Pumpkin seed oil alleviates oxidative stress and liver damage induced by sodium nitrate in adult rats: biochemical and histological approach

Background Nitrate (NO3) is the most common chemical contaminant in the world's ground water aquifer. Oxidative stress has been proposed as a possible mechanism involved in NO3 toxicity on non-target organism. Objectives The current study aimed to elucidate the potential protective effect of Telfairia occidentalis (pumpkin seed oil, PSO) against hepatotoxicity induced by sodium nitrate. Methods Wistar rats were exposed either to NaNO3 (200 mg/kg bw) in drinking water in drinking water, or to 4ml PSO/kg bw by gavage or to their combination. Oxidative stress parameters, biochemical biomarkers and liver histopathological examination were determined. Results Our data showed that the exposure of rats to NaNO3 caused significant changes of some haematological parameters compared to the control. In addition, there was a significant elevation of the levels of biochemical markers as that of aspartate aminotransferase, alanine aminotransferase, alkaline phosphatase and lactate dehydrogenase when compared with the control. Furthermore, exposure of rats to NaNO3 induced liver oxidative stress as indicated by the increase of malondialdehyde, progressive oxidation of protein products and protein carbonyl levels. In addition, a reduction in anti-oxidant status (catalase, glutathione peroxidase, glutathione-S-transferase and superoxide dismutase, reduced glutathione and vitamin C) was observed. Conclusion Co-administration of PSO to the NaNO3 restored most parameters cited above to near-normal values. Therefore, the present investigation revealed the ability of PSO to attenuate NaNO3-induced oxidative damage.


Introduction
Nitrate exposure may be considered as a causative factor in the context of the environmental pollutants. Drinking water is the most common pathway through which the population is exposed to nitrate 1 . In recent years, considerable attention has been paid to the intensive use of nitrates as agricultural fertilizers that reach humans and animals by different routes 2 . In fact, it penetrates through soil and remains in ground water for decades 3 . Moreover, nitrate levels in drinking water should not exceed Nitrate is relatively non-toxic 5 , but approximately 5% of all ingested nitrate is converted by microflora in the gastrointestinal tract to the most toxic nitrite 2 , which binds to haemoglobin to form methemoglobin. Thus, children are particularly susceptible to developing methemoglobinemia 3 . The risk of nitrate toxicity mainly belongs to formation of reactive oxygen species, free radicals as well as other toxic transient compounds, such as peroxynitrite, hydrogen peroxide and superoxide anion, which interrupt the equilibrium between oxidants and anti-oxidant, causing the so-called oxidative stress 6 . When produced in excess, ROS could damage critical molecules such as lipids, proteins and nucleic acid bases, thus resulting in cell cycle arrest and apoptosis 7 . Its presence may cause metabolic, and physiological modifications in hepatic cells 8 . Diet supplementation with natural anti-oxidants can serve as a type of preventive medicine, for this reason, research works dealing with the determination of natural antioxidant sources are important 9 . Therefore, the number of reports focussing on the identification, isolation and testing of natural anti-oxidants from plants has increased immesely during the last decade 9 .
Fluted pumpkin Telfairia occidentalis is a species of cucurbitaceae family in the tropics and largely consumed in some African countries 10 and frequently used as functional food or medicine 11 . The health benefits of pumpkin seeds are attributed to their macro-and microconstituents as proteins, triterpenes, lignans, phytosterols, polyunsaturated fatty acids, anti-oxidative phenolic compounds, carotenoids, tocopherol and minerals 12 .
Pumpkin seed oil is used in the preparation of some salads, giving them a very pleasant taste 13 . It is also an extraordinarily rich source of diverse bioactive compounds having functional properties used as edible oil or as a potential nutraceutical. In recent years, several studies have highlighted the medical properties of pumpkin seed oil known as strongly dichromatic viscous oil 14 .
The aim of the present study is to elucidate the possible beneficial effects of pumpkin seed oil in preventing sodium nitrate induced toxicity by evaluating biochemical, hematological and oxidative stress parameters as well as the liver histological architecture of wistar rats.

Materials and methods Chemicals
All chemical products used in this study were purchased from Sigma Chemical Co. (St. Louis, France).

Plant
Hemani pumpkin seed oil was provided from a local market. Commercialised Oil was prepared by pressing roasted pumpkin seeds in Pakistan.

