Introduction

Oncology Letters

1792-1074 1792-1082

D.A. Spandidos

10.3892/ol.2016.5346

OL-0-0-5346

Articles

Protective effect of selenium against cisplatin-induced nasopharyngeal cancer in male albino rats

Zhu

Kan

1 * Jiang

Lei

2 * Chu

Yun

3 Zhang

Yong-Sheng

1Department of Otorhinolaryngology, Wuxi No. 2 People's Hospital Affiliated to Nanjing Medical University, Wuxi, Jiangsu 214002, P.R. China 2Department of Neurosurgery, Wuxi No. 2 People's Hospital Affiliated to Nanjing Medical University, Wuxi, Jiangsu 214002, P.R. China 3Department of Surgery, Wuxi No. 2 People's Hospital Affiliated to Nanjing Medical University, Wuxi, Jiangsu 214002, P.R. China

Correspondence to: Dr Yong-Sheng Zhang, Department of Otorhinolaryngology, Wuxi No. 2 People's Hospital Affiliated to Nanjing Medical University, 68 Zhongshan Road, Wuxi, Jiangsu 214002, P.R. China, E-mail: yongshengzhang17@hotmail.com *

Contributed equally

12 2016

02 11 2016

12 6 5068 5074 23072015 09092016

2016

This is an open access article distributed under the terms of the Creative Commons Attribution-NonCommercial-NoDerivs License, which permits use and distribution in any medium, provided the original work is properly cited, the use is non-commercial and no modifications or adaptations are made.

The present study evaluated the protective effect of selenium against cisplatin-induced nasopharyngeal cancer in the cardiac tissue of adult rats. Male Wistar rats were divided into 4 groups of 6 rats each. Different combinations of selenium and cisplatin were administered for 45 days, following which the animals were sacrificed and the nasopharyngeal tissue was surgically removed. Lipid peroxidation, reduced glutathione, and the antioxidant enzymes superoxide dismutase (SOD), catalase and lactate dehydrogenase (LDH) were measured. Apoptotic-related gene (p53, bax and caspase 3) mRNA expression was determined using quantitative polymerase chain reaction. Caspase 3 activity was also measured in all the groups. The results demonstrated that selenium significantly reduced the levels of malondialdehyde. The levels of glutathione, SOD, LDH and catalase significantly increased following selenium treatment. Relative mRNA expression (p53, bax and caspase 3) was significantly reduced in the cisplatin-treated rats, but it significantly increased following selenium treatment. The anticancer activity of selenium was also investigated in HK1cells. Fluorescence and confocal microscopy were used to analyze apoptosis and reactive oxygen species. The protective effect of selenium was also evident through caspase 3 activity, which significantly increased following selenium treatment. Taken together, these results indicate that selenium may be beneficial against cisplatin-induced nasopharyngeal cancer.

selenium cisplatin rats antioxidant mRNA

Introduction

Selenium, an essential biological trace element, has received considerable attention as an important micronutrient for humans. Selenium serves a role in several cellular and physiological processes, including thyroid hormone production and immune responses (1). It has been reported that selenium has antioxidant properties (2). Food and drink are the primary natural sources of selenium. High levels of selenium are present in cereals, seafood and meat products, whereas there is little found in vegetables, milk or fruits (3). Selenium deficiency has been associated with several degenerative diseases (4). Selenium has been widely used to treat several pathophysiological conditions, including cervical, renal and liver cancer (5).

Nasopharyngeal carcinoma is an endemic disease in South Asia. There are several conventional treatments available, including radiotherapy. Chemotherapy has gained importance in the treatment of nasopharyngeal carcinoma (6). However, the complications are high. Chemotherapy treatment frequently fails due to multidrug resistance and cancer treatment requires selective action on the targeted site (6). Cisplatin is a widely used therapeutic agent that acts as a radiation sensitizer and a cytotoxic compound (6). Cisplatin-acquired resistance in patients may lead to the failure of chemotherapy treatment (6). Drug resistance and the establishment of cisplatin-resistant cells are considered to be possible ways to understand the chemoresistance mechanism (6).

To the best of our knowledge, cisplatin-resistant nasopharyngeal carcinoma cell establishment and associated studies are limited. Studies on selenium treatment against cisplatin-induced nasopharyngeal cancer are also limited. The ability of selenium to neutralize the toxicity of cisplatin in the nasopharyngeal tissue has yet to be investigated. The present study examines the impact of selenium on cisplatin-induced toxicity.

Materials and methods <sec> <title>Materials

Dimethyl sulfoxide was purchased from Sigma- Aldrich (Merck Millipore, Darmstadt, Germany). Dulbecco's modified Eagle's medium, fetal bovine serum (FBS), penicillin-streptomycin and trypsin-ethylenediaminetetraacetic acid were obtained from Welgene, Inc. (Gyeongsan-si, South Korea). Acridine orange (AO), ethidium bromide (EB) and 2′,7′-dichlorofluorescein diacetate (DCFH-DA) were purchased from Santa Cruz Biotechnology, Inc. (Dallas, TX, USA). Primers were obtained from Macrogen Inc. (Seoul, South Korea).

Animals

Healthy, male, albino rats were purchased from the Department of Otorhinolaryngology, Jiangsu Provincial People's Hospital Affiliated to Nanjing Medical University (Nanjing, China). Those weighing 160–180 g were selected for the present study. The rats were kept in polypropylene cages, at a temperature of 25±0.5°C, at a relative humidity of 60±5% and at a photoperiod of 12 h/day. The male albino rats were grouped into 4 groups of 6 rats each.

