Introduction
Alcohol is one of the most commonly consumed beverages by humans. However, excessive consumption of alcohol affects the immune system, alters cytokine production, increases liver triglycerides and lipid peroxidation, and causes many diseases, including alcoholic liver disease (ALD) [28]. Alcoholic liver disease poses a major threat to human health worldwide. When ALD progresses, it progresses to fatty liver (steatosis), fatty hepatitis, fibrosis/cirrhosis, and eventually it is a terrible disease that can lead to liver carcinoma [1]. ALD is known to occur due to overproduction of reactive oxygen species (ROS), lipid peroxidation damage, cytokine damage and inflammation. If inflammation continues, it induces cell death due to apoptosis and necrosis and stimulates ROS production, which is an important factor in the progression of alcoholic liver disease [11]. Also, ALD is associated with increased ROS levels resulting from cytochrome P450 2E1 (CYP2E1). CYP2E1 plays an important role in the production of ROS by alcohol in the liver and other tissues. CYP2E1 expression causes alcohol-dependent metabolic changes and trigger steatosis and fatty hepatitis in early liver damage. And CYP2E1 is known to be a toxic and carcinogenic substance [18,26]. Ethanol treatment in an in vivo model expresses the genes of the JNK pathways [6]. The JNK signaling pathway is activated by pro-inflammatory cytokines such as TNF-α and IL-1β [5]. This increase in inflammation continues to phosphorylate JNK, eventually leading to apoptosis, and further causing liver damage [15,20].
In a previous study, HepG2 cells were treated with ethanol to increase inflammatory cytokines such as TNF-α, which increases ROS, CYP2E1 is expressed, and JNK is activated, eventually promoting apoptosis [3,10,13,31]. From this, it seems that ethanol-induced liver damage is caused by ROS, inflammation, and CYP2E1 and phosphorylation of JNK. Thus, inhibition of CYP2E1, an inflammatory cytokine, activity or expression can interfere with ethanol metabolism and improve alcoholic liver disease. RYR (Red Yeast Rice) is a dark pink rice made by fermenting ordinary rice together in a fungus named Monascus purpureus for 15 to 30 days, and has long been used as a medicine in China [7,17]. RYR contains monacolin K as a potent inhibitor of HMG-CoA reductase and its consumption is known to decreases cholesterol and triglyceride levels [8,19]. RYR is produced many functional secondary metabolites and main 6 type pigments [19]. It is known that monacolin K, γ-aminobutyric acid (GABA), various pigments (yellow pigments, ankaflavin and monascin; orange pigments, monascorubrin and rubropunctanin; red pigments, monascorubramine and rubropuctamine) etc. are active substances of Monascus purpureus [21]. In previous studies have shown that Monascus purpureus extract has protective activity against alcoholic liver disease in animal models [14]. But it has not been proven through what mechanism the RYR extract is effective against alcoholic liver disease and gut leakiness. The present study aims to investigate the protective effects mechanism of RYR extract against ethanol-induced gut leakiness and liver injury.
Material and Methods
Materials
In this study, RYR was purchased from Han’s Bio (Andong, Republic of Korea). The RYR extract was prepared by extracting RYR powder and 70% ethanol at a ratio of 1:10 (w/w) for 24 hr at room temperature. Then the extraction was filtered through glass funnel and filter paper. Each filtrate was concentrated to dryness under reduced pressure using a rotary flash evaporator. The concentrated sample was freeze-dried for 72 hr.
Experimental animals
Male C57BL/6N mice (5-week-old, 23.9±1.0 g body weight) were purchased from Orient Bio (Seongnam, Korea) and housed in cages under automatically controlled conditions of temperature (22±2℃), humidity (30~70%), and lighting (12: 12 hr light–dark cycle). With food and water provided ad libitum. Andong National University’s Institutional Animal Care and Use Committee approved the protocol for the animal study (The animal protocol number is 2019-2-0510-02-01), and the animals were cared for in accordance with the “Guidelines for Animal Experiments” established by the university.