Determination of total phenols
Total phenolic compounds were determined using the Folin-Ciocalteau reagent according to the method described by Bouaziz et al 15 . The optical density was measured at λ = 727 nm by using the spectrophotometer (OPTIZEN 2120UV). The total phenolic content is expressed as milligram of gallic acid (GA) equivalent per gram of PSO.

Total flavonoid contents
Total flavonoids were measured by a colorimetric assay adopted by Zhishen et al 16 . The absorbance against blank was determined at 510 nm. The total flavonoid contents were expressed as milligram quercetin equivalents (QE)/g extract.

Condensed tannin contents
The method of Julkunen-Tiitto was applied to measure condensed tanins at 500 nm after 15 min. Total tannin contents were expressed as mg catechin equivalent (C)/g of PSO 17 .
Determination of antioxidant activity DPPH radical scavenging assay DPPH (1,1-diphenyl-2-picrylhydrazyl) radical-scavenging effect was evaluated following the procedure described in a previous study 18 . The absorbance was read against a blank at 517 nm. The inhibition of free radicals DPPH in percentage (IP %) was calculated as follows: IP%= [(Ablank -Ablank)/Ablank] ×100. The anti-oxidant activities of PSO were expressed as IC50, the amount of antioxidant necessary to decrease the initial concentration of DPPH by 50%. The lower IC50 values indicate a higher antioxidant activity. The synthetic anti-oxidants butylated hydroxytoluene (BHT) and ascorbic acid were used as positive controls.

Total anti-oxidant capacity by phosphomolybdenum method
The total antioxidant capacity was based on the reduction of ammonium molybdate (IV) to ammonium molybdate (V) by the sample and the subsequent formation of green phosphate/Mo (V) compounds with a maximum absorption at 695 nm 19 .

Total antioxidant capacity by ABTS method
The total antioxidant capacity of PSO was determined by the modified method proposed by Turoli et al 20 . The stock solution of the ABTS radical was prepared by dissolving 38.4 mg of 2,2'-azinobis (3-ethylbenzthiazoline-6-acid) (ABTS) in potassium persulfate solution (2.45 mM), and the mixture was dark stored for 12 hours. The working solution was obtained by diluting the stock solution of the ABTS radical cation with methanol to obtain an absorbance of 0.7 ±0.002 at 730 nm.

Animals
Male Wistar rats (fifteen weeks old, weighing between 200 and 260g), obtained from Pasteur institute (Algiers) were used for the experimental procedures. Animals were acclimated for 2 weeks under the same laboratory conditions of photoperiod, an average relative humidity of 60% and room temperature of 23±2°C. Food (standard food, supplied by the "ONAB, Bejaia", Algeria) and water were available ad libitum.

Experimental design
Rats were randomly divided into four groups of ten animals each (n=10). The first group served as a control. The second group was treated with sodium nitrate (200 mg / kg body weight / day) in drinking tap water throughout the experimental period (28 days) 3 , while the third group was treated with pumpkin seed oil daily by oral gavage (4ml/ kg body weight / day)13. The fourth group received a combination of NaNO3 and pumpkin seed oil in the same way as in group II and III. Body weight, water and food consumption were monitored during treatment. All protocols used in this study were approved by PNR/ SF 08/2012 and by the Ethical Committee of Directorate General for Scientific Research and Technological Development at Algerian Ministry of Higher Education and Scientific Research.

Blood collection
At the end of the experimental period, animals were fasted overnight, then weighted and sacrificed by cervical decapitation. Blood samples were immediately collected into two groups of ice-cold polypropylene tubes. While the first one contained ethylenediaminetetracetic acid (EDTA) used for the determination of haematological parameters, the second group (had no anticoagulant) was centrifuged at 3,000 rpm for 15 min at 4 o C and then used for the measurement of biochemical parameters. Serum samples were stored at -20°C.

Preparation of liver homogenates
Liver samples were quickly removed, washed in 0.9% NaCl solution and weighed after the careful removal of the surrounding connective tissues, and then 1 g was homogenized in 2ml of buffer solution (50mm Tris, 150mm NaCl, pH 7.4) in ice-cold condition. Homogenates were centrifuged at 10,000 rpm for 15 min at 4 °C (Presvac DCS-16RTV); the supernatants were divided into aliquots and then stored at -20 °C.

Nitric oxide serum levels
The level of nitric oxide (NO) in serum was measured by assaying total nitrate/nitrite, as described by Green et al 21 . The subsequent absorbance was determined using an ELISA reader (mindray MR-96A). The concentration of NO was determined using a standard curve prepared from NaNO2.

