Biochemical and Histological Studies of Goji Extract Role on Patulin Mycotoxin on Male Rat Kidney

Patulin caused severe damage in several organ systems like kidney, intestinal tissue and immune system. The objective of this study is to show the effects of patulin mycotoxin on some biochemical parameters and histological changes on male rats’ kidney. 50 adult albino male rats were divided randomly into 5 groups. Control group was injected subcutaneously daily with distilled water; groups I and II were injected subcutaneously daily with Patulin (0.2 mg/kg/day) for one and two weeks respectively. Group III was treated with the same dose of patulin for two weeks after that they were injected subcutaneously with Goji extract (2ml/ kg /day) for two weeks. Group IV was treated by Goji for two weeks after that they were treated with the same dose of patulin for two weeks. Level of total antioxidant stress (TAS), Blood urea nitrogen (BUN) and pyruvate kinase (M2-PK) were decreased significantly in serum of both treated groups compared with control group, but level of serum creatinine (SCr), Alpha feto protein (AFP) and carcinoembryonic antigen (CEA) were increased significantly in serum of both treated groups compared with control group. Histopathological changes of rat kidney coincided with biochemical changes. In conclusion, consumption of patulin induced renal toxicity. Goji extract may be used as a new therapeutic for patulin toxicity. *Corresponding Author: Nagwa M. Elsawi, Department of Chemistry, Faculty of Science, Sohag University, Sohag, Egypt. E-mail: elsawinagwa@yahoo.com Received Date: August 21, 2015 Accepted Date: October 29, 2015 Published Date: November 04, 2015


Introduction
Toxins produced by filamentous fungi are called mycotoxins. This term, by general consensus, is used almost exclusively for fungi associated with food products and animal feed, excluding toxins produced by mushrooms [1] . Mycotoxins are secondary metabolites, with no apparent function in the normal metabolism of fungi. They are produced mainly, although out exclusively, when the fungus reaches maturity [2] . Mycotoxins commonly occur in human and animal food derivatives and can appear in the field before harvest, post-harvest or during processing, storage and feeding, adversely affecting the quality of the food [3] .
Patulin ( Figure A), is an unsaturated heterocyclic lactone produced by certain fungal species of Penicillium, Aspergillus and Byssochlamys growing on fruit [4] . Patulin has been mainly found in apple and apple products and occasionally in pears, grapes, apricots, strawberries, blueberries and peaches [5] . Animal tissues affected by PAT administration included kidney and intestine [6,7] . PAT is believed to exert its cytotoxic effects mainly by forming covalent adducts with essential cellular thiols in proteins and amino acids [8] . The sub-acute administration of patulin has been mainly studied in rats, where it was shown to induce weight loss, gastric and intestinal changes and alterations in renal function [9] . Repetitive doses lead to signs of neurotoxicity (tremors, convulsions) as well as an inhibition of several enzymes (ATPase) in the intestine [10] , and the brain, in particular, with consequences in terms of lipid 2 metabolism [11] . Fresh extracts of fruits, herbs, vegetables, cereals and other plant materials rich in phenolics are of increasing interest in the food industry, because they retard oxidative degradation of lipids and thereby improve the quality and nutritive value offood [12] . Lyciumbarbarum (Goji) (Figure b) have been used in Chinese medicine for over 2000 years where their beneficial effects are claimed to enhance the immune system, improve eye sight, and circulation, and to possess anticarcinogenic properties. The immune enhancing, anti-cancer and antioxidative properties of Wolfberry polysaccharides are reported in several Chinese publications [13,14] . The present study was planned to assess the biochemical profile supported by histological evidence of patulin on kidney of male rat in order to evaluate the possible role of Goji extract in reversing patulin toxicity.

Extraction of Goji
Goji berry extract was made according to Yang and Baojun 2013 [15] .

Experimental Design and Animals
Fifty white male albino rats each weighs (240-300 g) were kept at 22°C, and 12 h light and 12 h dark cycle. They were given standard rat diet and had free access to tap water. The animals were divided randomly into five groups (10 rats each in two cages) and were subjected to the following schedule of treatments: Control group was injected subcutaneously daily with distilled water; groups I & II were injected subcutaneously daily with patulin 0.2 mg/kg/day [16] for one and two weeks respectively. Group III was treated by patulin as previous dose for two weeks after that they were injected subcutaneously with Goji extract 2 ml/kg/day for two weeks. Group IV was treated by Goji for two weeks after that they were injected subcutaneously with the same toxin for two weeks.

