Basic Research Open Access
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World J Gastroenterol. Jul 21, 2006; 12(27): 4345-4351
Published online Jul 21, 2006. doi: 10.3748/wjg.v12.i27.4345
Influence of zinc sulfate intake on acute ethanol-induced liver injury in rats
Sema Bolkent, Sukriye Yildirim, Department of Medical Biology, Cerrahpasa Faculty of Medicine, Istanbul University, Cerrahpasa 34098, Istanbul, Turkey
Pelin Arda-Pirincci, Sehnaz Bolkent, Department of Biology, Faculty of Science, Istanbul University, Vezneciler 34459, Istanbul, Turkey
Refiye Yanardag, Sevim Tunali, Department of Chemistry, Faculty of Engineering, Istanbul University, Avcilar 34850, Istanbul, Turkey
Supported by the Research Fund of Istanbul University, No. UDP-324/03062004
Correspondence to: Dr. Sema Bolkent, Department of Medical Biology, Cerrahpasa Faculty of Medicine, Istanbul University, Cerrahpasa 34098, Istanbul, Turkey. bolkent@istanbul.edu.tr
Telephone: +90-212-4143000 Fax: + 90-212-6320050
Received: March 18, 2006
Revised: March 28, 2006
Accepted: April 21, 2006
Published online: July 21, 2006

Abstract

AIM: To investigate the role of metallothionein and proliferating cell nuclear antigen (PCNA) on the morphological and biochemical effects of zinc sulfate in ethanol-induced liver injury.

METHODS: Wistar albino rats were divided into four groups. Group I; intact rats, group II; control rats given only zinc, group III; animals given absolute ethanol, group IV; rats given zinc and absolute ethanol. Ethanol-induced injury was produced by the 1 mL of absolute ethanol, administrated by gavage technique to each rat. Animals received 100 mg/kg per day zinc sulfate for 3 d 2 h prior to the administration of absolute ethanol.

RESULTS: Increases in metallothionein immunoreactivity in control rats given only zinc and rats given zinc and ethanol were observed. PCNA immunohistochemistry showed that the number of PCNA-positive hepatocytes was increased significantly in the livers of rats administered ethanol + zinc sulfate. Acute ethanol exposure caused degenerative morphological changes in the liver. Blood glutathione levels decreased, serum alkaline phosphatase and aspartate transaminase activities increased in the ethanol group when compared to the control group. Liver glutathione levels were reduced, but lipid peroxidation increased in the livers of the group administered ethanol as compared to the other groups. Administration of zinc sulfate in the ethanol group caused a significant decrease in degenerative changes, lipid peroxidation, and alkaline phosphatase and aspartate transaminase activities, but an increase in liver glutathione.

CONCLUSION: Zinc sulfate has a protective effect on ethanol-induced liver injury. In addition, cell proliferation may be related to the increase in metallothionein immunoreactivity in the livers of rats administered ethanol + zinc sulfate.

Key Words: Liver, Ethanol, Zinc sulfate, Metallothionein, Proliferating cell nuclear antigen, Rat

INTRODUCTION

The liver is the main site of ethanol biotransformation and it plays a key role in zinc metabolism[1,2]. Acute ethanol exposure causes liver injury in experimental animals. The mechanisms of ethanol-induced liver injury are not fully elucidated[3,4]. Metallothionein is an intracellular protein capable of binding metals and can scavenge reactive oxygen species[5,6] . The mechanism of action for metallothionein is also unknown. Although all tissues are able to synthesize metallothioneins, the main place of synthesis is in the liver[7]. Ethanol is a potent inducer of liver metallothionein[8-12]. proliferating cell nuclear antigen (PCNA) is an essential protein in both DNA replication, DNA repair and possibly cell-cycle control[13]. Zinc is an essential nutrient that is required in humans and animals for many physiological functions, including antioxidant functions. Zinc has been shown to be essential for the structure and function of a large number of macromolecules and is also essential for over 300 enzymatic reactions[14]. Zinc is an antioxidative element and it probably mediates the protective action of metallothionein[15]. Changes in the metabolism of some elements such as zinc can lead to disorders in the antioxidant defense system of liver[16-17]. It has been shown that zinc plays an important role in the maintenance of glutathione[18]. Zinc deficiency is important in liver damage, although it is unclear whether zinc supplementation has a place in the treatment of ethanol-induced liver injury[19,20]. Although some studies have addressed the relationship between zinc-metallothionein and ethanol toxicity, the results obtained from these studies are in conflict[4,21,22]. The aim of this study was to examine the role of metallothionein and PCNA, and the effects of zinc sulfate on ethanol-induced liver injury morphologically and biochemically.