Liver MDA, PCO and AOPP measurement
Lipid peroxidation in liver was realised by measuring malondialdehyde (MDA) levels according to the method of Esterbauer et al 22 . The absorbance of TBA-MDA complex was recorded at 530 nm. The MDA content was expressed as nmol MDA/mg proteins. Protein carbonyl (PCO) levels in liver tissue were determined using the 2,4-Dinitrophénylhydrazine (DNPH) method by Reznick and Packer 23 . The absorbance of the sample was read against a blank with guanidine at 370 nm. Protein Carbonyl (PCO) contents was calculated based on the molar extinction coefficient of DNPH (ε = 2.2 104cm M-1) and expressed as nmol/mg proteins. Liver tissue contents of advanced oxidation protein products (AOPP) were determined at 340nm according to the method of Kayali et al 24 . The concentration of AOPP for each sample was calculated using the extinction coefficient of 261cm-1mM-1 and the results were expressed as nmol/mg proteins.

Estimation of liver enzymatic antioxidants
Glutathione peroxidase (GSH-Px) activity was measured according to the procedure of Flohe and Gunzler 25 . The absorbance was recorded at 412 nm and the specific activity of this enzyme is expressed as μmol GSH/mg proteins. Glutathione-S-transferase (GST) activity was measured by the method of Habig et al 26 . The 1-Chloro-2,4-dinitrobenzène (CDNB) was used as electrophilic substrate that binds to GSH with the participation of the enzyme and forms a colored GSH-substrate complex, detected at 340 nm. The activity of GST was expressed in terms of nmol GST/min/mg proteins. Catalase activity (CAT) was measured using the method of Aebi 27 . It is based on the ability of the enzyme to induce the disappearance of hydrogen peroxide monitored by following the decrease in the absorbance at 240 nm for 1 min. CAT activity was calculated in terms of µmol H 2 O 2 consumed/min/mg of proteins. Superoxide dismutase (SOD) specific activity was determined according to the method described by Beyer and Fridovich 28 . One unit of SOD activity corresponded to the amount of enzyme required to cause 50% inhibition of Nitro blue tetrazolium (NBT) reduction at 560nm. SOD activity was expressed as units'/mg proteins.

Estimation of liver non-enzymatic antioxidants
Reduced glutathione (GSH) concentrations in liver homogenates were performed with the method described by Ellman 29 modified by Jollow et al 30 . It is based on the development of a yellow color when DTNB [5,5`-dithio-bis-(2-nitrobenzoic acid)] is added to compounds containing sulfhydryl groups. The absorbance was recorded at 412 nm. Total GSH content was expressed as nmol GSH/mg proteins. Liver vitamin C level was performed as described by Jacques-Silva et al 31 . The absorbance was measured at 540 nm. The data are expressed as µmol/mg proteins.

Histopathological examinations
Liver samples were dissected and immediately fixed in 10% formalin solution for histopathological analysis. The organ tissues were processed using a graded ethanol series, and embedded in paraffin. The paraffin sections were cut into 5μm (Microtome Leica RM 2125RTS) thick slices and stained with hematoxylin and eosin for light microscopic examination.

Statistical analysis
All data were expressed as mean ± SD for 10 rats of each group using Microsoft Excel (2016). Significant differences between group's means were determined by Student's t test. The statistical significance was taken at p≤0.05.

Polyphenolic contents and antioxidant activity of PSO
Results for the quantitative determination of total phenols, flavonoids and tannins contents of PSO are shown in Table 1. The assessment of the DPPH showed an IC50 value (µg/ml PSO), total antioxidant capacity by phosphomolybdeneum (mg Vit C/g extract) and ABTS radical scavenging (mg trolox equivalent/g PSO).

Effect of treatments on body and liver weight
Changes in body, relative and absolute liver weights are presented in Table 2. Our results showed a significant decrease in the body weigt of NaNO 3 group (-8.79%). Their absolute and relative liver weight was increased sig-nificantly by (+13.77%), and (+25%), respectively, when compared to that of the control. However, in NaNO 3 / PSO treated rats, a significant decrease in absolute and relative liver weight compared to NaNO 3 were registered (-11% and -15.6% respectively). Values are means ± SEM, n: number of animals in each group. *p<0.05, **p<0.01, ***p<0.001: significantly different from control group. #p<0.05, ##p<0.01, ###p<0.001: significantly different from NaNO3.