Biochemical Studies
Animals were anesthetized under light diethyl ether and blood samples were collected from the heart into plain tubes and stored at-20°C until analysis was performed. Sera were used for the measurement of Blood Urea Nitrogen (BUN), Serum Creatinine (SCr), total antioxidant stress (TAS), Alpha feto protein (AFP), Carcinoembryonic Antigen (CEA) and Pyruvate Kinase (M2-PK). Level of (BUN) was measured according to Urease-Berthelot method. Level of (SCr) was measured by Jaffe Reaction. In addition, (TAS) concentration was measured by reaction of antioxidants in the sample with a defined amount of hydrogen peroxide (H 2 O 2 ); the antioxidants in the sample eliminate a certain amount of the hydrogen peroxide. The residual H 2 O 2 is determined colorimetrically by an enzymatic reaction which involves of 3,5, dichloro-2-hydroxybenzensulphonate to a colored product. (AFP) and (CEA) were determined by ELISA kit was purchased from Elab Science. (M2-PK) was determined by ELISA kit was purchased from Wkeamed supplies.

Histological Studies
For the histological preparations, the abdomen was opened and dissected to remove their right and left kidneys at the end of the treatment. Renal tissues were cut into small pieces and then fixed in 10% neutral buffered formalin for 24h and 4% glutaraldehyde for light and electron microscope [17,18] , examined and photographed using a JEOL JEM 1010 electron microscope (JEOL Ltd, Tokyo, Japan) in the Electron Microscope Research Laboratory of the Histology and Cell Biology Department, Faculty of Medicine, Sohag University (Egypt).

Statistical Analysis
Statistics was performed using the statistical graph pad prism 5. One way analysis of variables (ANOVA) was used posted by Newman-keuls test. All results are expressed as mean ± SE and the level of significance between groups were *p<0.05, **p<0.01, ***p<0.0001 (Table 1).

Biochemical Results
The Data in Table 1 Indicated That The mean value of serum BUN concentration (mmol/L) showed highly significant decrease (P > 0.01) in G I and G II as compared with control. The mean value of serum SCr concentration (mg/dl) showed highly significant increase (P >0.001) in G I and G II as compared with control. The mean value of serum TAS concentration (mμ/l) showed highly significant decrease (P >0.001) in G I and G II as compared with control.The mean value of serum AFP and CEA concentration (ng/ml) showed highly significant increase (P > 0.001) in G I and G II as compared with control .The mean value of serum M2-PK concentration (ng/ml) showed significant decrease (P > 0.05) in G I and G II as compared with control.However, Non-significant changes in the mean value of all previous biochemical parameters in G III and G IV were observed as compared to control.

Histological Results
In light microscopic examination the renal cortex of the control group was characterized by the presence of renal corpuscles, proximal and distal convoluted tubules (PCT&DCT). Each renal corpuscle was consisted of a glomerular capillary tuft surrounded by capsular space and Bowman's capsule (Figure 1a). Ultrastructure, glomerular capillaries were lined by a thin layer of fenestrated endothelial cells and surrounded by podocytes's foot processes (Figure 1b). The PCT rested on a thin regular basement membrane and lined by cuboidal cells with profuse luminal microvilli. They had large rounded euchromatic nuclei with prominent nucleoli, many apical pinocytotic vesicles, lysosomes, basal infoldings and longitudinal arranged mitochondria  The light microscopic examination of group II revealed persistence histological changes of the previous group with appearance of hyaline casts in the lumen of some tubules ( Figure  3a). Ultrastructure, irregular thickened GBM and loss of endothelial fenestrae were seen (Figure 3b). The PCTs showed thickened basement membrane and destructed basal infoldings. Some cells revealed karyolitic nuclei, few mitochondria, numerous vacuoles and absence of luminal microvilli (Figure 3c). DCT cells exhibited heterochromatic irregular nuclei, apical migration of the mitochondria, numerous vacuoles and absence of apical microvilli (Figure 3d). The therapeutic use of Goji group III led to decrease in the histological changes of the kidney. Most of the renal cortical tissues were more or less similar to the control group. Some tubules were lined with vacuolated cells. Others with dilated and destructed wall were still seen. Dilated congested blood capillaries were also observed (Figure 4a). On the other hand, the prophylactic use of goji group IV revealed marked improvement as compared with group III (Figure 5a). Ultrastructure podocytes, GBM and blood capillaries were more or less similar to the control group (Figures 4b,5b). Some PCT cells appeared with vacuolated cytoplasm (Figures 4c, 5c). Most of DCT cells were more or less similar to the control group (Figures 4d, 5d).

