key: cord-0686212-fivkx8yk
authors: Tawfeek, Shereen E.; Domouky, Ayat M.; Abdel-Kareem, Reham H.
title: Protective effect of vitamin C against ivermectin induced nephrotoxicity in different age groups of male wistar rats: bio-histopathological study
date: 2021-12-31
journal: Anat Cell Biol
DOI: 10.5115/acb.21.124
sha: 0461279f8f3ba74cefb4d4b9ac9d53f7df05a789
doc_id: 686212
cord_uid: fivkx8yk

Ivermectin (Ive) has exceedingly efficient against several microorganisms including viruses; therefore, it could help as a potential treatment of COVID-19. Because of increasing consumption of ivermectin and vitamin C (Vit.C) in hope to treat COVID-19, and because of ivermectin nephrotoxic effects have not been fully clarified especially in juvenile age, it was conducted to examine the histopathological and biochemical effects of ivermectin on adult and juvenile kidneys, and to assess the possible protective role of Vit.C against this potential toxicity. Rats were divided to 4 subgroups (Control subgroup, Vit.C subgroup, Ive subgroup, and Vit.C+Ive subgroup), 1 week after 4 doses of ivermectin (0.4 mg/kg Ive±1.25 mg/kg Vit.C), blood samples obtained for assessment of kidney function test, part of kidneys prepared for determination of matrix metalloproteinase-9 and antioxidant enzymes essay. Other parts prepared for histopathological and ultrastructural examination. Results showed that administration of ivermectin led to attenuation in kidney function and in activities of the antioxidant enzymes and increase in matrix metalloproteinase-9 activity. In addition, there were histological damages (shrunken glomeruli, widened urinary space, cytoplasmic vacuolation and pyknotic nuclei with epithelial exfoliation, extravasated blood, and mononuclear cell infiltration) and immunohistochemistry revealed increase in percentage of Bax proapoptotic protein expression. Also, ultrastructure examination showed alteration in cell architecture. All these changes were more obvious in juvenile group while co-administration of Vit.C led to significant protection more in adult group. In conclusion, Ivermectin should be used cautiously especially in juvenile age, and co-administration of Vit.C is highly recommended.

Ivermectin offers many potential effects to treat a range of diseases, with its antimicrobial, antiviral, and anti-cancer properties as a marvel drug. It is exceedingly efficient against several microorganisms including some viruses; therefore it could help as a prospective candidate in the treatment of a broad range of viruses including COVID-19 alongside other types of single-stranded RNA viruses [6] . It interferes with nerve and muscle function of helminths and insects by binding to their glutamate-gated chloride channels driving them to open, increasing chloride ions flow, hyper-polarizing the cell membranes, paralyzing the affected tissue and finally killing them. In mammals (including humans) these channels are present only in brain and spinal cord and not affected by Ive because it cannot cross the blood brain barrier [7] .

Added to having antiparasitic and antiviral effects, ivermectin triggers immunomodulation in the host, inhibiting the proliferation of cancer cells, and regulating glucose and cholesterol, some of these effects may be secondary to toxic effects on cells [8] . Recent studies demonstrated that ivermectin has antiviral action against the SARS-CoV-2 clinical isolate in vitro, with a single dose able to control viral replication within 24-48 hours in our system [5] . This is likely through inhibiting IMPα/β1-mediated nuclear import of viral proteins for other RNA viruses, confirmation of this mechanism in the case of SARS-CoV-2, and if given to patients early in infection, could help to limit the viral load, prevent severe disease progression and limit person to person transmission [9] . Moreover, Shoumann et al. [10] , reported that ivermectin is suggested to be a promising, effective and safe chemoprophylactic drug in management of With increasing extensive demand to fight COVID-19, it is important to search about ivermectin toxic effect on several body organs. Ivermectin can enter the body orally and reach the blood and organs as the liver and kidney for metabolism. Even though it has been established as a safe and nontoxic medication for mammals [11] , considering that it is a xenobiotic for the body, it probably has some effects on the oxidative stress system of the mammalian. Since xenobiotic is unknown to the host, it is expected to cause adverse effects such as toxicity, allergic response, and cancer [12] . Moreover, ivermectin has stimulated oxidative stress in the tissue of North African catfish [13] . Common adverse effects of ivermectin such as headache, pruritus, muscle pain, cough, dyspnea, nausea, vomiting, diarrhea, blurred vision, postural hypotension, and confusion were reported by clinical trials [14, 15] . Also, it may cause nephropathy [16] , psychiatric disorders [17] , hepatic disorders [18] , and multiorgan dysfunction syndrome [19] .