Effect of treatments on food intake and water consumption
The PSO and NaNO 3 /PSO groups induced significant reduction in food intake -7.08 % and -8.34 %) and water consumption (-10.88 % and -5.92%) compared with the control rats. However, NaNO 3 group had no effect on water consumption and significantly decreased food intake by -5span style="font-family:'Times New Roman'">.26%.

Effects of treatments on haematological parameters
The treatment of animals with NaNO 3 significantly decreased RBC, Hb and Ht by -11.41%, -20.39%) and -7.02%, respectively, and considerably increased WBC count by +62.12% in comparison to the control (Table  3). However, the administration of PSO alone caused a significant increase of WBC by +10.7% as compared to the control. The PSO co-treatment (NaNO 3 +PSO) ameliorated these parameters when compared to NaNO 3 group.

Effects of treatments on biochemical parameters
Compared to the control, NaNO 3 treated animals had a significant increase in serum AST, ALT, ALP and LDH activities ( Table 4). The administration of PSO alone caused a significant decrease of ALT and LDH activities compared to the control. In addition, the levels of serum glucose, total bilirubin and total proteins of Na-NO 3 -treated rats were significantly increased. The com-bined treatment (NaNO 3 +PSO) restored all biochemical parameters studied.

Effect of treatments in nitric oxide levels
The treatment of rats with NaNO 3 induced substantial increase of serum nitric oxide (NO), while the co-treatment preserved the NO at its normal levels (Table 4). MDA, PCO and AOPP levels  Table 5, a considerable increase in MDA, PCO and AOPP contents of liver by +105.13%, +47.34% and +90.57%, respectively, was observed in NaNO 3 treated animals when compared to the control. The treatment with PSO alone caused a decrease in MDA and AOPP levels (-27.62% and -30.43%, respectively) compared to the control. The co-administration of NaNO 3 and PSO induced a significant amelioration of MDA, PCO and AOPP levels compared to the control. Table 5. MDA, PCO, AOPP and non-enzymatic antioxidant (GSH, vitamin C) levels in liver of control and treated rats with NaNO 3 , PSO or their combination (NaNO 3 /PSO) during 28 days.

Non-enzymatic and enzymatic anti-oxidant status
The concentration of glutathione and Vit C showed a significant decrease by -18.87% and -38.08%, respectively, in NaNO 3 treated group compared to the control ( Table 5). The GPx, GST, CAT and SOD antioxidant activities also decreased. In NaNO 3 group, GPx, GST, CAT and SOD activities were significantly decreased by -35.54%, -50%, -25.47% and -17.2 %, respectively, when compared to the control. These modifications were changed by the co-administration of PSO with NaNO 3 in animals as indicated in the significant increase of GPx, GST, CAT and SOD activities compared to that of NaNO 3 group (Table 6).

Histopathological profiles
The histopathological examination of liver is shown in Table 7 and Fig. 1. In fact, the microscopic observation of the control group revealed a normal architecture ( Fig.  1-A). In contrast, NaNO 3 -treated liver revealed hepatocytes degeneration (black arrow), vein congestion (white arrow), inflammatory cell infiltration (circle) and sinusoi-dal dilatation (Star) (Fig1-B). However, no histological alterations were observed in the livers of PSO group when compared to the control (Fig 1-C). Furthermore, the co-administration of NaNO 3 and PSO (Fig 1-D) has reduced the inflammatory cell infiltration, kept normal hepatocytes architecture and lowered the degree of sinusoidal dilatation compared to sodium nitrate treated group.