Animal treatments
The 5-weeks old male C57BL/6 mice kept in their cages for 7 days prior to dosing to allow for acclimatization to the laboratory conditions. For the in vivo hepatoprotective test against ethanol-induced oxidative stress, 40 mice were divided into four groups (n=10 per group). Age matched 6-weeks old male C57BL/6 mice were orally administered test materials i) CON; mice received distilled water, ii) EtOH; After distilled water pretreatment for 10 days, mice was exposed to 3 oral doses of binge alcohol (5 g/kg/dose) at 12 hr intervals. iii) RYR+EtOH; After 200 mg/kg RYR pretreatment for 10 days, mice were exposed to 3 oral doses of binge alcohol (5 g/kg/dose) at 12 hr intervals. iv) SM+EtOH; After 800 mg/kg Silymarin pretreatment for 10 days, mice were exposed to 3 oral doses of binge alcohol (5 g/kg/dose) at 12 hr intervals. Each group was administered 10% volume (10 ml/kg) of distilled water or silymarin and RYR daily through gastric intubation for 10 days, and alcohol was administered three times at 12 hr intervals. At the end of the experiment, the mice were sacrificed to collect serum and liver 1 hr after final administration of alcohol.
Histological analysis
Mice was briefly sedated to carbon dioxide gas followed by decapitation and immediate collection of liver from each mice. In this study, part of the largest liver lobe from each mice exposed to RYR pretreatment or control with or without binge ethanol exposure was fixed in neutral formalin. Paraffin embedded blocks of formalin-fixed individual liver or small intestine sections were cut at 4 µm, stained with hematoxylin/eosin (H/E) by American Histolabs, Inc. (Gaithersburg, MD). To further support fat accumulation, frozen liver samples embedded in optimal cutting temperature compound were cut (10 µm) and stained with Oil Red O.
Endotoxin assay
Plasma endotoxin levels were determined using the commercially available endpoint LAL Chromogenic Endotoxin Quantitation Kit with a concentration range of 0.015~1.2 EU/ml (Thermo Fisher Scientific, Waltham, MA as described [12].
Triglyceride determination in liver and plasma AST/ALT measurement
The amounts of hepatic triglyceride (TG) were assessed by using a commercially available kit (Asan Co., Ltd, Gimpo, South Korea).
Serum alanine aminotransferase (ALT) and asparate aminotransferase (AST) activities in each mice was determined by using the standard end-point colorimetric assay kit (Asan Co., Ltd, Gimpo, South Korea) as described [12]
Western blot analyses
Liver tissue was homogenized in buffer containing 0.5% Triton X-100 and protease inhibitor cocktail (1:1,000, Sigma-Aldrich Chemical Co.). Then, the lysates were centrifuged at 12,000 rpm for 30 min at 4℃. The SMART BCA Protein Assay Kit (iNtRON Biotechnology, Seongnam-si, Republic of Korea) was used to measure protein concentration. This homogenate was further mixed with buffer (60 mM Tris–HCl, 2% SDS and 2% β-mercaptoethanol, pH 7.2), and boiled for 5 min. The 60 μg of the protein was electrophoresed by SDS-PAGE, transferred to a nitrocellulose membrane, and blocked with 5% non-fat dry milk in 1×Tris buffered saline containing 0.05% Tween-20 (TBST) at room temperature for 1 hr. After that, the membranes were incubated with the appropriate mouse anti-CYP2E1 (1:1,000), anti-iNOS, anti-P-JNK, anti-P-BAX (1:1,000) primary antibody on a rocker at 4℃ overnight. After overnight incubation, membranes were washed with TBST and probed with horseradish peroxidase-conjugated secondary antibody at room temperature for 2 hr. For visualization, the membranes were incubated with Enhanced Chemiluminescence reagents (Dogen, Seoul, South Korea) and analyzed by using Chemi-Doc (Vilver, France).
Statistical analysis and other methods
The effect of each treatment was analyzed from 10 mice (n=10) in each group. All data were expressed as mean ± standard deviation (SD). Statistical significance was determined using one-way ANOVA and Dunnet's multiple comparison post-tests were used to compare the means of different groups. All the experiments were repeated at least twice unless otherwise stated. Data were presented as mean ± SD. Different letters in actual figures stand for significant difference between various treatments at p<0.05 by one-way ANOVA.