Several studies showed that antioxidant substances guard cells against harmful effects of several environmental agents [20] . Vitamins, as antioxidants may preserve cells membrane function including ion transport and membrane flexibility, they may also prevent the release of Fe2+ and Mg2+ from their binding protein possibly decrease the rate of lipid peroxidation [21] . Ascorbic acid (AA) "vitamin C" is an important adjunctive therapy for respiratory infection, sepsis and COVID-19 [22] . It is a highly water soluble and acts as an efficient reducing agent [23, 24] . Vitamin C is hydrophilic and a most significant free radical scavenger in extracellular fluids, trapping radicals in the aqueous phase, and protecting bio-membranes from oxidative injury [25] . While most mammals are capable of synthesizing vitamin C in their liver or kidneys, the majority of primates (including humans), guinea pigs and some Birds and fish cannot synthesize it and must draw it from their diet. This is due to a genetic mutation that occurred 40 million years ago, blocking the transformation of glucose into AA [26] .

Based on over-increasing consumption of ivermectin and vitamin C in hope to treat COVID-19 with emerging of questions about safety of its use in contact or infected children, and because of ivermectin nephrotoxic effects have not been fully clarified especially in juvenile age, this present study was conducted to examine the histopathological and biochemical effects of ivermectin on both adult and juvenile kidneys in male wistar rats, and to assess the possible protective role of vitamin C against this potential toxicity.

Ivermectin Ivermectin (22,23-dihydroavermectin B) was purchased from Unipharma Egypt Company, El Obour City, Egypt as tablets each tab-6 mg. Suspension of ivermectin was dissolved in saline to make 0.2 solution.

Vitamin C Vitamin C was purchased from Chemical Industries Development (CID) Company, Al-Harm, Giza, Egypt as tablets, each tab-500 mg was dissolved in water to make solution.

Eighty animals from 2 age groups (newborn and adults) were used in this study 40 rats each. Each group was divided randomly to 4 subgroups 10 rats each. They were obtained from the animal house, Faculty of Medicine, Zagazig University. The rats were housed in separate cages (2 rats per each cage) and maintained under standard laboratory and environmental conditions with standard rat chow. All animal experiments were carried out in accordance with relevant guidelines and regulations of the Institutional Animal Care and Use Committee, Zagazig University (ZU-IACUC committee), approval number ZU-IACUC/3/F/84/2020.

The animal groups classified as following: juvenile group (40 newborn male rats aged 2 days weighted 9-12 g) and adult group (40 adult rats aged 3 months and weighted 220-250 g) each group was randomly divided to 4 subgroups: control subgroup of each group was received 0.5 cm physiological saline, Vit.C subgroup of each group received 1.25 mg/kg vitamin C [27] , Ive subgroup of each group received 0.4 mg/kg ivermectin [28] and Vit.C+Ive subgroup of each group: received 0.4 mg/kg ivermectin in concomitant with 1.25 mg/kg vitamin C. The treatments were given orally once a week for four consecutive weeks to the animals in all subgroups using gastric intubations.

One week after the last dose of ivermectin (the newborn rats become juvenile about one-month age weighted 70-90 g), blood samples were obtained for assessment of biochemical markers of kidney from all groups, body weight was measured before sacrifice. Moreover, the kidneys were harvested and weighted and immediately immersed and fixed in buffered formalin 10%, (relative kidney weight was calculated "kidney weight/body weight %"). After 24 hours of fixation the kidneys were further carefully dissected, excised and parts of it prepared for histopathological examinations and ultrastructural study. Other parts were dissected, washed with ice-cold saline, frozen in liquid nitrogen (170°C) and kept at -80°C for PCR and homogenate tissue analysis.

Blood samples were collected, under complete aseptic conditions, from the rat retro-orbital venous plexus by means of micro-capillary glass tubes. Blood was allowed to coagulate at room temperature and then samples were centrifuged at 4,000 rpm for 20 minutes using a cooling centrifuge (Sigma 3-30 k; Sigma-Aldrich, St. Louis, USA). The clear serum layer was separated and stored at -80°C biomarkers. Serum creatinine concentrations (SCr) (mg/ dl), blood urea nitrogen (BUN) (mg/dl), were measured spectrophotometrically.