Discussion
In the present investigation, the effect of patulin on BUN, SCr, TAS, AFP,CEA and M2-PK was studied in male albino rats.
The mean value of BUN concentration (mmol/L) showed highly significant decrease (P >0.01) in G I and G II. Urea is amajornitrogenous end product of protein and amino acid catabolism, produced by liver. In kidneys urea is filtered out of blood by glomerulli and is partially being reabsorbed with water [19] . these results may be attributed to the varying toxic effect of patulin on kidney function as indirect effect that the low value of urea could be referred to acute liver failure (decreased urea synthesis), and repeated peritoneal dialysis [20] and also low levels of urea are seen in trauma, surgery, opioids, malnutrition, and anabolic steroid use [21] . Rats treated with patulin showed highly significant increase (P > 0.001) in the mean value in G I and G II. This increased level of SCr may be due to acute renal insufficiency [22] and in most cases of mycotoxin nephrotoxicity [23] and also the observed elevation in creatinine may be related to several factors controlling urea metabolism such as homeostasis of amino acids in the body, suppression of gluconeogenesis, presence of tissue damage and liver or kidney lesions. All these factors are proved to be affected by patulin as reported by [24,25] . In the current study, the mean value of serum TAS concentration (mμ/l) showed highly significant decrease (P > 0.001) in G I and G II, this was most probably point to presence of an oxidative stress due to mycotoxicty, immune dysfunction and a poor outcome [26] . On the other hand, Trace amount of AFP is also produced in the fetal gastrointestinal tract, kidney and placenta [27] . In this study, the mean value of AFP concentration (ng/ml) showed significant increase (P > 0.05) in G I and G II, this results from nephrotoxicity of patulin where, Aoki, et al. 2001 said that Serum elevation of AFP has been reported in renal cell carcinomas. AFP-producing neoplasm of the urinary tract is one case of renal pelvic carcinoma [28] . Also, the mean value of serum CEA concentration (ng/ ml) showed highly significant increase (P > 0.001) in G I and G II. This could be due to insufficient elimination of CEA through the kidneys, dialysis membranes and peritoneum [29] . It is clearly from Table 1 that the mean value of serum M2-PK concentration (ng/ml) showed significant decrease (P >0.05) in G I and G II. It is well documented in literature that the first step during multistep carcinogenesis is the loss of the tissue-specific isoenzymes, e.g. L-PK in liver and kidney and M1-PK in brain and muscle, followed by the subsequent expression of the M2-PK isoenzyme as was demonstrated for renal cell carcinoma [30] . The impairment in renal function that revealed by these biochemical results was parallel to the histological findings. There was thickening of the glomerular and tubular basement membrane. This might result from an increase in the amount of collagen fibers secondary to their overproduction from regenerated epithelial cells. In accordance to these suggestions some authors found that reactive oxygen species (ROS) led to GBM components oxidation and changed type IV collagen formation [31,32] . Fusion of broad flat processes of podocyte led to disappearance of the slit diaphragm leading to the onset of protein uria that was manifested as hyaline casts. This could be due to direct injury to the podocyte skeleton by increased the production of ROS and decreased antioxidant levels. Moreover, this might occur with thickened GBM to compensate the increased glomerular permeability [33] . However some authors suggested that this fusion might be as a result of podocyte epithelial-to-mesenchymal cell transition [34][35][36] , found that patulin caused endoplasmic reticulum stress response and the induction of the mitochondrial apoptotic pathway in kidney cells. In accordance with this suggestion it was proved that patulin led to membranes depolarization, increased Ca 2+ level and cell damage by forming adducts with thiol-containing cellular components [37,38] , On the other hand [39] noted that patulin caused p38 kinase and c-Jun N terminal kinase phosphorylation. However, it was found that patulin could disrupt the apoptotic mechanism [40] . In association with these tubular changes there were some dysplastic tubules, frequent mitotic figures and high level of AFP, and CEA. This might refer to the ability of patulin to induce precancerous changes in the renal tissue [41] . In coincide to that it was proved that some apoptotic triggers are important in tumor progression as UV radiation [42] .
However, there were no significant changes in the mean value of all previous biochemical parameters, BUN, SCr, TAS, and M2-PK were observed in III (therapeutic) and IV (prophylactic) groups compared to control. This is due to the effective role of Lycium Barbarum in reducing oxidative stress induced by a chemical toxin where Lyciumbarbarum extract as effective free radical scavengers, was demonstrated and has antioxidant activity [43] . On the other hand, it has the ability for absorption or elimination of the mycotoxinand inhibiting its transformation resulting in the increase of its toxicity [44] . Lyciumbarbarum (Goji) contain pharmacologically Active constituents that offer a variety of indications that affect different organs of the body [45] .
It was proved that it could decrease the expression of CYP2E1 [46] . The improvement in the degenerative changes in the renal tubules could be due to the direct effect of the extract on DNA [14] and cell membrane [47,48] found that, Lyciumbarbarum could reduce diabetic nephropathy. However non-significant changes of AFP and CEA with absence of the mitotic figures and dysplastic tubules might be secondary to anticancer activity of Goji. In accordance with this suggestion it was proved that its aqueous extract could inhibit proliferation in hepatocellular cancer in rat and growth of sarcoma in mice [49,50] .

Conclusion
In Conclusion, this study has described several biochemical assays of kidney after administration of patulin mycotoxin to rats. These results add to our knowledge of one of the most important Penicillium and Aspergillus mycotoxins occurring naturally in agriculture products and it is found that treatment of rats with Goji extract ameliorated the adverse effects of mycotoxins. The results suggest that Goji extracts may be used asantioxidant and antidote for patulin in mice.