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Black Soybean Shows Protective Function against Carbon Tetrachloride-induced Liver Damage in Sprague-dawely Rats

Wei-Hsuan Lin1, Huai-Wen Yang1, Cheng-Kuang Hsu1*, Jyun-Kai Jhan2, Dan-Yuan Lo3

Department of Food Science, National Chiayi University, 300 Syuefu Rd. Chiayi City 60004, Taiwan, ROC

Department of Food and Nutrition, Providence University, 200 Chung-Chi Rd., Shalu, Taichung City 43301, Taiwan, ROC

Department of Veterinary Medicine, National Chiayi University, 300 Syuefu Rd. Chiayi City 60004, Taiwan, ROC

*Corresponding Author:
Cheng-Kuang Hsu
Department of Food Science, National Chiayi University, 300 Syuefu Rd., Chiayi City 60004, Taiwan ROC
Tel: +886-5- 2717618
E-mail: ckhsu@mail.ncyu.edu.twM

Received date: 12/10/2015 Accepted date: 09/02/2016 Published date: 12/02/2016

Visit for more related articles at Research & Reviews: Journal of Botanical Sciences

Abstract

Anthocyanins are abounding in the seed coat of black soybean (BS) (Glycine max (L.) Merrill), which contribute to anti-oxidative and anti-antiinflammatory activities. It leaded us to investigate the protective function of BS against a strong oxidant carbon tetrachloride (CCl4) induced liver damage in rats. BS was baked at 130°C for 5 min and then was submerged in 100°C hot water for 20 min to produce an anthocyanin enriched tea/decoction (BST). Protective function of BST against CCl4-induced liver damage in Sprague-Dawely rats was investigated with six experimental groups: control, high BST (1 g BS/kg bw), CCl4 (0.5 ml 20% CCl4), CCl4 + silymarin (0.2 g/kg bw), CCl4 + low BST (0.1 g BS/kg bw) and CCl4 + high BST (1 g BS/kg bw). BST enhanced GSH and GSSH contents, as well as antioxidant enzymes activities (superoxide dismutase (SOD), glutathione peroxidase (GPx) and glutathione reductase (GR) activities) in the liver tissue of normal rats. BST also attenuated the elevation of serum glutamate oxaloacetate transaminase (GOT) and glutamate pyruvate transaminase (GPT) levels in CCl4 treated rats. Liver histopathology revealed that BST reduced fatty liver and liver fibrosis caused by CCl4. It was suggested that anthocyanins in the seed coat of black soybean contributed to such hepatoprotective effect.

Keywords

Black soybean, Tea, Antioxidant, Liver protection, Carbon tetrachloride.

Introduction

Black soybean (Glycine max (L.) Merrill) is commonly used as medicinal food and herb in oriental countries. It has antiinflammatory activity, antiproliferative effect, and antioxidant capacity, as well as the ability to reduce the risk of cancer [1-4]. The biological functions of black soybean are mainly associated with its anthocyanin compounds, which are abundant in the seed coat of black soybean [5-8]. It has been reported that anthocyanin extract from black rice bran has hepatoprotective effect against carbon tetrachloride-induced liver injury in mice and the extract from black rice can inhibit alcohol-induced chronically liver damage in rats [9,10]. Moreover, it is found that cyanidin-3-O-glucoside (C3G), an anthocyanin commonly found in many natural plants, showed hepatoprotective function in carbon tetrachloride treated mice [11]. Since the seed coat of black soybean contains high amount of anthocyanins and the major anthocyanin in the seed coat is C3G, it leads us to consider that black soybean may also exhibit such hepatoprotective functions. Thus, in this study, we evaluate the protective effect of black soybean on carbon tetrachloride-induced liver damage using Sprague-Dawely (SD) rats as the animal model [5].

Carbon tetrachloride (CCl4) is a strong oxidant for the production of chemical hepatic injury [12,13]. CCl4 is transformed to trichloromethyl free radicals and these active free radicals are capable of attacking cellular macromolecules such as lipids, proteins, and DNA [14,15]. It has been reported that CCl4 can decrease the antioxidant enzymes activities in the liver of rats, including superoxide dismutase, glutathione peroxidase, and glutathione reductase activities [16,17]. Intoxication with CCl4 causes cellular necrosis, oxidative stress and inflammation, which leads to hepatic damages, such as fibrosis, cirrhosis, and atrophy [18].