Part of kidneys were separated instantly and homogenized in a phosphate buffer (pH 7.6), centrifuged at 20,000 rpm, 4°C for 2 hours to obtain a soluble salt part. Re-extraction of the pellets was carried out to get a soluble detergent part. The supernatant was collected and stored at −20°C. Protein concentrations were determined by the Bradford assay with Bovine serum albumin as standard (0.05-1.00 mg/ml) [29] .

Total antioxidant capacity (TAC) of kidney homogenate was evaluated using FRAP assay. The FRAP reagent was prepared as a mixture of 5 ml of 10 mM of 2,4,6-tris (2-pyridyl)s-triazine in 50 ml of 0.1 M acetate buffer (pH 3.6) and 5 ml of FeCl3 (20 mM) in HCl (40 mM). Then, prepared FRAP reagent was incubated at 37°C for 15 minutes, and 200 ml of a kidney homogenate was mixed with 1.5 ml of the FRAP reagent and incubated for 15 minutes. The mixture was centrifuged at 12,000 rpm/15 min. Absorbance of the supernatant and standard sample was measured at 593 nm against blank [30] .

Catalase assay (CAT) was performed according to Maehly and Chance [31] . One unit of catalase activity was defined as an absorbance change of 0.01 as units/min (U/min), superoxide dismutase assay (SOD) was performed according to Kakkar et al. [32] . Results are expressed in units/mg protein (U/mg protein), and glutathione peroxidase assay (GPx) was performed according to Mohandas et al. [33] . Enzyme activity was calculated as nmol NADPH oxidized/ min/mg protein using a molar extinction coefficient of 6.22×103 M -1 cm -1 , results are expressed in nmol/mg protein.

Determination the reactive oxygen species (ROS) content in kidney tissues: ROS test kit (Beyotime, Shanghai, China) was used to determinate the ROS content in kidney homogenates. ROS formation was quantified and expressed as pmol DCF/min/mg protein.

Total RNA was extracted from kidney tissue using SV Total RNA Isolation System (Promega, Madison, WI, USA) and quantified spectrophotometrically at 260/280 nm. Residual www.acbjournal.org https://doi.org/10.5115/acb. 21.124 genomic DNA was removed by incubating RNA with Rnasefree DNase I. The total extracted RNA was reverse transcribed into complementary DNA (cDNA) using RTPCR kit (Stratagene, USA). Random hexamers (primers) for MMP-9 (GenBank accession number NM_009660.3 gene was used for reverse transcription of RNA. Using Forward primer: 50 -CACAGACAGCCTTCTGCAAC-30, reverse primer: 50 -CATTTCCCACAGCCTTGAAT-30 in 60°C, product size 141 bp. Relative changes in gene expression levels of samples to control were determined using the comparative (2DDCt) method [34, 35] .

Kidney specimens were embedded in paraffin after fixation in 10% formalin solution in normal saline. Blocks were sectioned at 4-5 microns then they were collected on glass slides, deparaffinized, and stained by Hematoxylin and Eosin for histopathological examination. Also, Periodic acid-Schiff (PAS) stain was used for the demonstration of polysaccharides content. The slides examined by the light electric microscope (LEICA ICC50 W), anatomy department, faculty of medicine, Zagazig University.

Image analysis software (ImageJ 1.36b; http://rsbweb.nih. gov/ij) was utilized to estimate histopathological findings by measuring the Cortex area (mm 2 ), areas of glomerulus (mm 2 ) and urinary space cross sectional (mm) in H&E kidneystained sections. Quantitative data were estimated in 5 different non-overlapped fields for the same slide of each animal, in each animal 5 slides were counted and a total number of 25 fields of each group were counted [36] .

Immunohistochemistry paraffin-embedded kidney sections (4-mm-thick) were f loated onto aminopropyltriethoxysilane-coated slides, deparaffinized with xylene and hydrated in graded series of ethanol. Immunohistochemical staining was performed using avidin-biotin peroxidase complex. Endogenous peroxidase was quenched with 3% hydrogen peroxide: methanol (1:1) for 30 minutes at room temperature. Staining of formalin-fixed tissues requires boiling of tissue sections in 10 mM citrate buffer, pH 6.0 for 20 minutes followed by cooling at room temperature for 20 minutes. The primary antibodies (mice polyclonal anti-Bax, Santa Cruz Biotechnology, Dallas, Texas, USA) were diluted (1:1,000) and added to the slides. Sections were washed twice for 5 minutes in phosphate-buffered saline (PBS), followed by the addition of appropriate secondary antibody (biotinylated goat anti-rabbit immunoglobulin G diluted to 1:500), followed by incubation with peroxidase-conjugated streptavidin diluted to 1:3,000 in PBS for 15 minutes. The peroxidase reaction was performed using 0.02% chromogen 3,30 diaminobenzidine tetrahydrochloride. Sections were then counterstained with hematoxylin, dehydrated and mounted in Canada balsam [37] . Image analysis software (ImageJ 1.36b, http://rsbweb.nih.gov/ij) was utilized to estimate Bax immunoreactivity in 5 different non-overlapped fields About 100 epithelial cells for the same slide of each animal, in each animal 5 slides were counted and a total number of 25 fields of each group were counted. The percentage of Bax positivity was calculated. 