MATERIALS AND METHODS
Experimental design and treatment of animals

In this study, 2.5-3 mo-old male Wistar albino rats (n = 41) from DETAM (Istanbul University, Centre for Experimental Medical Research and Application) were used. The experiments were reviewed and approved by the Local Institute’s Animal Care and Use Committees. The animals were fed with pellet chow and tap water ad libitum. The animals were randomly divided into four groups. Group I (n = 8) was intact control animals. The control rats of group II (n = 8) were treated only with 100 mg/kg per day zinc sulfate (ZnSO4.7 H2O) (Merck) for 3 d, by gavage technique. The animals of group III (n = 14) received 1 ml of absolute ethanol once, by the same method. The animals of group IV (n = 11) were treated with zinc sulfate and absolute ethanol at the same dose and time. After 2 h from the time when the last dose of zinc sulfate was given, acute ethanol toxicity on the liver of rats was produced by administration of absolute ethanol. The animals were sacrificed by ether 2 h after treatment with absolute ethanol.

Morphological study

On the 3rd day of the experiment, all of the animals were fasted overnight and sacrificed under ether anesthesia. Liver samples were taken from the animals for morphological studies. The tissues were fixed with Bouin fixative for light microscopic studies and subsequently a routine paraffin embedding method was used. Liver sections of 5 µm thickness were stained by HE and Masson’s triple dyes (Masson), and examined under Carl Zeiss Ultraphot II microscope. Liver samples were fixed in 20 g/L glutaraldehyde and post-fixed in 10 g/L of phosphate-buffered osmium tetraoxide. The samples were dehydrated in ethanol and embedded in epon. Specimens were examined with JEM 1011.

Immunohistochemical study

Sections were dewaxed and rehydrated. The tissues were rendered permeable with 3 g/L Triton-X 100 for 10 min and then rinsed in phosphate-buffer saline (10 mmol/L, pH 7.5). For antigen retrieval, the slides were kept in 0.01Mol/L citrate buffer for 10 min in a microwave oven. Endogenous peroxidase was blocked with 30 mL/L hydrogen peroxide. An Ultra Vision Detection System for streptavidin-biotin-peroxidase technique (Lab Vision, USA) was employed. Sections were covered with blocking serum for 10 min to block non-specific binding sites. They were then incubated with metallothionein antibody for 1 h (Zymed Laboratories, USA) at room temperature with 1:50 dilution. Slides were then incubated with PCNA mouse monoclonal antibody for 30 min (Neomarkers, USA) at room temperature with 1:50 dilution. They were incubated for 15 min with biotinylated secondary antibody and then incubated with the streptavidin-peroxidase conjugate for 15 min. The enzyme activity was developed using aminoethylcarbazole (AEC) and then the sections were counterstained with hematoxylin. Negative control sections were prepared by substituting the metallothionein or PCNA antibodies with phosphate-buffer saline. Hepatocytes were viewed using a light microscope (Olympus, CX41) at a magnification of 400X. Approximately 400 cells from 10 randomly selected fields (0.0506 mm2 per field) of vision were counted. The PCNA and metallothionein labeling indices were expressed as a percentage of positive stained cells relative to the number of counted cells. (i.e., PCNA or metallothionein labeling index = PCNA or metallothionein positive hepatocytes/total hepatocytes per high power field ×100).

Biochemical study

In this study, biochemical investigation was carried out in serum, blood, and liver tissues. The blood samples were taken by a syringe from the heart. Blood glutathione (GSH) levels were measured according to the method of Beutler, Duron and Kelly using Ellman’s reagent[23]. Serum alkaline phosphatase activities (ALP) were determined by the Two Point method[24]. Serum aspartate transaminase (AST) was assessed by the Reitman-Frankel method [25]. The liver tissues were homogenized in cold 9 g/L saline by means of a glass homogenizer to make up a 100 g/L homogenate. The homogenates were centrifuged and the clear supernatants were used for GSH, lipid peroxidation (LPO) and protein levels. Liver GSH levels were determined according to Beutler’s method, using Ellman’s reagent[26]. Liver LPO levels were measured by Ledwozyw’s method[27], liver protein levels were assessed by Lowry’s method using bovine serum albumin as the standard[28].

Statistical analysis

The biochemical results were evaluated using an unpaired t-test and analysis of variance (ANOVA) using the NCSS statistical computer package (Kaysville, Utah, USA)[29]. The microscopic results were analyzed by one-way ANOVA followed by the Scheffe and Student’s t-test for multiple comparisons of the control against all other groups using SPSS 13 for Windows. Data were expressed as mean ± SD. P < 0.05 was considered to be significant.

RESULTS
Morphological results

The livers of control and zinc-treated rats were visually normal. Acute ethanol exposure caused degenerative morphological changes in the liver. The hepatocyte of rats exposed to absolute ethanol alone had occasional diffuse vacuolar degeneration. Vacuolar degeneration was found in hepatocytes of zones 2 and 3. In the alcohol group, there was a mild dilation of the sinusoids and hyperemia. Moreover, mononuclear cell infiltrations were evident in this group. These alcohol-induced hepatic pathological changes were significantly inhibited in the zinc-pretreated rats. A moderate degree of mucosal hyperemia was observed in the group given ethanol and zinc sulfate. In addition, less vacuolar degeneration was observed in this group (Figure 1).