Results
RYR ameliorates liver injury in binge alcohol exposed mice
H&E staining showed markedly elevated fat accumulation in the liver after binge alcohol-exposure (Fig. 1A, Fig. 1B). However, RYR or SM treatment prevented the hepatic fat accumulation. Our results showed that plasma ALT and AST levels elevated in binge alcohol induced liver injury (Fig. 1C, Fig. 1D). However, pretreatment with RYR and SM significantly suppressed ethanol-induced increases in these serum ALT and AST. RYR and SM also inhibited hepatic TG elevated by binge alcohol exposure (Fig. 1E). Therefore, liver injury by binge alcohol is prevented with the pretreatment RYR.
Fig. 1. RYR prevented binge alcohol-induced fatty liver injury in mice. (A) Representative H&E staining of formalin-fixed or frozen liver sections for control (CON), ethanol (EtOH), after 200 mg/kg RYR pretreatment for 10 days, mice were exposed to 3 oral doses of binge alcohol (5 g/kg/dose) at 12 hr intervals (RYR+EtOH), or after 800 mg/kg Silymarin pretreatment for 10 days, mice were exposed to 3 oral doses of binge alcohol (5 g/kg/dose) at 12 hr intervals (SM+EtOH) mouse groups. (B-E) The levels lipid droplet, plasma ALT, AST, and hepatic triglyceride (TG) are shown. Data represent means±SD. Significances between values for each group were determined using ANOVA and Tukey’s HSD test. EtOH; ethanol, RYR; red yeast rice, SM; silymarin.
RYR prevents the elevation of hepatic oxidative stress and apoptosis marker proteins in binge alcohol-exposed mice
Cytochrome P450 2E1 (CYP2E1) causes oxidative stress and hepatotoxicity by binge and chronic alcohol. Our data showed that hepatic oxidative stress maker proteins were significantly increased in binge alcohol-exposed mice. However, RYR and SM treatments reduced the elevation of the hepatic oxidative stress maker proteins (Fig. 2A).
Fig. 2. RYR prevented hepatic oxidative stress and apoptosis maker proteins in binge alcohol exposed mice. (A) The levels of hepatic CYP2E1 and iNOS in the indicated groups are presented. (B) The levels of hepatic p-JNK and BAX in the indicated groups are presented. Densitometric quantitation of the immunoblots for each protein relative to β-actin is shown. Data represent means ± SD. Significances between values for each group were determined using ANOVA and Tukey’s HSD test. CON; control, EtOH; ethanol, RYR; red yeast rice, SM; silymarin.
RYR and SM has been shown to protect the liver injury by decreased levels of hepatic apoptosis caused by alcoholic hepatotoxicity (Fig. 2B). These results show that RYR significantly inhibited the oxidative stress and apoptosis of hepatic damage in bine alcohol exposed mice.
RYR inhibits binge alcohol induced gut leakiness
H&E stained histology revealed disorganization and detachment of many intestinal epithelial cells in binge alcohol-exposed mice (Fig. 3A). Both RYR and SM pretreatment significantly prevented the abnormal villi structure caused by ethanol exposure. Consistently, binge alcohol exposure markedly elevated the plasma endotoxin concentration compared to the control mice, whereas RYR and SM pretreatment significantly attenuated the elevation of endotoxin (Fig. 3B).
Fig 3. RYR prevented binge alcohol-induced small intestine injury and elevated the plasma endotoxin in mice. (A) Representative H&E staining of formalin-fixed or frozen small intestine sections for control (CON), ethanol (EtOH), RYR+EtOH, or SM+EtOH mouse groups. (B) The levels plasma endotoxin is shown. Data represent means ± SD. Significances between values for each group were determined using ANOVA and Tukey’s HSD test. CON; control, EtOH; ethanol, RYR; red yeast rice, SM; silymarin.
RYR prevents the elevation of intestinal oxidative stress and apoptosis marker proteins in binge alcohol-exposed mice
Oxidative stress maker iNOS was markedly elevated in binge alcohol exposed mice. However, RYR and SM pretreatment reduced the iNOS protein expression (Fig. 4A). RYR has been shown to protect the gut leakiness by decreased levels of intestinal apoptosis caused by binge alcohol induced gut leaky (Fig. 4B). These results show that RYR significantly inhibited the oxidative stress and apoptosis of gut damage in bine alcohol exposed mice.
