis) on aflatoxin B1 toxicity in terms of the performance, liver histopathology, immunity and antioxidant activity of Nile Tilapia (Oreochromis niloticus). Aquac 511
Ponnampalam EN et al (2022) The importance of dietary antioxidants on oxidative stress, meat and milk production, and their preservative aspects in farm animals: antioxidant action, animal health, and product quality—invited review. Animals 12(23):3279
Bhattacharyya A et al (2014) Oxidative stress: an essential factor in the pathogenesis of gastrointestinal mucosal diseases. Physiol Rev 94(2):329–354
Lefèvre G et al (1998) Evaluation of lipid peroxidation by measuring thiobarbituric acid reactive substances. Ann Biol Clin (Paris) 56(3):305–319
Draper HH, Hadley M (1990) Malondialdehyde determination as index of lipid peroxidation. Meth Enzymol 186:421–431
Shen HM et al (1994) Aflatoxin B1-induced lipid peroxidation in rat liver. Toxicol Appl Pharmacol 127(1):145–150
Piotrowska M, Masek A (2015) Saccharomyces cerevisiae cell wall components as tools for ochratoxin a decontamination. Toxins (Basel) 7(4):1151–1162
Kabak B, Dobson AD, Var I (2006) Strategies to prevent mycotoxin contamination of food and animal feed: a review. Crit Rev Food Sci Nutr 46(8):593–619
Petruzzi L et al (2014) In vitro removal of ochratoxin A by two strains of Saccharomyces cerevisiae and their performances under fermentative and stressing conditions. J Appl Microbiol 116(1):60–70
Hong SY et al (2013) Evidence that a transcription factor regulatory network coordinates oxidative stress response and secondary metabolism in aspergilli. Microbiologyopen 2(1):144–160
Lubos E, Loscalzo J, Handy DE (2011) Glutathione peroxidase-1 in health and disease: from molecular mechanisms to therapeutic opportunities. Antioxid Redox Signal 15(7):1957–1997
Abd El-Kader MF et al (2021) Ameliorative effect of dietary lipopolysaccharides on Oreochromis niloticus juveniles submitted to aflatoxin B1-induced oxidative stress and bacterial challenge. Aquac Res 52(8):3660–3676
Li M et al (2022) Dietary aflatoxin B1 caused the growth inhibition, and activated oxidative stress and endoplasmic reticulum stress pathway, inducing apoptosis and inflammation in the liver of northern snakehead (Channa argus). Sci Total Environ 850:157997
Ferraboschi P, Ciceri S, Grisenti P (2021) Applications of lysozyme, an innate immune defense factor, as an alternative antibiotic. Antibiotics (Basel) 10(12)
Hedayati M et al (2014) Commercial broilers exposed to aflatoxin b1: efficacy of a commercial mycotoxin binder on internal organ weights, biochemical traits and mortality. Int J Agric For 4(5):351–358
Whitlow LW (2006) Evaluation of mycotoxin binders. InProceedings of the 4th Mid-Atlantic Nutrition Conference
Holanda DM, Kim SW (2021) Mycotoxin occurrence, toxicity, and detoxifying agents in pig production with an emphasis on deoxynivalenol. Toxins 13(2):171
Al-Afifi S, Manal I, Bayomi A (2018) Biochemical effects of Saccharomyces cerevisiae (biological product) and hydrated sodium calcium alimono-silicate” HSCAS”(chemical compound) as anti-aflatoxin in chicken rations. Anim Health Res Rev 6(1):19–38
Di Gregorio MC et al (2014) Mineral adsorbents for prevention of mycotoxins in animal feeds. Toxin Reviews 33(3):125–135
Hassaan MS et al (2020) Nano-zeolite efficiency to mitigate the aflatoxin B1 (AFB1) toxicity: effects on growth, digestive enzymes, antioxidant, DNA damage and bioaccumulation of AFB1 residues in Nile tilapia (Oreochromis niloticus). Aquac 523
Funding
Open access funding provided by The Science, Technology & Innovation Funding Authority (STDF) in cooperation with The Egyptian Knowledge Bank (EKB).
Author information
Authors and Affiliations
Contributions
All authors contributed to the study's conception and design. Material preparation, data collection, and analysis were performed by Amr I. Zaineldin, Mahmoud A.O. Dawood, Ehab Elsebaey, Ola A. Habouta, and Walied S. Abdo. The first draft of the manuscript was written by Amr Zaineldin, Mahmoud A.O. Dawood, and Mohammed F. El Basuini. All authors commented on previous versions of the manuscript. All authors read and approved the final manuscript.
Corresponding author
Ethics declarations
Consent to Participate
All authors consent to participating in a study and have no objection to having their data published in a journal article.
Consent for Publication
Authors obtained consent from all individuals to publish their data prior to submitting their paper to a journal.
Conflict of Interest
The authors declare no competing interests.
Declaration of Generative AI in Scientific Writing
The authors disclose that they did not employ any AI technologies as part of the research process to assess and/or derive insights from data.
Additional information
Publisher's Note
Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Rights and permissions
Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons licence, and indicate if changes were made. The images or other third party material in this article are included in the article's Creative Commons licence, unless indicated otherwise in a credit line to the material. If material is not included in the article's Creative Commons licence and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this licence, visit http://creativecommons.org/licenses/by/4.0/.
About this article
Cite this article
Zaineldin, A.I., Elsebaey, E., Habotta, O.A. et al. Mitigating Aflatoxin B1-Induced Growth Impairment and Hepatic Stress in Nile Tilapia (Oreochromis niloticus): Comparative Efficacy of Saccharomyces cerevisiae and Silicate-Based Detoxifiers. Probiotics & Antimicro. Prot. (2024). https://doi.org/10.1007/s12602-023-10210-2
Accepted:
Published:
DOI: https://doi.org/10.1007/s12602-023-10210-2