Figure 1
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Figure 1 Histological appearance of rat liver tissue. Masson X 270. A: Intact control; B: Control, zinc sulfate; The liver showing vacuolated hepatocytes (→) in the centrilobuler area with mild dilation of sinusoids (►) and hyperemia (*); C: Absolute ethanol; D: Zinc pre-treatment.

An increase in hepatic metallothionein-producing cells in control rats given only zinc, when compared to intact controls, was observed. In addition, an increase in hepatic metallothionein-producing cells was observed in the rats given zinc and ethanol, when compared to the group given ethanol. Immunoreactive metallothionein-producing cells in the control group were rarely found to be scattered in lobular hepatocytes or around the periportal area. In the control rats given only zinc, more metallothionein-producing cells were observed in hepatocytes of zones 1 around the periportal area as compared with the control group. Metallothionein was observed significantly in the cytoplasm of cells by immunohistochemical staining in the rat livers of all groups. The intensity of immunoreactivity of metallothionein-producing cells in the group given ethanol and zinc was generally higher in hepatocytes of zones 1 compared to zones 2 (Figure 2). The metallothionein labeling index was determined to be 27.27% ± 2.02% in the group given zinc sulfate, while in intact control group the index was 2.44% ± 0.50%. The metallothionein labeling index was increased 55-fold in the group administered ethanol + zinc sulfate (26.32% ± 3.09%) compared to the group administered only ethanol (0.48% ± 0.19%) (aPt-test = 0.018). (Figure 3A)

Figure 2
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Figure 2 Immunreactive metallothionein-producing cells (►) in rat liver. Streptavidin-Biotin-Peroxidase x 270. A: Intact control; B: Control, zinc sulfate; The reduced metallothionein expression (►); C: Ethanol; Note the increase of immunoreactivity of metallothionein-producing cells, D: Ethanol + zinc sulfate; E: Intact control, PCNA-positive hepatocytes (►); F: Control, zinc sulfate; G: Ethanol; The increase in immunoreactivity of PCNA-positive cells, H: Ethanol + zinc sulfate.
Figure 3
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Figure 3 A: Metallothionein, aP = 0. 018 vs Ethanol; B: PCNA labeling indeces, bP = 0.007 vs Ethanol.

Hepatocyte proliferation was measured by immuno-histochemical identification of PCNA. The PCNA labeling index was determined to be 0.73% ± 0.17% in the intact control group and 0.32% ± 0.02% in the group given zinc sulfate. PCNA immunohistochemistry showed that the number of PCNA-positive hepatocytes was increased significantly in the livers of rats administered ethanol + zinc sulfate (2.40% ± 0.57%) compared to the group given only ethanol (0.19% ± 0.10%) (bPt-test = 0.007) (Figure 3B). However, according to semiquantitative evaluations, most of the PCNA-positive hepatocytes were in S phase of proliferation in all groups.

Ultrastructurally, proliferation of smooth endoplasmic reticulum, degenerative mitochondria, condensation of chromatin and increased lipid droplets were observed after alcohol treatment. However, administration of zinc sulfate caused a remarkable decrease in the lipid droplets, smooth endoplasmic reticulum, and mitochondria degeneration of the hepatocytes (Figure 4).

Figure 4
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Figure 4 Ultrastructure of the hepatocytes of the rat. TEM X5000. A: Control; B: Ethanol; C: Zinc sulfate + ethanol. An increase in smooth endoplasmic reticulum (SER), lipid vacuoles (L) and degeneration in mitochondria (M) of the hepatocyte of a rat given ethanol. These ultrastructural changes were improved by zinc pre-treatment.
Biochemical results

Blood GSH levels are presented in Table 1. From the obtained results, values of GSH in the blood of the group administered ethanol showed a significant decrease when compared to the control group (bPt-test = 0.0001). Also, a marked increase in blood GSH level was observed in the group administered ethanol + zinc sulfate when compared to the group administered ethanol (Pt-test = 0.005). According to Table 1, a significant difference in the blood GSH levels of four groups was observed (PANOVA = 0.0001).

Table 1 Blood glutathione and serum enzymes (mean ± SD).
GroupnGSH (mg %)Pt-testALP (U/L)Pt-testAST(U/L)Pt-test
Control852.59 ± 2.44101.12 ± 1.64122.55 ± 2.61
0.009
0.00010.001
Control + Zinc sulfate846.65 ± 4.9073.91 ± 6.28106.03 ± 8.97
Ethanol1435.09 ± 2.31b110.02 ± 2.88b133.00 ± 4.82b
0.0050.00010.0001
Ethanol + Zinc sulfate1138.39 ± 6.1884.80 ± 7.09112.56 ± 8.18
PANOVA0.00010.00010.0001
bPt-test = 0.0001 vs Control.