Discussion
From the above data, pumpkin seed oil seems to contain high amount of polyphenols, flavonoids and tannins. Accordingly, Que et al 32 have reported that PSO is rich in phenolic and flavonoid compounds. These components are said to possess many functional groups, including hydroxyl groups, which have very strong anti-oxidant potential 33 . In consequence, polyphenols and flavonoids are able to scavenge hydroxyl radicals, superoxide anion and peroxylipidic radicals 34 . Moreover, it was clearly shown in this study that PSO had a potential antioxidant to scavenge DPPH, phosphomolybdenum and ABTS radical. This is why pumpkin is a plant that has been frequently used as functional food or medicine 11 . Anti-oxidant properties, especially radical scavenging activities, are very important due to the harmful role of free radicals in foods and in biological system. DPPH is a stable free radical, which accepts an electron or hydrogen radical to become a stable diamagnetic molecule 35 .
This research work showed that the treatment of rats with sodium nitrate induced a significant decrease in body weight and daily food consumption, which may be due to the toxicity induced by this toxicant. This result is in agreement with that obtained previously 8,36 . Other data suggested that nitrate can exert its effect on the body weight through increasing protein catabolism 37 . Therefore, the decreased serum and tissue proteins may indicate the enhanced protein catabolism associated with weight loss 1 . Although the treatment of rats with PSO had no significant effect on body weights 14 , it had a significant decrease in food intake and water consumption, but it normalises serum total proteins. The decrease in food intake and water consumption are probably due to the presence of tannins and gallic acid in pumpkin seed oil, which can decrease food ingestion and the growth rate 34 . Furthermore, the increase of the total proteins perhaps is due to the fact that pumpkin seeds (Cucurbita spp.) are rich in mineral, calories and proteins 38 .
The exposure of rats to NaNO 3 increased glycaemia and nitric oxide serum levels, which are in accordance with the study of El-wakf et al, who demonstrated that hyperglycaemia could be a cause of insulin deficiency 1 . However, the increased generation of NO could lead to tissue damage, which can have a direct effects mediated by NO itself or an indirect effect mediated by reactive nitrogen species 1 . Yet, the co-administration of PSO to treated rats resulted in significant improvement in serum level of the previous parameters, which are in good agreement with the earlier studies 39,40 .
The exposure to NaNO 3 is also characterized by the depletion of RBCs, HT and Hb and increased WBC counts. The significant reduction in RBC and Hb is probably due to the effect of the free radicals generated by nitrate on the red cells when certain free radicals, as O 2 .-and OH, are very reactive species able to cause membrane lipid damage. Moreover, in the presence of strong concentrations of these radicals, haemoglobin can easily oxidised 41,42 . Furthermore, PSO co-administration in rats' was found to keep the investigated parameters within their physiological ranges. Such effect might be related to the phenolic compounds, which act to scavenge the free radicals. Soltan 38 showed an increase in RBC, Hb and HT levels in rats fed with pumpkin powder seed and ascorbic acid. Contrary, Kuku et al 43 showed a lowering in WBC counts in animals fed unprocessed and under-processed fluted pumpkin seeds.
Our results demonstrated a significant increase in serum AST, ALT, LDH and ALP activities of NaNO 3 treated rats. The increases in enzymes activities may be owed to hepatic cell damage or dysfunction, which results in the leakage of these enzymes from hepatocytes into the blood and/or to the disturbance in the balance between biosynthesis and degradation 9 . The present results are in agreement with those obtained previously 8 . Meanwhile, NaNO 3 treatment also caused a significant increase in serum bilirubin levels, emanating from the toxic effect of nitrates by destructing red blood cells. However, serum bilirubin increases could also be of hepatic origin (hepatitis, cirrhosis). Indeed, Al-Ezzy et al 5 showed a rise in the serum total bilirubin level of mice treated with sodium nitrate. In fact, the co-administration of PSO was proven to ameliorate the levels of all studied biochemical parameters. Our findings are consistent with those of Abou Seif 11 who reported that pre-treatment of rats with PSO improved the serum total proteins and bilirubin levels and the activities of LDH, ALT and ALP. The administration of proteins extracted from pumpkin seeds after CCl4 intoxication had significantly reduced the LDH, ALT, AST, and ALP activities 44 . The possible explanation is that PSO had hepathoprotective effects on nitrate toxicity, by scavenging free radicals, quenches their damaging effects and remedies liver injury.
Among the various oxidative modifications of amino acids in proteins, PCO formation may be an early marker for protein oxidation 7 . From this information, we proceeded to assay MDA, PCO and AOPP levels in liver tissue. The actual data showed an increase of all these parameters in NaNO 3 group in the presence of sodium nitrate, which induces the formation of free radicals that attack lipids and proteins of hepatic cells. In parallel, Bouaziz-ketata et al 8 have shown that the administration of NaNO 3 caused a remarkable rise of rat liver MDA contents. Owing to the MDA cytotoxicity and inhibitory action on cellular protective enzymes, it is suggested to act as a tumour promoter 45 .