Preheating treatments have been found to enhance the antioxidant activity in the extracts from black soybean. The water extract from black soybean baked at 130°C for 5 min showed higher total anthocyanin content and higher antioxidant activity than the water extract from un-preheated black soybean [19]. Such preheating processes are considered to increase the extractability of anthocyanin from black soybean. In this study, pre-baked (at 130°C for 5 min) whole black soybean was submerged in 100°C hot water for 20 min to produce a decoction. The liver protective function of the black soybean decoction was evaluated using carbon tetrachloride treated SD rats.

Materials and Methods

Chemicals

Carbon tetrachloride (CCl4) and silymarin were purchased from Sigma Co. (St. Louis, MO). Glutathione disulfide (GSSG), glutathione reductase (GR), nicotinamide adenine dinucleotide phosphate (NADPH), glutathione (GSH) and N-ethylmaleimide were purchased from Wako Pure Chemical Industries (Osaka, Japan). Hydrodrogen peroxide and cumene hydroperoxide were purchased from Alfa Aesar (Heysham, UK). Total protein biuret reagent was purchased from thermo (Rockford, IL, USA).

Preparation of Black Soybean Tea (BST)

Black soybean (Glycine max (L.) Merrill, Tainan No. 3) was purchased from a local farmer in Chiayi county, Taiwan, ROC. After washing, whole black soybean was put in an aluminum pan (20*15*1.5 cm) and preheated in an oven (model SO-1199, Sunpentown, Taipei, Taiwan) at 130°C for 5 min. A digital pocket thermometer (model DGS-A9SA-ST9215C, Dogger Co., Taipei, Taiwan) was used to monitor the environmental temperature around the black soybean. Preheated black soybean was then submerged in 10 times (w/v) of 100°C hot distilled water for 20 min. After removing the bean, the decoction was served as the sample for animal treatments.

Experimental Animals

Six-month old male Sprague-Dawely (SD) rats were purchased from Biolasco Taiwan Co., Ltd. (I-Lan, Taiwan). The rats were housed in stainless wire-bottom cages in an environmentally controlled room (22 ± 2°C, 65 ± 5% relative humidity) with a 12 hr night and dark cycle. During the experiment, the rats were fed with a regular diet (Fu-So pellet chow, Taichung, Taiwan) and water ad libitum. The body weights were recorded weekly. This study protocol was approved by the Animal Research Ethics Committee at Providence University, Taichung, and Taiwan ROC.

Forty-eight rats were randomly divided into six groups, eight rats each. They were: control (the regular diet), high BST (1 g BS/ kg bw), CCl4 (0.5 ml 20% CCl4/olive oil), CCl4 + silymarin (0.5 ml 20% CCl4/olive oil + 0.2 g silymarin/kg bw), CCl4 + low BST (0.5 ml 20% CCl4/olive oil + BST at 0.1 g BS/kg bw) and CCl4 + high BST (0.5 ml 20% CCl4/olive oil + BST at 1 g BS/kg bw). For the groups that CCl4 was required (CCl4 + silymarin, CCl4 + low BST and CCl4 + high BST), the rats received an intraperitoneal injection of 0.5 mL CCl4 (20% CCl4/olive oil) twice a week for 9 weeks. The control and CCl4 group received distilled water every day for 9 weeks; while high BST, CCl4 + silymarin, CCl4 + low BST and CCl4 + high BST groups received BST (1 g BS/kg bw), silymarin (0.2 g/kg bw), BST (0.1 g BS/kg bw) and BST (1 g BS/kg bw) everyday, respectively.

At week 1, 3, 6 and 9, blood samples were collected in blood tube and then were centrifuged at 4°C for 10 min. After centrifugation, the supernatant were collected for blood biochemical analyses. After 9 weeks, the rats were fasted for 24 h and sacrificed via cervical dislocation. The livers were immediately collected, washed and weighted. For antioxidant enzyme activity measurements, 1 g of liver tissue was homogenized with 1 ml 0.05 M phosphate buffer (pH 7.4) at 4°C, 13000 rpm for 10 min. The dissected livers were immediately fixed in 6% formaldehyde for specimen preparation and histochemical staining analysis.