Fig. 4. RYR reduced the elevation of oxidative stress and apoptosis maker proteins in binge alcohol-mediated gut damage. (A) The levels of intestinal iNOS in the indicated groups are presented. (B) The levels of intestinal p-JNK and BAX in the indicated groups are presented. Densitometric quantitation of the immunoblots for each protein relative to β-actin is shown. Data represent means ± SD. Significances between values for each group were determined using ANOVA and Tukey’s HSD test. CON; control, EtOH; ethanol, RYR; red yeast rice, SM; silymarin.
Discussion
Excessive ethanol exposure causes various ethanol metabolic reactions in the liver [29]. Binge ethanol exposure is known to have a significant impact on immunity, but it is not known exactly. Alcoholic liver disease (ALD) caused by binge ethanol is known to increase human or mouse inflammation, increasing the mortality rate from complications [23,28]. Many studies have shown that oxidative stress and inflammation have played an important role in the development of ALD and that compounds with antioxidant or anti-inflammatory activity improve the progression of ALD in animal models [2,9,12]. RYR is known to be effective for liver-related diseases such as ALD and arteriosclerosis [33]. Therefore, in this study was to investigate the anti-inflammation effect of RYR on the improvement of binge alcohol induced liver and gut injury.
The clinical spectrum of alcoholic liver disease (ALD) includes an increased risk of alcoholic fatty liver (AFLD), steatohepatitis (ASH), and hepatocellular carcinoma [12]. Alcoholic fatty liver is caused by excessive fatty acid synthesis and is characterized by deposition of TG in the liver [24]. The effects of RYR treatment were confirmed by the H&E staining microscopic histological characterization in liver tissue. In addition, a significant increase in plasma ALT, AST and liver TG level was observed in the binge-alcohol model. Treatment of RYR (200 mg/kg B.W) on the alcohol induced mice normalized liver TG concentrations as well as plasma ALT and AST, liver function marker. Our observation suggests that RYR treatment can be effective against liver damage in binge alcohol.
Until now, continuous or excessive alcohol intake is well known to break down alcohol into acetaldehyde by alcohol dehydrogenase (ADH) and cytochrome P450 2E1 (CYP2E1), which are key enzymes that break down alcohol in the liver [4]. CYP2E1 is one of the major P450 forms both in human and rat liver that has been shown to be sensitive to inflammatory stimulus and cytokines both in vivo and in primary hepatocytes [25]. In particular, CYP2E1 is known to continuously induce reactive oxygen species (ROS) in the process of decomposing alcohol into acetaldehyde. ROS damages cells and it is a cause of toxicity and carcinogenicity [25]. In addition, which is well known as a major cause of liver damage that causes hepatitis [32,33]. The administration of RYR suggests that it can down-regulate oxidative stress markers, effectively remove apoptosis markers induced by binge alcoholic liver injury.
According to a recent study, binge alcohol intake causes gut leakiness, which causes an imbalance of the bacterial balance axis and secretes endotoxins into the blood [12]. Previous studies have shown that alcohol-induced hepatotoxicity is triggered by increased endotoxin delivery [27]. A distinctive feature of alcohol abuse is the disruption of the intestinal barrier. Animal models of ALD represent gut leaky, and impairment of intestinal barrier function were found in alcohol-dependent patients [16]. Alcohol has a direct effect on these functions of the gut and indirect effects by alcohol and/or alcohol metabolites distributed through the blood stream [22]. In addition, alcohol-induced lesion severity is positively correlated with Lipopolysaccharide (LPS) blood endotoxin [12]. Therefore, it is important to evaluate the beneficial effects of RYR on binge alcohol-induced gut intestinal leaks in animal model. In endotoxin level, the elevated plasma levels LPS were significantly reduced to control group levels due to RYR treatment. Protein expression of oxidative stress marker and apoptosis were significantly decreased in the RYR treated group compared to the EtOH group. In addition, the RYR treatment group showed a superior effect than the positive control group, silymarin treatment.
Our results show that RYR has been shown to be effective for binge alcohol by reducing oxidative stress in the liver and various apoptosis markers and protecting the gut leakiness. Therefore, it is suggested that RYR could be a potential remedy for the treatment of binge alcohol disease.
Acknowledgement
This work was supported by a Research Grant of Andong National University.
The Conflict of Interest Statement
The authors declare that they have no conflicts of interest with the contents of this article.
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