Serum ALP and AST activities are given in Table 1. From the obtained results, values of ALP in the serum of the group administered ethanol showed a notable increase when compared to the control group (bPt-test = 0.0001). Also a considerable decrease was noted in the group administered ethanol + zinc sulfate when compared to the group administered ethanol (Pt-test = 0.0001). According to Table 1, a significant difference in the ALP activities of the four groups were observed (PANOVA = 0.0001). In this study, a statistically marked increase was observed in serum AST activity of the group administered ethanol, in comparison with the control group (bPt-test = 0.0001). On the other hand, in the group to which ethanol + zinc sulfate was administered, the AST activity decreased compared to the ethanol group. A significant difference in the serum AST activities of four groups was observed (PANOVA = 0.0001).

Table 2 shows the effects of zinc sulfate on liver GSH and LPO. The GSH levels were significantly reduced in the group administered ethanol as compared to the other groups (PANOVA = 0.0001). A significant decrease of liver GSH levels in the group administered ethanol was determined in comparison to the control group (bPt-test = 0.0001). After zinc sulfate administration to ethanol-treated rats, liver GSH levels increased greatly when compared to the ethanol group (Pt-test = 0.0001). Zinc sulfate had no significant effect on liver GSH levels in the control group (Pt-test = 0.589). An eminent difference in the liver LPO levels of the four groups was observed (PANOVA = 0.0001). A significant increase of liver LPO levels in the group administered ethanol was determined in comparison to the control group (bPt-test = 0.0001). After the administration of ethanol + zinc sulfate, the liver LPO levels decreased notably when compared to the ethanol group (Pt-test = 0.001).

Table 2 Effects of zinc sulfate on the levels of lipid peroxidation and glutathione in the liver (Mean ± SD).
GroupnGSHnmol GSH/mgPt-testLPOnmol MDA/mgPt-test
proteinprotein
Control816.64 ± 1.240.52 ± 0.12
0.5890.065
Control + Zinc sulfate815.84 ± 3.870.69 ± 0.06
Ethanol1412.23 ± 2.92b0.93 ± 0.06b
0.00010.001
Ethanol + Zinc sulfate1120.74 ± 5.110.51 ± 0.10
PANOVA0.00010.0001
bPt-test = 0.0001 vs Control.
DISCUSSION

Ethanol-indued diseases in humans are important in clinical gastroenterology. Animal models in alcohol research have already been applied to study acute and chronic ethanol damage of the liver. Ethanol may accelerate oxidative stress via increased production of active oxygen species. Ethanol-induced oxidative stress plays a major role in liver injury[30]. Ethanol causes a notable fall in the level of zinc in the liver[1]. Zinc may play a key role in certain alterations observed in alcoholic patients[31]. The antioxidant defensive system of the liver might be influenced by changes in the zinc content of the liver[16]. Floersheim[32] suggested that zinc salts reduce tissue injury caused by a free radical-mediated mechanism. The present study suggests that ethanol-induced hepatic injury is related to the formation of free radicals and pretreatment of zinc prior to the administration of ethanol prevents toxicity. Ethanol treatment is accompanied by the generation of free radicals which stimulate LPO and decrease GSH levels. Therefore, zinc supplementation prevented ethanol-induced decreases in GSH and increases in LPO.

Under light and electron microscopes, the decrease of degenerative changes in the livers of rats administered ethanol + zinc sulfate indicates that zinc ameliorates the damage in the liver tissue of the group given ethanol. An increase in hepatic metallothionein-producing cells in control rats given only zinc as compared to intact controls was observed. This increase shows that metallothionein is required for high zinc levels in liver. In this study, synthesis of metallothionein was shown to increase in the livers of rats given zinc + ethanol, immunohistochemically, in accordance with previous findings[33]. Our results indicate that metallothionein induction by zinc sulfate has a protective effect against the injury of acute ethanol administration in liver. Elevation of metallothionein may maintain the integrity of the membrane of the organelles, as observed in the group given ethanol + zinc sulfate. Metallothionein expression may vary with types of tissue and physiological and nutritional factors such as zinc. There are limited studies on hepatic metallothionein levels following acute adminisration of ethanol to rats[4,11]. An over-expression of metallothionein serves to protect cells from the alkylating agents[14]. In the ethanol-intoxicated group, metallothionein levels increased nearly 3.5-times when compared to the control group[7]. Ebadi et al[22] also reported that the administration of zinc sulfate increased the synthesis of metallothionein mRNAs. It has been reported that hepatic metallothionein synthesis is stimulated by dietary zinc supplementation[34]. Koterov[11] reported that there was a linear dependence of the hepatic levels of metallothioneins with the dosage of alcohol. However, recent studies have shown that zinc inhibition of acute alcohol-induced liver injury is independent of metallothionein[35,36]. In the present report, the metallothionein labeling index correlated positively with the PCNA index in the rats given zinc + ethanol. It is suggested that enhanced antioxidant proteins such as metallothionein may be involved in hepatocyte proliferation. This finding supports a previous study showing an impairment of liver regeneration in metallothionein-I and metallothionein-II gene knockout mice after partial hepatectomy[37].