Kidney specimens were fixed using 2.5% glutaraldehyde for 24-48 hours, followed by washing three to four times in phosphate buffer (pH 7.2-7.4). The specimens were then post-fixed in in a buffered solution of 1% osmium tetroxide for 2 hours, after that washed in a similar buffer four times for 20 minutes each. Fixed specimens were dried out in increasing concentrations of ethyl alcohol (30%, half, 70%, 90%, and 100%), cleared in two changes of propylene oxide and inserted in Epon resin. The pitch squares underwent a process of trimming to get rid of the surplus tissue. Ultrathin sections (60-90 nm thick) and illustrative fields of semithin sections were chosen and were cut with a diamond knife using a Reichert OMVs ultra microtome, mounted on copper frameworks. These semi-thin sections were subjected to double staining with uranyl acetate and lead citrate [38] . The grids were examined and photographed using using a transmission electron microscope (JEOL JEM-1010, Tokyo, Japan) at the Mycology and Regional Biotechnology Center, Al Azhar University for Boys, Cairo, Egypt. 

The collected biochemical and morphometric data was statistically analyzed using SPSS program (Statistical Package for Social Science) version 18.0. Descriptive statistics were given as mean±standard deviation (SD). Numbers with percentages (%) were used for nominal variables. One-way ANOVA were used to compare the mean values of different groups. Multiple comparisons were estimated by the least significant difference (LSD) test. Moreover, t-test was used to show significance between corresponding subgroups in the two study groups, a value of P<0.05 was statistically significant, a value of P<0.001 was highly statistically significant, and a value of P>0.05 was non-statistically significant.

Juvenile rats treated with ivermectin (Ive subgroup) showed a significant decrease in body weight and kidney weight compared with control and Vit.C subgroups, while kidney weight/body weight % remained insignificant difference. Consumption of vitamin C parallel with ivermectin in Vit.C+Ive subgroups led to partial protection from this weight loss. On the other hand, adult rats revealed significant difference in body weight and no significant difference neither in kidney weight nor kidney weight/body weight % between all subgroups (Table 1 , Fig. 1A-F) .

When comparing the percentage of change happened in corresponding Ive subgroups (from the control subgroup) in the two study groups, the juvenile rats exhibited more body weight loss (-15.3±2.5 vs -11.3±2.8 in adult), also more kidney weight loss (-18.4±0.5 vs -9.2±0.4 in adult). Vitamin C supplementation in Vit.C+Ive subgroups showed protective effect in both groups, but it was relatively less in juvenile group due to more effect of ivermectin at this young age ( Table 1 , Fig. 1G -I).

Kidney function test showed that rats treated with ivermectin (Ive subgroup) had a highly significant increase in the kidney function marker; SCr, BUN, as compared to control and Vit.C subgroups. Consumption of vitamin C parallel with ivermectin in juvenile rats led to partial protection from this deterioration, while in adult rats vitamin C led to nearly full protection from this deterioration. Accordingly, comparing of both Ive, subgroups the juvenile group showed more elevated kidney function marker however vitamin C gave better protection in adult group ( Table 2 , Fig. 2A, B ).

Measuring TAC as well as the activities of the antioxidant www.acbjournal.org enzymes CAT, SOD and GPx in the kidney tissues of different study subgroups in both juvenile and adult rats showed that administration of vitamin C alone led to increase in TAC and antioxidant enzymes activities, on the other hand, rats treated with ivermectin (Ive subgroups) displayed a highly significant decrease in the activities of the TAC, CAT, SOD, and GPx with significant increase in ROS. While consumption of vitamin C parallel with ivermectin in both Vit. C+Ive subgroups exhibited stability of oxidant/antioxidant activities near control group. Comparing juvenile and adult groups showed that juvenile rats had more decline in oxidants activity in treated group and less protected effect of vitamin C ( Table 2 , Fig. 2C -G).