Measurement of Superoxide Dismutase (SOD) Activity

The superoxide dismutase (SOD) activity was measured using the method reported by Marklund and Marklund with a slight modification [20]. One hundred microliters of the liver supernatant was mixed with1 mL of a 0.05 M Tris–HCl and 7 μl of l50 mM pyrogallol, and then incubated at 25°C for 10 min, then the activity was measured at 325 nm with a spectrophotometer (model U-2800, Hitachi). One unit was determined as the amount of enzyme that inhibited the oxidation of pyrogallol by 50%.

Measurement of Catalase (CAT) Activity

The CAT assay was carried out by the method reported by Aebi [21]. Liver homogenate from all groups were taken with 1.9 ml of phosphate buffer (pH 7.4), and the reaction was initiated by adding of 1 ml of H2O2 (30 mM). Blank without liver homogenate was prepared with 2.9 ml of phosphate buffer and 1 ml of H2O2. The decrease in optical density due to the decomposition of H2O2 was measured at the end of 1 min against the blank at 240 nm.

Measurement of Glutathione Peroxidase (GPx) Activity

The activity of glutathione peroxidase was measured by a modification of the method of Paglia and Valentine [22]. The oxidation of NADPH was recorded as the decrease in absorbance at 340 nm with a spectrophotometer (model U-2800, Hitachi). The assay mixture contained 620 μl 0.25 M phosphate buffer (pH7.4), 200 μl 5 unit/ml GR, 50 μl 40 mM GSH, 100 μl liver supernatant, 10 μl 20 mM NADPH and 20 μl 15 mM cumene hydroperoxide.

Measurement of Glutathione Reductase (GR) Activity

Determination of GR activity was performed by a modification of the method of Paglia and Valentine [22]. The assay mixture contained 30 μl liver homogenate, 750 μl GSSG and150 μl NADPH, then the activity was measured at 340 nm with a spectrophotometer (model U-2800, Hitachi).

Determination of GSH and GSSG Contents

GSH content was determined by a modification of the method of Hissin and Hilf [23]. To 0.5 ml of the 10,000 g supernatant, 4.5 ml of the phosphate-EDTA buffer, pH 8.0, was added. The final assay mixture (2.0 ml) contained 100 μl of the diluted tissue supernatant, 1.8 ml of phosphate-EDTA buffer, and 100 μl of the OPT solution, containing 100 μg of OPT. After thorough mixing and incubation at room temperature for 15 min, the solution was transferred to a quartz cuvette. Fluorescence at 420 nm was determined with the activation at 350 nm.

GSSH content was also determined using the method reported by Hissin and Hilf [23]. A 0.5 ml portion of the original 10,000 g supernatant was incubated at room temperature with 200 μl of 0.04 M NEM for 30 min to interact with GSH present in the tissue. To this mixture, 4.3 ml of 0.1 N NaOH was added. A portion of this mixture (100 μl) was taken for measurement of GSSG, using the procedure outlined above for GSH assay, except that 0.1 N NaOH was employed as diluent rather than phosphate-EDTA buffer.

Determination of Malondialdehyde (MDA) Content

MDA determination was performed according to the method of Tatum et al. [24]. To liver homogenate, 0.4% TBA and 75 μl 0.2% BHT was added, and then the mixture was vigorously agitated in a vortex and placed in a boiling water bath for 45 min. After cooling, to 500 μl of the 10,000 g supernatant, 1000 μl n-butanol was added. After thorough mixing and incubation at room temperature for 10 min, the mixture was centrifuged at 10,000 g for 10 min. The supernatant was transferred to a quartz cuvette. Fluorescence at 550 nm was determined with the activation at 515 nm.

Determination of tissue protein concentration

The tissue protein concentration was estimated according to the method of Lowry et al using bovine serum albumin as the standard [25].

Histopathology Analysis

The liver samples were paraffin-embedded for histological analysis. Hematoxylin-eosin (HE) stain was performed.

Statistical Analysis

One-way analysis of variance (one-way ANOVA) was conducted using a package (SAS Institute Inc., Cary, NC). Duncan’s multiple ranges test was used to determine the significant difference between different treatments.