The liver is the most important organ in alcohol metabolism. The increase in AST and ALP activities in serum is an indicator of liver destruction. Their increase in the serum activities of these enzymes was directly proportional to the degree of cellular damage. The activity of AST in the serum of the group administered ethanol showed a statistically significant increase when compared to the control group. AST activity decreased in the group administered ethanol + zinc sulfate. This suggests that zinc pretreatment of rats prevented the elevation of serum AST. Acute ethanol exposure caused a 4-fold increase in the levels of serum AST compared with control animals[3]. The activity of ALP in the serum of the group administered ethanol has shown a significant increase when compared to the control group. The increase of alkaline phosphatase in the serum may be a result of damage to liver cells. Since zinc is a component of many enzymes, including alkaline phosphatase, a significant decrease was found in the activity of ALP in the group administered ethanol + zinc sulfate when compared to the group administered ethanol.

Glutathione plays a major role as a reductant in oxidation-reduction processes and also serves in detoxification[38]. Ethanol, or its metabolites, can alter the balance in the liver toward auto-oxidation, either acting as pro-oxidants, or reducing the antioxidant levels, or both[39]. The pathogenesis of alcohol-induced liver disease involves the adverse effect of ethanol metabolites and oxidative tissue injury[40]. The most prominent defensive system in the liver is reduced GSH. The values of GSH in blood of the rats administered ethanol have shown a significant decrease when compared to the control group. Metallothionein shares an important similarity with glutathione due to the fact that one-third of their amino acids are cysteines. Experimental depletion of glutathione in isolated rat hepatocytes has been shown to induce metallothionein expression and to create a new pool of thiol groups in the cell[41]. Glutathione provides a protective action against damage from reactive oxygen species and free radicals formed during drug metabolism[42,43]. On the other hand, Dreosti et al[44] reported that ethanol alone had no effect on glutathione levels. Cho et al[45] reported that ethanol and zinc sulfate administration did not affect hepatic glutathione levels in mice. It is reported that zinc supplementation prevented ethanol-induced decreases in glutathione concentration in the liver[36], in accordance with our findings.

Chronic ethanol administration induces oxidative stress and increases lipid peroxidation of the cell membrane. This leads to increased membrane fluidity, disturbances of calcium homeostasis, and finally results in cell death[46]. Oxidative stress is characterized by increased lipid peroxidation. A remarkable increase of liver lipid peroxidation levels in the group administered ethanol was determined in comparison to the control group. The present results suggest that zinc sulfate supplementation has a protective effect against lipid peroxidation in liver. Lipid peroxidation was observed to increase prominently in ethanol-fed rats after 4 and 8 wk when compared to the controls[47]. Patients and experimental animals with acute and chronic ethanol exposure have a depleted liver glutathione content, correlated with an increase in lipid peroxidation[48,49]. Zinc supplementation for 12 wk caused a decrease in lipid peroxidation, together with an increase in metallothionein concentration in rats[50]. However, 100 mL/L ethanol ingestion for 8 wk enhanced lipid peroxidation in liver[51]. Cabre et al[50] reported that zinc is an efficient hepato-protective agent against lipid peroxidation in alcoholic rats.

In conclusion, microscopic and biochemical evaluations reveal that zinc sulfate has a protective effect on ethanol-induced liver injury. Our results demonstrate that zinc acts as an antioxidant agent in hepatic antioxidant systems after acute ethanol administration. In addition, this protective effect against acute ethanol injury has also included proliferation in hepatocytes. Zinc may be a therapeutic agent in the prevention and treatment of ethanol-induced liver injury.