PCR examination of samples obtained from different study subgroups had convincingly showed that matrix metalloproteinase 9 (MMP9) was statistically significantly higher in ivermectin treated subgroups compared to control which indicate basement membrane degradation as MMP9 has been regarded as one of the major enzymes responsible for basement membrane degradation. While consumption of vitamin C parallel with ivermectin exhibited partial stability against this degradation. Comparing juvenile and adult groups showed that adult rats had higher level of MMP9 in all subgroups ( Table 2 , Fig. 2H ).

H&E stained sections of control as well as Vit.C subgroups in both juvenile and adult rats showed nearly similar results with normal renal histology; corpuscles formed of a dense rounded glomerulus surrounded by a parietal layer of Bowman's capsule with the urinary space in-between, moreover, proximal convoluted tubules were lined with low columnar cells with spherical basal nuclei and distal convoluted tubules were lined with low cuboidal cells with rounded central nuclei (Fig. 3A-D) .

On other hand, sections of Ive subgroup of juvenile rats showed extensive renal damage with extremely shrunken glomeruli and a widened urinary space in-between, proximal and distal convoluted tubules were dilated, and their lining cells showed extensive cytoplasmic vacuolation with pyknotic nuclei, and also epithelial cell exfoliations were present, moreover, there were extensive extravasated blood and mononuclear cell infiltration (Fig. 3E, G) . Sections of Ive subgroup of adult rats showed less extensive renal damage with shrunken glomeruli and widened urinary space, fewer areas of extravasated blood and mononuclear cell infiltration, with also some of proximal and distal convoluted tubules are dilated and their lining cells showed pyknotic nuclei with some cytoplasmic vacuolation and epithelial cell exfoliations (Fig. 3F, H) .

Vit.C+Ive subgroups in both juvenile and adult rats showed improvement in the renal alterations. This improvement was more obvious in adult rats as the damage was less extensive than the juvenile ones. Some glomeruli were slightly shrunken with relatively wide renal space and there was few extravasated blood in both groups. Few tubules exhibit pyknotic nuclei with cytoplasmic vacuolation and epithelial cell exfoliation in juvenile group (Fig. 3I, J) .

The histopathological alterations were confirmed mor- sectional. Consumption of vitamin C parallel with ivermectin led to partial protection from these histopathological changes (Table 3 , Fig. 3K-O) .

PAS-stained sections of control as well as Vit.C subgroups in both juvenile and adult rats showed that, convoluted tu- 4A-D) . On other hand, sections of Ive subgroups revealed strong positive PAS reaction of thickened basement membrane of both Bowman's capsule and renal tubules. But PAS reaction showed discontinuity at the brush borders of proximal tubular cells (Fig. 4E, F) . Vit.C+Ive subgroups in both juvenile and adult rats showed improvement in the renal alterations, as PAS positive reaction at the thin Bowman's capsule and tubular basement membrane and brush border of proximal tubules to some degree was preserved. This improvement was more obvious in adult rats as the damage was less extensive than the juvenile ones (Fig. 4G, H) .

Immune-stained for Bax proapoptotic protein showed normal expression in cytoplasm of tubular epithelial cells in both control and Vit.C subgroups in both juvenile and adult rats (Fig. 5A-D) . Otherwise, Ive subgroups in both groups displayed patchy expression of Bax proapoptotic protein in the cytoplasm of renal tubules which was more obvious in juvenile group than in adult (Fig. 5E, F) . Vit.C+Ive subgroups in both groups demonstrated a marked improvement in the Bax proapoptotic protein expression especially in adult group rats (Fig. 5G, H) .

Morphometrical analysis of percentages of Bax positivity in control and Vit.C subgroups were 5.23%±0.15% and 5.09%±0.32% in juvenile rats and 6.32%±0.09% and 6.02%±0.43% in adult rats, respectively. These percentages were highly increased in Ive subgroups (35.37%±4.43% in juvenile rats and 29.07%±1.16% in adult rats), and in Vit.C+Ive subgroups were significantly increased (17.23%±2.43% in juvenile rats and 9.16%±1.94% in adult rats) ( Table 3 , Fig. 5I , J).