Results and Discussion

The Effects of CCl4 and BST on the Body Weight and Liver Weight of SD Rats

Figure 1A shows the change of body weight in SD rats during 9 weeks experimental period. It was found that CCl4 group had significantly lower body weight than the control group at 3 week and after. In this study, CCl4 was used as a strong oxidant to induce liver damage in SD rats. Therefore, the decline of the body weight was considered as the damage induced by CCl4. Hsu et al. used 8% CCl4 (1 ml CCl4/kg bw) to induce liver damage in male Wistar rats and they found no significant difference in the body weight between CCl4 treated and normal rats [18]. However, Li et al. and Lin et al. stated that CCl4 significantly decreased the body weight of male Wistar rats [26,27]. In our case, we found that CCl4 treated SD rats had diarrhea problem which might result in the decline of body weight. The administration of BST at 1 g BS/kg bw alone or co-treatment of BST at 0.1 g BS/kg bw or 1 g BS/kg bw with CCl4 resulted in similar body weight profile with the control group, indicating that co-treatment of BST could reduce the damage caused by CCl4.

botanical-sciences-body-weight

Figure 1. Changes of body weight (A) in SD rats fed with different experimeral diets for 9 weeks ( imagecontrol, image high BST (1 g BS/kg bw), image CCl4, image CCl4+Silymarin (0.2 g/kg bw, image CCl4+ low BST (0.1 g BS/kg bw), image CCl4+ high BST (1 g BS/kg bw) and the liver weight (B) of SD rats in week 9.

At the end of 9 weeks experimental period, SD rats were sacrificed and the liver tissues were collected for testing. The liver weights of SD rats increased significantly by CCl4 treatment. It was found that the liver weight in CCl4 group was about twice of the control group (Figure 1B). Our data indicated that co-treatment of BST at 0.1 g BS/kg bw or 1 g BS/kg bw with CCl4 decreased the liver weight, and showed no significant difference with the control group.

The Effects of CCl4 and BST on GOT and GPT Levels of SD Rats

Direct evidences of liver damage were associated with the increases of serum GOT and GPT levels in CCl4 treated SD rats. Compare to the control group, GOT level in CCl4 group increased 26%, 66%, 223% and 402% at week 1, 3, 6 and 9, respectively (Table 1). GPT level in CCl4 group also increased 26%, 74%, 275% and 805% at week 1, 3, 6 and 9, respectively. The data indicated that CCl4 induced severe liver damage in SD rats at week 6 and 9. However, co-treatment of BST at 0.1 g BS/kg bw or 1 g BS/kg bw completely recovered both the GOT and GPT levels; there were no significant differences (p>0.05) in those levels between the co-treatment group and the control group. The recovery effect of BST was similar to a well known liver protective agent, silymarin, at 0.2 g/kg bw in CCl4 treated SD rats.

Treatments GOT (U/L)
  Week 1 Week 3 Week 6 Week 9
control 141.4 ± 10.05c 134.0 ± 5.03b 130.6 ± 13.70b 97.1 ± 9.75b
high BST 133.9 ± 9.34c 121.0 ± 11.25b 126.1 ± 10.02b 76.6 ± 6.53b
CCl4 178.6 ± 12.62a 222.3 ± 40.79a 420.6 ± 107.15a 487.7 ± 76.32a
CCl4+Silymarin 148.3 ± 14.28bc 138.4 ± 5.29b 151.0 ± 5.16b 103.3 ± 13.14b
CCl4+low BST 159.9 ± 27.72b 138.6 ± 7.09b 147.9 ± 7.90b 105.7 ± 11.21b
CCl4+high BST 141.1 ± 7.99c 139.7 ± 28.56b 149.0 ± 7.05b 104.0 ± 10.39b
Treatments GPT(U/L)
  Week 1 Week 3 Week 6 Week 9
control 49.9 ± 9.92b 43.6 ± 3.69c 45.9 ± 3.89b 34.3 ± 2.14b
high BST 47.1 ± 7.20b 43.0 ± 3.61c 41.9 ± 4.45b 32.1 ± 2.41b
CCl4 62.6 ± 8.79a 75.1 ± 19.66a 169.6 ± 57.87a 308.6 ± 47.82a
CCl4+Silymarin 52.0 ± 12.69ab 61.0 ± 10.58b 58.1 ± 6.20b 43.3 ± 5.71b
CCl4+low BST 53.6 ± 9.16ab 61.0 ± 10.39b 54.4 ± 8.50b 44.9 ± 7.13b
CCl4+high BST 53.3 ± 8.79ab 63.3 ± 11.87ab 52.3 ± 4.11b 45.6 ± 7.89b

Table 1: Effect of BST on the activities of serum GOT and GPT in CCl4-treated rats at 1, 3, 6 and 9 weeks.