Footnotes

S- Editor Pan BR L- Editor Lutze M E- Editor Ma WH

References
1.  Floriańczyk B. Zinc level in selected tissues of ethanol and morphine intoxicated mice. Med Sci Monit. 2000;6:680-683.  [PubMed]  [DOI]  [Cited in This Article: ]
2.  Brzóska MM, Moniuszko-Jakoniuk J, Piłat-Marcinkiewicz B, Sawicki B. Liver and kidney function and histology in rats exposed to cadmium and ethanol. Alcohol Alcohol. 2003;38:2-10.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 82]  [Cited by in F6Publishing: 75]  [Article Influence: 3.6]  [Reference Citation Analysis (0)]
3.  Lambert JC, Zhou Z, Wang L, Song Z, McClain CJ, Kang YJ. Prevention of alterations in intestinal permeability is involved in zinc inhibition of acute ethanol-induced liver damage in mice. J Pharmacol Exp Ther. 2003;305:880-886.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 103]  [Cited by in F6Publishing: 109]  [Article Influence: 5.2]  [Reference Citation Analysis (0)]
4.  Zhou Z, Sun X, Lambert JC, Saari JT, Kang YJ. Metallothionein-independent zinc protection from alcoholic liver injury. Am J Pathol. 2002;160:2267-2274.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 66]  [Cited by in F6Publishing: 65]  [Article Influence: 3.0]  [Reference Citation Analysis (0)]
5.  Sato M, Bremner I. Oxygen free radicals and metallothionein. Free Radic Biol Med. 1993;14:325-337.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 632]  [Cited by in F6Publishing: 567]  [Article Influence: 18.3]  [Reference Citation Analysis (0)]
6.  Floriańczyk B. [Function of metallothionein in the body]. Postepy Hig Med Dosw. 1996;50:375-382.  [PubMed]  [DOI]  [Cited in This Article: ]
7.  Floriańczyk B, Stryjecka-Zimmer M. Induction of metallothioneins by ethanol and morphine. Ann Univ Mariae Curie Sklodowska Med. 2001;56:183-187.  [PubMed]  [DOI]  [Cited in This Article: ]
8.  Carey LC, Berbée PL, Coyle P, Philcox JC, Rofe AM. Zinc treatment prevents lipopolysaccharide-induced teratogenicity in mice. Birth Defects Res A Clin Mol Teratol. 2003;67:240-245.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 35]  [Cited by in F6Publishing: 37]  [Article Influence: 1.8]  [Reference Citation Analysis (0)]
9.  Carey LC, Coyle P, Philcox JC, Rofe AM. Zinc supplementation at the time of ethanol exposure ameliorates teratogenicity in mice. Alcohol Clin Exp Res. 2003;27:107-110.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 23]  [Cited by in F6Publishing: 23]  [Article Influence: 1.1]  [Reference Citation Analysis (0)]
10.  Zheng H, Berman NE, Klaassen CD. Chemical modulation of metallothionein I and III mRNA in mouse brain. Neurochem Int. 1995;27:43-58.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 62]  [Cited by in F6Publishing: 63]  [Article Influence: 2.2]  [Reference Citation Analysis (0)]
11.  Koterov AN. [Metallothionein level in liver, bone marrow, and lymphocytes of rats after administering ethanol]. Vopr Med Khim. 1994;40:15-17.  [PubMed]  [DOI]  [Cited in This Article: ]
12.  Ebadi M, Pfeiffer RF, Huff A. Differential stimulation of hepatic and brain metallothioneins by ethanol. Neurochem Int. 1992;21:555-562.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 11]  [Cited by in F6Publishing: 10]  [Article Influence: 0.3]  [Reference Citation Analysis (0)]
13.  Cox LS. Who binds wins: Competition for PCNA rings out cell-cycle changes. Trends Cell Biol. 1997;7:493-498.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 33]  [Cited by in F6Publishing: 33]  [Article Influence: 2.8]  [Reference Citation Analysis (0)]
14.  Tapiero H, Tew KD. Trace elements in human physiology and pathology: zinc and metallothioneins. Biomed Pharmacother. 2003;57:399-411.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 624]  [Cited by in F6Publishing: 495]  [Article Influence: 24.8]  [Reference Citation Analysis (0)]
15.  Bray TM, Bettger WJ. The physiological role of zinc as an antioxidant. Free Radic Biol Med. 1990;8:281-291.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 627]  [Cited by in F6Publishing: 632]  [Article Influence: 18.6]  [Reference Citation Analysis (0)]
16.  Jurczuk M, Brzóska MM, Moniuszko-Jakoniuk J, Gałazyn-Sidorczuk M, Kulikowska-Karpińska E. Antioxidant enzymes activity and lipid peroxidation in liver and kidney of rats exposed to cadmium and ethanol. Food Chem Toxicol. 2004;42:429-438.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 172]  [Cited by in F6Publishing: 182]  [Article Influence: 9.1]  [Reference Citation Analysis (0)]
17.  Stohs SJ, Bagchi D. Oxidative mechanisms in the toxicity of metal ions. Free Radic Biol Med. 1995;18:321-336.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 3001]  [Cited by in F6Publishing: 2544]  [Article Influence: 87.7]  [Reference Citation Analysis (0)]