The ultrastructure examinations of control along with Vit. C subgroups in both juvenile and adult rats showed normal renal architecture. The proximal convoluted tubular cells displayed rounded heterochromatic nucleus with prominent nucleolus and intact nuclear envelop, intact apical microvilli prominent in adult group while the microvilli were less developed or absent in juvenile group, abundant parallel electron dense mitochondria were observed situated between the nucleus and uniformly thin basal cell membrane ( Fig. 6A www.acbjournal.org podocytes had several cytoplasmic extensions (the primary processes) which wrapped around the glomerular capillaries giving rise to numerous secondary foot processes called pedicles (Fig. 6E, F) .

Nevertheless, Ive subgroups displayed severe damage of renal ultrastructure in both groups where the proximal convoluted tubular cells displayed wide areas of cytoplasmic rarefaction, extremely degenerated irregular nuclei, mitochondria appeared ballooned with damaged cristae, large secondary lysosomes, markedly thickened irregular basal cell membrane and completely degenerated microvilli with extrav-asated blood in the lumen or intraluminal casts (Fig. 7A-D) . In glomerular cells, most of the foot processes were destructed or lost or fused together (Fig. 7E, F) .

Consumption of vitamin C parallel with ivermectin led to partial protection from this deterioration in adult rats as well as the juvenile ones, in adult rat there was adequate improvement of viability of the cells of convoluted tubules which exhibited normal heterochromatic nucleus, intact nuclear envelop, intact basal infoldings and relatively thick basal lamina (Fig. 7H ) some cells still exhibited apoptotic shrunken nucleus (Fig. 7J) mix of normal cells and apoptotic cells with scattered lysosomes (Fig. 7G) , and the region of glomerulus showed intact podocytes and relatively normal foot processes and thick basement membrane (Fig. 7I ).

Ivermectin has been used for several years to treat many infectious diseases in mammals. Ivermectin was identified in late 1970 and first approved for animal use in 1981. Its potential use in humans was confirmed a few years later. Subsequently, Crump and Ōmura [39] who discovered and developed ivermectin owned the 2015 Nobel Prize [40] . Previous studies proved that ivermectin is a broad-spectrum drug [39, 40] , having antiparasitic, antiviral, immunomodulation, cancer cells suppression and glucose and cholesterol regulation effects [8] , consequently, it may play a essential role in the treatment of different types of viruses including COVID-19 [6] , hope to help solving this pandemic disaster COVID-19 and because that adverse effects of ivermectin not yet investigated especially in juvenile age, this work was done to assess the toxic effect of ivermectin on renal structure and function in both juvenile and adult rats as recently it has consumed in high doses as a potent drug for treatment of cases of SARS-CoV-2 in both children and adult and also study the possible potential protective role of vitamin C since it was reported as the main additive drug used.

Effect of ivermectin investigated biochemically and the results showed an elevation in serum kidney function markers as presented in Table 2 , the serum level of urea and creatinine increased upon treatment with ivermectin in comparison with the control group in both adult and juvenile rats. Comparing of both Ive subgroups, the juvenile group showed more elevated kidney function marker. Furthermore, consumption of vitamin C parallel with ivermectin in juvenile rats led to partial protection from this deterioration, while in adult rats vitamin C led to nearly full protection. These findings also highlighted the synergistic effect of oral antioxidant vitamin C on improving metabolism and renal function. These results were in line with [41] where the rabbits treated with ivermectin plus vitamin C showed a significant decrease in serum urea, supporting the action of vitamin C as a scavenger of free radicals. Also, Arise and Malomo [42] reported that ivermectin treated rats for 15 days developed a significant increase in urea and creatinine compared with the untreated group, thereby confirming reduced renal glo-merular filtration.

Homogenate tissue analysis was done trying to understand the way by which ivermectin affect renal function, the TAC and activities of the antioxidant enzymes CAT, SOD, and GPx showed that rats treated with ivermectin (Ive subgroups) displayed a highly significant decrease TAC, CAT, SOD, and GPx with significant increase in ROS. While consumption of vitamin C parallel with ivermectin in both Vit. C+Ive subgroups exhibited stability of oxidant/antioxidant activities near control group. These results suggest that ivermectin causes damage in the kidney tissue due to production of an oxidative stress and that it's why the anti-oxidative activities of vitamin C could prevent these pathological and biochemical damage to kidney. Comparing juvenile and adult groups showed that juvenile rats had more decline in oxidants activity in treated group and less protected effect of vitamin C this was in accordance with Atakisi et al. [11] , who revealed a decrease in the TAC in animal group that was treated with ivermectin. Carr and Maggini [43] reprted that Impaired immunity and higher susceptibility to infections are outcomes of vitamin C deficiency . In turn, infections significantly impact on vitamin C levels due to enhanced inflammation and metabolic requirements. Furthermore, supplementation with vitamin C appears to be able to both prevent and treat respiratory and systemic infections. Moreover, vitamin C supplementation to Gulo -/mice, lacking the enzyme gulonolactone oxidase (Gulo) required for the biosynthesis of it, improves their metabolic profile and endoplasmic reticulum stress response and raises their life span [44] .