The antioxidant and other cell redox state modulating enzyme systems act as the first-line defense against ROS in all cellular and extra cellular compartments 46 . Oxidative damage is aggravated by the decrease in antioxidant enzymes activities as SOD, CAT, GPx and GST, which act as free radical scavengers in conditions associated with oxidative stress 47 . More specifically, SOD is the first line of antioxidant defense, which accelerates the dismutation of superoxide ion into less toxic H 2 O 2 . The latter is subsequently converted into nontoxic water and oxygen molecules by the action of CAT 48 . Nevertheless, GPx plays a pivotal role in H 2 O 2 catabolism and GST acts a key role in cellular detoxification 41,49 . It was found that small deviations in physiological concentrations may have dramatic effects on the resistance of cellular lipids, proteins and DNA to oxidative damage 49 . Moreover, the treatment of rats with sodium nitrate lowered the levels of SOD, CAT and GPx activities 8 .
In addition, a reduction of Vit C and GSH levels in NaNO 3 treated rats were recorded in this study. It is postulated that the hepatoprotective effect of vitamin C is associated with its antioxidative property by decreasing lipid peroxidation either directly or indirectly through the regeneration of vitamin E 5 . Moreover, GSH, the most abundant thiol in the cell, is considered as the major cellular redox buffer 46 . The decrease of GSH level of liver tissue can be provoked by the toxic effect of NaNO 3 , by blocking its thiol function with direct conjugation of nitrate and/or its metabolite, or through the inhibition of glutamyl-cysteine-synthetase activity. Furthermore, decreased hepatic GSH level was noticed after the treatment of rats with sodium nitrate 8 .
In parallel, the treatment of rats with pumpkin seed oil have not disturbed the concentrations of MDA, PCO and AOPP. In addition, PSO supplementation ameliorated the non-enzymatic GSH and Vit C and the enzymatic antioxidant activities of SOD, GST, CAT and GPx. This rebalance of the antioxidant status is certainly related to the high antioxidant potential of PSO that contains polyphenols, flavonoids acids and tannins detected in its phytochemical study. The PSO is also known to contain high amounts of tocopherols and selenium, which are powerful anti-oxidants. The latter are suggested to provide good tissue oxygenation 50 . On the same way, the pre-treatment of rats with pumpkin seed oil induced a noticeable re-duction in lipid peroxidation and boosted the antioxidant status represented by hepatic CAT, GST and GSH 11 . Moreover, hepatoprotection was observed through the decrease of MDA level after supplementation of flax and pumpkin seed mixture 53 . Makni et al. (2011) 39 also showed a rise in anti-oxidant enzymes activities and GSH level in diabetic rats supplemented with flax and pumpkin seed. Likewise, polyunsaturated fatty acids (linoleic acid and α -linoleic acid) have been shown to display protective roles against lipid peroxidation, by increasing the levels of several cellular antioxidants, such as ascorbic acid, α-tocopherol and GSH 11 . Furthermore, the essential trace mineral zinc in pumpkin seeds was suggested to neutralize free radical generation, or directly occupy the iron or copper binding sites of lipids, proteins, and DNA molecules 51 .
In fact, the relative and absolute liver weight of rats treated by nitrate was significantly increased. This increase may be due to the toxic effect of nitrate or its metabolites, which could induce liver injury and hepatocytes necrosis. These results agree well with those of Ogur et al 52 who showed that nitrate intake caused hepatomegaly.
In the present study, the liver histology of NaNO 3 -treaded rats showed an infiltration of inflammatory cell, vein congestion, hepatocytes degeneration, and sinusoidal dilatation, which may be due to the formation of free radicals, protein carboxylation and lipids peroxidation that caused plasma membrane destruction. Therefore, the histopathological study of liver tissues confirms the changes of the previously studied parameters. In nitrate-treated rats, liver showed a vein inflammation, cellular degeneration and cell necrosis 8 . Fortunately, PSO co-administration showed only slight histological alteration, by reducing inflammatory cell infiltration and lowering the degree of sinusoidal dilatation. This result is in accordance with those of Makin et al 53 who showed a normal architecture of rat liver tissues fed with cholesterol and pumpkin seed mixture.

Conclusion
The results obtained in this study revealed the presence of phenolic, flavonoids, tannins and antioxidant scavengers in pumpkin seed oil. However, PSO co-administration with sodium nitrate decreased liver injury, and maintained haematological, biochemical and oxidative stress parameters of rats within the physiological ranges. This finding suggests the possible protective roles of pump-kin seed oil towards the cytotoxicity induced by sodium nitrate.