18.  Cho CH. Current views of zinc as a gastrohepatic protective agent. Drug Dev Res. 1989;17:185-197 Available from: http: //www3.interscience.wiley.com/cgi-bin/abstract/109670957.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 18]  [Cited by in F6Publishing: 18]  [Article Influence: 0.5]  [Reference Citation Analysis (0)]
19.  Tuormaa TE. The adverse effects of zinc deficiency. J Orth Med. 1995;10:149-164 Available from: http: //www.foresight-preconception.org.uk/booklet_zinc.htm.  [PubMed]  [DOI]  [Cited in This Article: ]
20.  Yousef MI, El-Hendy HA, El-Demerdash FM, Elagamy EI. Dietary zinc deficiency induced-changes in the activity of enzymes and the levels of free radicals, lipids and protein electrophoretic behavior in growing rats. Toxicology. 2002;175:223-234.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 116]  [Cited by in F6Publishing: 116]  [Article Influence: 5.3]  [Reference Citation Analysis (0)]
21.  Zhou Z, Wang L, Song Z, Saari JT, McClain CJ, Kang YJ. Abrogation of nuclear factor-kappaB activation is involved in zinc inhibition of lipopolysaccharide-induced tumor necrosis factor-alpha production and liver injury. Am J Pathol. 2004;164:1547-1556.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 64]  [Cited by in F6Publishing: 66]  [Article Influence: 3.3]  [Reference Citation Analysis (0)]
22.  Ebadi M, Leuschen MP, el Refaey H, Hamada FM, Rojas P. The antioxidant properties of zinc and metallothionein. Neurochem Int. 1996;29:159-166.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 83]  [Cited by in F6Publishing: 75]  [Article Influence: 2.7]  [Reference Citation Analysis (0)]
23.  Beutler E, Duron O, Kelly BM. Improved method for the determination of blood glutathione. J Lab Clin Med. 1963;61:882-888.  [PubMed]  [DOI]  [Cited in This Article: ]
24.  Walter K, Schütt C.  Acid and alkaline phosphatase in serum (Two point method). HU Bergmeyer (Ed. ) Methods of enzymatic analysis Vol: 2, Verlag Chemie Gmbh, Florida 1974; 865-860.  [PubMed]  [DOI]  [Cited in This Article: ]
25.  Reitman S, Frankel SA. A colorimetric method for the determination of serum glutamic oxalacetic and glutamic pyruvic transaminases. Am J Clin Pathol. 1957;28:56-63.  [PubMed]  [DOI]  [Cited in This Article: ]
26.  Beutler E Glutathione in red cell metabolism: a manual of biochemical methods. New York: Grune and Stratton 1975; 112-114.  [PubMed]  [DOI]  [Cited in This Article: ]
27.  Ledwozyw A, Michalak J, Stepień A, Kadziołka A. The relationship between plasma triglycerides, cholesterol, total lipids and lipid peroxidation products during human atherosclerosis. Clin Chim Acta. 1986;155:275-283.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 306]  [Cited by in F6Publishing: 312]  [Article Influence: 8.2]  [Reference Citation Analysis (0)]
28.  Lowry OH, Rosebrough NJ, Farr AL, Randall RJ. Protein measurement with the Folin phenol reagent. J Biol Chem. 1951;193:265-275.  [PubMed]  [DOI]  [Cited in This Article: ]
29.  Hintze JL Copright C. 865, East 400. North Kaysville, Utah. 1986;84037 (801), 546-0445.  [PubMed]  [DOI]  [Cited in This Article: ]
30.  Dey A, Cederbaum AI. Alcohol and oxidative liver injury. Hepatology. 2006;43:S63-S74.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 398]  [Cited by in F6Publishing: 412]  [Article Influence: 22.9]  [Reference Citation Analysis (0)]
31.  Rodríguez-Moreno F, González-Reimers E, Santolaria-Fernández F, Galindo-Martín L, Hernandez-Torres O, Batista-López N, Molina-Perez M. Zinc, copper, manganese, and iron in chronic alcoholic liver disease. Alcohol. 1997;14:39-44.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 76]  [Cited by in F6Publishing: 77]  [Article Influence: 2.9]  [Reference Citation Analysis (0)]
32.  Floersheim GL. Synergism of organic zinc salts and sulfhydryl compounds (thiols) in the protection of mice against acute ethanol toxicity, and protective effects of various metal salts. Agents Actions. 1987;21:217-222.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 8]  [Cited by in F6Publishing: 8]  [Article Influence: 0.2]  [Reference Citation Analysis (0)]
33.  Arda-Pirincci P, Bolkent S, Yanardag R. The role of zinc sulfate and metallothionein in protection against ethanol-induced gastric damage in rats. Dig Dis Sci. 2006;51:2353-2360.  [PubMed]  [DOI]  [Cited in This Article: ]
34.  Krebs NF. Overview of zinc absorption and excretion in the human gastrointestinal tract. J Nutr. 2000;130:1374S-1377S.  [PubMed]  [DOI]  [Cited in This Article: ]
35.  Kang YJ, Zhou Z. Zinc prevention and treatment of alcoholic liver disease. Mol Aspects Med. 2005;26:391-404.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 73]  [Cited by in F6Publishing: 59]  [Article Influence: 3.1]  [Reference Citation Analysis (0)]
36.  Zhou Z, Wang L, Song Z, Saari JT, McClain CJ, Kang YJ. Zinc supplementation prevents alcoholic liver injury in mice through attenuation of oxidative stress. Am J Pathol. 2005;166:1681-1690.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 135]  [Cited by in F6Publishing: 138]  [Article Influence: 7.3]  [Reference Citation Analysis (0)]