In pathological conditions, over expression of MMP9 causes damage to epithelial lining leading to loss of cellular matrix and cytoskeleton damage [45] , MMP9 mediate acute kidney injury due to different agents in glomeruli and tubular epithelial cells [46] . Furthermore, previous studies [47, 48] stated that induction of MMP9 promoted cytoskeleton disruption and loss of cell-cell adhesion. In this study, PCR examination had convincingly showed that MMP9 was statistically significantly higher in Ive subgroups compared to control which indicate basement membrane degradation. While consumption of Vit. C parallel with ivermectin exhibited partial stability against this degradation. Comparing juvenile and adult groups showed that adult rats had higher level of MMP9 in all subgroups. This was in accordance with Khan et al. [47] , who stated that nephrotoxicity is correlated strongly with induction of MMP9 mRNA and protein in a Anat Cell Biol 2021;54:501-517 515 www.acbjournal.org dose dependent manner. Further, while induction of MMP9 promoted cytoskeleton disruption and loss of cell-cell adhesion, inhibition of MMP9 was found to reduce these disruptions.

Further histological and morphometric examination of renal tissue confirmed the results obtained for the effect of ivermectin on serological and biochemical parameters in both juvenile and adult rats. Kidney sections revealed extremely shrunken glomeruli and a widened urinary space in between, proximal and distal convoluted tubules are dilated and their lining cells showed pyknotic nuclei with extensive cytoplasmic vacuolation, and epithelial cell exfoliations were also present, moreover, there were extensive extravasated blood and mononuclear cell infiltration. PAS-stained sections of Ive subgroups revealed strong positive PAS reaction of thickened basement membrane of both Bowman's capsule and renal tubules and discontinuity at the brush borders of proximal tubular cells, beside that there were ultra-structural alterations in which tubular cells displayed wide areas of cytoplasmic rarefaction, extremely degenerated irregular nuclei, mitochondria appeared ballooned with damaged cristae, markedly thickened irregular basal cell membrane and completely degenerated microvilli with extravasated blood in the lumen. The administration of vitamin C ameliorated the impact of the drug on the renal tissue. That was more obvious in adult rats as the pathological alteration in adult rats were less than the juvenile ones this was in agreement with Al Drees et al. [49] , who studied the effect of ivermectin on multiple organs such as kidney, liver and testis and the role of vitamin C in correction of these alterations however they stated that combination of the use supplemented vitamins A and C showed promising results than vitamin C alone in ameliorating this toxic effects of ivermectin.

Immunohistochemically, significant increase of Bax expression (a proapoptotic protein) in our study especially in Ive subgroup in juvenile rats where the toxicity and renal damage were more abundant than adult group and that was corrected partially in juvenile and was nearer to normal in adult group after administration of vitamin C. This was in agreement with other studies that found the same result in rats experiencing other pathological conditions such as hemorrhagic shock [49] . Tait and Green [50] demonstrated that apoptosis is completely dependent on Bax/Bak at the level of the mitochondria because the lack of genes encoding these two proteins results in cells that resist apoptosis by preventing release of cytochrome c. However, other studies have shown an indirect role of Bax/Bak in apoptosis and necrosis through release of cytochrome c and activation of caspases 3 and 8 [51] . In addition, Bax is responsible for the formation of these permeability pores leading to cell necrosis [52] . Therefore, the increased expression and activation of Bax as a result of ivermectin toxicity in both juvenile and adult rats may induce cell apoptosis.

In conclusion, administration of ivermectin led to attenuation in kidney function, decrease in the activities of the antioxidant enzymes and increase in MMP9 activity, significant histological and ultrastructural changes and increase in percentage of Bax proapoptotic protein expression. All these changes were more obvious in juvenile group while co-administration of vitamin C led to significant protection which was more in adult group. So, ivermectin should be used cautiously especially in juvenile age, and co-administration of vitamin C is highly recommended. 

No potential conflict of interest relevant to this article was reported.