The Effects of CCl4 and BST on Blood Lipids of SD Rats

The effects of CCl4 and BST on serum triglyceride and cholesterol levels in SD rats are shown in Table 2. Compared to the control group, CCl4 caused 32% decrease in the triglyceride level at week 9. It was possible that CCl4 reduced the formation of very low-density lipoprotein (VLDL) in endoplasmic reticulum of the liver, thus it prevented the transfer of triglyceride to blood and resulted low serum triglyceride level in the blood system [28]. The co-treatment of BST at 0.1 g BS/kg bw or 1 g BS/kg bw recovered the triglyceride level in CCl4 treated SD rats. Hsu et al. also found that CCl4 reduced 28% triglyceride level in male Wistar rats [16]. However, our data showed that CCl4 did not differ cholesterol level in SD rats. BST also showed no significant effect on the cholesterol level in normal or CCl4 treated SD rats.

Treatments Cholesterol (mg/dL)1
  Week 1 Week 3 Week 6 Week 9
control 85.5±11.05 75.4±8.19 68.5±5.98 61.0±11.34
high BST  94.4±13.65 81.8±11.07 73.8±14.85 59.9±5.17
CCl4 85.3±17.77 75.5±10.03 70.4±23.26 73.9±13.38
CCl4+Silymarin 91.1±18.60 74.9±6.10 61.3±7.25 66.9±6.77
CCl4+low BST 95.8±13.13 76.3±6.32 69.6±10.93 70.3±13.02
CCl4+high BST 84.1±15.16 74.9±11.95 67.6±4.34 64.4±12.15
Treatments Triglyceride (mg/dL)
  Week 1 Week 3 Week 6 Week 9
control 107.9 ± 54.46a 135.6 ± 101.86a 104.0 ± 17.55a 76.8 ± 16.45ab
high BST 101.8 ± 34.69ab 141.6 ± 43.06a 112.8 ± 10.81a 86.8 ± 5.39a
CCl4 72.3 ± 17.62ab 95.3 ± 45.27ab 102.9 ± 18.67ab 52.4 ± 9.10c
CCl4+Silymarin 101.4 ± 42.93ab 87.3 ± 21.48ab 90.4 ± 9.59bc 68.9 ± 19.33b
CCl4+low BST 67.8 ± 19.83b 57.0 ± 16.52b 80.3 ± 6.88c 63.3 ± 15.40bc
CCl4+high BST 75.6 ± 25.15ab 64.0 ± 14.71b 90.8 ± 2.43bc 67.0 ± 13.16bc

Table 2: Effect of BST on the activities of serum cholesterol and triglyceride in CCl4-treated rats at 1, 3, 6 and 9 weeks.

The Effects of CCl4 and BST on Antioxidant Status of SD Rats

SD rats with the administration of BST alone at 1 g BS/kg bw had higher SOD, GPx and GR activities in the liver tissue than the control group, but no significant difference was found in the catalase activity (Figure 2A-2D). However, CCl4 treatment declined SOD, GPx, GR and catalase activities in the liver tissue. Co-treatment of BST at 0.1 g BS/kg bw or 1 g BS/kg bw increased all antioxidant enzymes activities in the liver tissue of CCl4 treated SD rats. The data indicated that the administration of BST enhanced antioxidant enzymes activities in both normal and CCl4 treated liver tissue of SD rats.

botanical-sciences-glutathione-peroxidase

Figure 2. Superoxide dismutase (SOD) activity (A), catalase (CAT) activity (B), glutathione peroxidase (GPx) activity (C) and glutathione reductase (D) (GR) activity in the liver tissue of normal and liver-damaged SD rats fed with different experimental diets for 9 weeks.