37.  Oliver JR, Mara TW, Cherian MG. Impaired hepatic regeneration in metallothionein-I/II knockout mice after partial hepatectomy. Exp Biol Med (Maywood). 2005;230:61-67.  [PubMed]  [DOI]  [Cited in This Article: ]
38.  Smith CV, Jones DP, Guenthner TM, Lash LH, Lauterburg BH. Compartmentation of glutathione: implications for the study of toxicity and disease. Toxicol Appl Pharmacol. 1996;140:1-12.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 253]  [Cited by in F6Publishing: 261]  [Article Influence: 9.3]  [Reference Citation Analysis (0)]
39.  Suresh MV, Sreeranjit Kumar CV, Lal JJ, Indira M. Impact of massive ascorbic acid supplementation on alcohol induced oxidative stress in guinea pigs. Toxicol Lett. 1999;104:221-229.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 45]  [Cited by in F6Publishing: 45]  [Article Influence: 1.8]  [Reference Citation Analysis (0)]
40.  Niemelä O, Parkkila S, Ylä-Herttuala S, Villanueva J, Ruebner B, Halsted CH. Sequential acetaldehyde production, lipid peroxidation, and fibrogenesis in micropig model of alcohol-induced liver disease. Hepatology. 1995;22:1208-1214.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 137]  [Cited by in F6Publishing: 116]  [Article Influence: 4.0]  [Reference Citation Analysis (0)]
41.  Haïdara K, Moffatt P, Denizeau F. Metallothionein induction attenuates the effects of glutathione depletors in rat hepatocytes. Toxicol Sci. 1999;49:297-305.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 48]  [Cited by in F6Publishing: 49]  [Article Influence: 2.0]  [Reference Citation Analysis (0)]
42.  Afifi NM, Abdel-Rahman MS, Nassar AM. Effect of alcohol and/or cocaine on blood glutathione and the ultrastructure of the liver of pregnant CF-1 mice. Toxicol Lett. 1998;98:1-12.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 8]  [Cited by in F6Publishing: 8]  [Article Influence: 0.3]  [Reference Citation Analysis (0)]
43.  Morton S, Mitchell MC. Effects of chronic ethanol feeding on glutathione turnover in the rat. Biochem Pharmacol. 1985;34:1559-1563.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 84]  [Cited by in F6Publishing: 83]  [Article Influence: 2.1]  [Reference Citation Analysis (0)]
44.  Dreosti IE, Partick EJ. Zinc, ethanol, and lipid peroxidation in adult and fetal rats. Biol Trace Elem Res. 1987;14:179-191.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 30]  [Cited by in F6Publishing: 28]  [Article Influence: 0.8]  [Reference Citation Analysis (0)]
45.  Cho CH, Fong LY. The interaction of ethanol and zinc on hepatic glutathione and glutathione transferase activity in mice. Agents Actions. 1990;29:382-385.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 10]  [Cited by in F6Publishing: 11]  [Article Influence: 0.3]  [Reference Citation Analysis (0)]
46.  Nordmann R. Alcohol and antioxidant systems. Alcohol Alcohol. 1994;29:513-522.  [PubMed]  [DOI]  [Cited in This Article: ]
47.  Pathak A, Mahmood A, Pathak R, Dhawan D. Effect of zinc on hepatic lipid peroxidation and antioxidative enzymes in ethanol-fed rats. J Appl Toxicol. 2002;22:207-210.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 17]  [Cited by in F6Publishing: 18]  [Article Influence: 0.8]  [Reference Citation Analysis (0)]
48.  Farinati F, Cardin R, de Maria N, Lecis PE, Della Libera G, Burra P, Marafin C, Sturniolo GC, Naccarato R. Zinc, iron, and peroxidation in liver tissue. Cumulative effects of alcohol consumption and virus-mediated damage--a preliminary report. Biol Trace Elem Res. 1995;47:193-199.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 15]  [Cited by in F6Publishing: 16]  [Article Influence: 0.6]  [Reference Citation Analysis (0)]
49.  Videla LA, Valenzuela A. Alcohol ingestion, liver glutathione and lipoperoxidation: metabolic interrelations and pathological implications. Life Sci. 1982;31:2395-2407.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 172]  [Cited by in F6Publishing: 177]  [Article Influence: 4.2]  [Reference Citation Analysis (0)]
50.  Cabré M, Folch J, Giménez A, Matas C, Parés A, Caballería J, Paternain JL, Rodés J, Joven J, Camps J. Influence of zinc intake on hepatic lipid peroxidation and metallothioneins in alcoholic rats: relationship to collagen synthesis. Int J Vitam Nutr Res. 1995;65:45-50.  [PubMed]  [DOI]  [Cited in This Article: ]
51.  Flora SJ, Kumar D, Sachan SR, Das Gupta S. Combined exposure to lead and ethanol on tissue concentration of essential metals and some biochemical indices in rat. Biol Trace Elem Res. 1991;28:157-164.  [PubMed]  [DOI]  [Cited in This Article: ]  [Cited by in Crossref: 18]  [Cited by in F6Publishing: 18]  [Article Influence: 0.5]  [Reference Citation Analysis (0)]