Review of the clinical characteristics of coronavirus disease 2019 (CO-VID-19)

Outbreak of pneumonia of unknown etiology in Wuhan, China: the mystery and the miracle

World Health Organization declares global emergency: a review of the

COVID-19 and Ophthalmology: a new chapter in an old story

The FDA-approved drug ivermectin inhibits the replication of SARS-CoV-2 in vitro

Ivermectin: a systematic review from antiviral effects to COVID-19 complementary regimen

Ivermectin: panacea for resource-poor communities?

Ivermectin -old drug, new tricks?

The broad spectrum antiviral ivermectin targets the host nuclear transport importin α/β1 heterodimer

Use of ivermectin as a potential chemoprophylaxis for COVID-19 in Egypt: a randomized clinical trial

Effects of therapeutic dose of ivermectin on plasma nitric oxide and total antioxidant capacity in rabbits

Role of free radicals, oxidative stress and xenobiotics in carcinogenesis by environmental pollutants

Short-term effects of Albendazole on the oxidative stress markers and hematological parameters in tissues of African Catfish Clarias gariepinus

Adverse events following single dose treatment of lymphatic filariasis: observations from a review of the literature

Adverse reactions to ivermectin treatment for onchocerciasis. Results of a placebo-controlled, double-blind trial in Malawi

A possible case of spontaneous Loa loa encephalopathy associated with a glomerulopathy

Delirium induced by albendazole-ivermectin combination: report of the first case in an older patient

First case of ivermectin-induced severe hepatitis

Multiorgan dysfunction syndrome from strongyloides stercoralis hyperinfection in a patient with human T-cell lymphotropic virus-1 coinfection after initiation of ivermectin treatment

P1C84 -Modulation of hexachlorobenzene induced liver oxidative stress by α-Tocopherol

Regional accumulation of aluminium in the rat brain is affected by dietary vitamin E

Vitamin C-an adjunctive therapy for respiratory infection, sepsis and COVID-19

Stannous chloride induces alterations in enzyme activities, lipid peroxidation and histopathology in male rabbit: antioxidant role of vitamin C

Vitamin C: basic metabolism and its function as an index of oxidative stress

Vascular wall damage in rats induced by methidathion and ameliorating effect of vitamins E and C

We are addicted to vitamins C and E-A review

The role of vitamin C in alteration of enzymes responsible of energy metabolism induced by administration of tamoxifen to mouse

Histological changes in selected tissues of ivermectin and/or albendazole treated rats

Brain antioxidant markers, cognitive performance and acetylcholinesterase activity of rats: efficiency of Sonchus asper

Renal tissue damages and its antioxidant status improved by crab shell extract in streptozotocin-induced diabetic rat

The assay of catalases and peroxidases

A modified spectrophotometric assay of superoxide dismutase

Differential distribution of glutathione and glutathione-related enzymes in rabbit kidney. Possible implications in analgesic nephropathy

MMP9 and SCF protect from apoptosis in acute kidney injury

Analyzing real-time PCR data by the comparative C(T) method

Effects of oral exposure to diazinon on mice liver and kidney tissues: biometric analyses of histopathologic changes

Increased apoptosis and expression of FasL, Bax and caspase-3 in human lupus nephritis class II and IV

Biological Specimen Preparation for Transmission Electron Microscopy

wonder drug' from Japan: the human use perspective

The pharmacokinetics and interactions of ivermectin in humans--a mini-review

Histopathological and biochemical effects of ivermectin on kidney functions, lung and the ameliorative effects of vitamin C in rabbits (Lupus cuniculus)

Effects of ivermectin and albendazole on some liver and kidney function indices in rats

Vitamin C and immune function

Vitamin C modulates the metabolic and cytokine profiles, alleviates hepatic endoplasmic reticulum stress, and increases the life span of Gulo-/-mice

Matrix metalloproteinase 9 modulates collagen matrices and wound repair

Role of matrix metalloproteinases in renal pathophysiologies

Mercury exposure induces cytoskeleton disruption and loss of renal function through epigenetic modulation of MMP9 expression

ULP-2 SUMO protease regulates E-cadherin recruitment to Adherens junctions

Histological and immunohistochemical basis of the effect of aminoguanidine on renal changes associated with hemorrhagic shock in a rat model

Mitochondria and cell death: outer membrane permeabilization and beyond

Bax regulates primary necrosis through mitochondrial dynamics

Bax and Bak function as the outer membrane component of the mitochondrial permeability pore in regulating necrotic cell death in mice