GSH and GSSH contents in liver tissue of SD rats are shown in Figure 3A and 3B respectively. The administration of BST alone at 1 g BS/kg bw significantly increased both GSH and GSSH contents in the liver tissue than the control group. The rates of increase were 77% and 72% for GSH and GSSH, respectively. Using CCl4 to induce liver damage, it was found that both GSH and GSSH contents in CCl4 group were only about 31% of the control group. Compare to CCl4 group, the co-treatment of BST showed significant higher GSH and GSSH levels in the liver, regardless the concentration of 0.1 g BS/kg bw or 1 g BS/kg bw. The data indicated that the administration of BST alone enhanced both GSH and GSSH contents in the liver, BST could also raise both GSH and GSSH contents in the liver tissue of CCl4 treated SD rats. It is well known that both GSH and GSSH played important roles in the defense system for oxidative stress; our results indicated that BST could enhance the antioxidant status in the liver tissue of SD rats.

botanical-sciences-malondialdehyde

Figure 3. GSH content (A), GSSG content (B) and malondialdehyde (MDA) content (C) in the liver tissue of normal and liver-damaged SD rats fed with different experimental diets for 9 weeks.

The free radicals derived from CCl4 might cause peroxidation of the membrane lipid and subsequently disrupt membrane integrity [19]. Measurement of malondialdehyde content is often used as an index for lipid peroxidation in cell or animal model. The malondialdehyde level in CCl4 group was twice of that in the control group (Figure 3C). While, co-treatment of BST at 0.1 g BS/kg bw or 1 g BS/kg bw significantly reduced the malondialdehyde level in the liver tissue of CCl4 treated SD rats.

The Effects of CCl4 and BST on the Liver Histopathology of SD Rats

Liver histopathology revealed that liver sections from the control and BST treated rats showed normal liver architecture, but CCl4 induced serious fatty liver and liver fibrosis in SD rats (Figure 4). Co-treatment of BST at 0.1 g BS/kg bw or 1 g BS/kg bw prevented the development of histopathological changes induced by CCl4. The percentages of fat acumination in the liver for the control group and BST alone groups were 0%, for CCl4 group was 33~66%, and for co-treatment of silymarin or BST at 0.1 g BS/ kg bw or 1 g BS/kg bw was less than 10%. The data indicated that CCl4 group showed serious fatty liver, while co-treatment of silymarin or BST group had slight fatty liver. Metavir score revealed that the level of liver fibrosis in CCl4 treated SD rats was rigid, while the other groups did not show any sign of fibrosis.

botanical-sciences-Hematoxylin-eosin

Figure 4. Sections of the liver of SD rats staining with Hematoxylin-eosin (HE) (×600).

Our results showed that co-treatment of BST could reduce the lipid peroxidation, enhance the antioxidant enzyme activities, recover serum GOT and GPT levels, decrease the liver weight and increase the body weight in CCl4 treated SD rats. Histopathology analysis also showed that co-treatment of BST could significantly recover the fatty liver and liver fibrosis in CCl4 treated SD rats. It demonstrated, for the first time, that BST could reduce the liver damage caused by CCl4. Treatment of BST alone also enhanced GSH and GSSH contents, as well as antioxidant enzymes activities (SOD, GPx and GR activities) in the liver tissue, while maintained normal liver weight and body weight, normal GOT and GPT levels and normal liver architecture. In general, the protective effect of BST was similar to that of silymarin at the level of 0.2 g/kg bw. Therefore, BST could be considered as a potential liver protective agent.

It is worth to mention that BST was prepared simply by immerging preheated black soybean in 100°C hot water for 20 min. The concentrations of BST used in this study were 0.1 g BS/kg bw and 1 g BS/kg bw, and the amount of BST was based on the weight of whole black soybean, not the weight of the extract from black soybean. It is possible that the extracts from black soybean may have better liver protective function than BST; in other words, lower concentrations may be enough for the extracts to achieve the same effect as BST. Therefore, the application of proper extraction techniques to obtain the active compounds in black soybean is important and requires further investigation.

Anthocyanins are the main biological compounds in the seed coat of black soybean currently receiving many attentions. And cyanidin-3-O-glucoside (C3G) is the main anthocyanin in the seed coat of black soybean [12]. It has been reported that administration of a pure C3G attenuates the levels of serum aspartate aminotransferase and alanine aminotransferase and reduces the incidence of liver lesions in CCl4-treated mice. C3G apparently protects the liver from CCl4-induced hepatic damage through antioxidant and anti-inflammatory mechanisms [11]. In this study, BST shows significant protective effect against CCl4 induced liver damage in rats. BST could release CCl4 induced oxidative stress by enhancing antioxidant enzymes activities. And this may be due to the antioxidant activity of C3G.

Acknowledgement

This research was partially supported by Ministry of Science and Technology, Taiwan, ROC. (NSC 102-2313-B-415-009).

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