Experimental induction of cancer

The application of carcinogens was achieved by means of cisplatin treatment prior to the experiments. Cisplatin (10 µg) was administered for 45 days for the induction of diabetes with final tumor incidences close to 100%.

Treatment

The experimental groups were designated as follows: Group I, normal saline (10 µl); Group II, 10 µg cisplatin; Group III, 10 µg selenium+10 µg cisplatin; and Group IV 20 µg selenium+20 µg cisplatin. The drug was administered intraperitoneally for 45 days. The dose level and duration of the experiment was selected based on our preliminary study. The preliminary study was conducted with a different dose level (range, 1–100 µg). The animals were sacrificed by decapitation, and nasopharyngeal tissue was surgically removed. Animal tissues were homogenized using a Potter-Elvehjem glass-Teflon homogenizer and a Dounce hand homogenizer (Sigma-Aldrich; Merck Millipore). This method is rapid and poses little risk to proteins, other than the release of proteases from other cellular compartments. Proteolytic degradation was reduced by adding protease inhibitors to the homogenization buffers. The prepared tissue homogenate was used immediately in subsequent investigations.

In vivo studies Determination of lipid peroxidation

Lipid peroxidation (LPO) was determined using the Lipid Peroxidation (MDA) assay kit (ab118970; Abcam, Cambridge, MA, USA). This was based on the spectrophotometric method of Pandurangan et al (7). Malondialdehyde (MDA) was measured by determining the thiobarbituric acid reactive species. The absorbance of the resulting product was measured at 534 nm (Cary 100 UV-Vis spectrophotometer; Agilent Technologies, Inc., Santa Clara, CA, USA).

Determination of reduced glutathione

Glutathione (GSH) level was measured using the gluathione assay kit (Abcam). This was based on the spectrophotometric method of Pandurangan et al (7). The yellow product color was measured at 405 nm (Cary 100 UV-Vis spectrophotometer; Agilent Technologies, Inc.).

Determination of superoxide dismutase (SOD) and catalase enzyme activities

SOD, catalase and lactate dehydrogenase (LDH) enzyme activities were determined using the antioxidant enzyme assay kit method (Abcam) which was based on the method of Pandurangan et al (7).

Quantitative polymerase chain reaction (qPCR)

The qPCR was performed using a cDNA equivalent of 10 ng total RNA from each sample, withspecific primers for p53 (forward, 5′-TAACAGTTCCTGCATGGGCGGC-3′ and reverse, 5′-AGGACAGGCACAAACACGCACC-3′), bax (forward, 5′-TGGAGCTGCAGAGGATGATTG-3′ and reverse, 5′-GAAGTTGCCGTCAGAAAACATG-3′), caspase 3 (forward, 5′-TTAATAAAGGTATCCATGGAGAACACT-3′ and reverse, 5′-TTAGTGATAAAAATAGAGTTCTTTTGTGAG-3′) and a housekeeping gene, glyceraldehyde 3-phosphate dehydrogenase (forward, 5′-GGTCACCAGGGCTGCTTTT-3′ and reverse, 5′-ATCTCGCTCCTGGAAGATGGT-3′). Time, temperature and cycles were performed as previously described (8). The reaction was performed in a 10 µl reaction volume using SYBR Green Master mix (Bioneer Corporation, Daejeon, Korea) according to the manufacturer's protocol (8).

Caspase activity assay

Caspase 3 enzyme activity was measured using an activity assay kit (Sigma-Aldrich; Merck Millipore) based on the method of Muthuraman (9).

In vitro studies Cell culture

HK1 cells were obtained from the American Type Culture Collection (Manassas, VA, USA). 10% FBS and 1% antibiotics (1% penicillin-streptomycin) were used for cell growth. The cells were grown to 90% confluence in a CO₂ incubator at 37°C with 5% CO₂.

Fluorescence microscopy

The HK1 cells (2.5×10⁴) were cultured in 6-well plates and treated for 48 h with either 10 µg/ml selenium, 10 µg/ml selenium+10 µg/ml cisplatin or 20 µg selenium+20 µg cisplatin. Control cells were incubated with growth medium only. The cells were examined with a fluorescence microscope (10) (Axiovert 2000; Carl Zeiss AG, Oberkochen, Germany).

Confocal laser scanning (CLS) microscopy

The HK1 cells (2.5×10⁴) were grown at a volume of 2×10⁴ cells/well in 6-well plates. The cells were treated for 48 h with either 10 µg/ml selenium, 10 µg/ml selenium+10 µg/ml cisplatin or 20 µg selenium+20 µg cisplatin. Control cells were incubated with growth medium only. Cells were stained with EB and AO stains. The cells were viewed immediately under a CLS microscope (1X81^R Motorized Inverted Microscope; Olympus Corporation, Tokyo, Japan) (10).

Determination of reactive oxygen species (ROS) production

The HK1 cells (2.5×10⁴) were cultured in6-well plates and treated for 48 h with either 10 µg/ml selenium, 10 µg/ml selenium+10 µg/ml cisplatin or 20 µg selenium+20 µg cisplatin. Control cells were incubated with growth medium only. The cells were incubated with 5 µM of DCFH-DA in a growth medium (Sigma-Aldrich; Merck Millipore) for 30 min at 37°C and 5% CO₂. The fluorescence was measured at 485/525 nm (Ex/Em) based on the method of Muthuraman et al (10) (Axiovert 2000; Carl Zeiss AG).

Statistical analysis

All values are expressed as the mean ± standard deviation. Test and control values were compared using the Student's t-test (SPSS 16, Statistical Package; SPSS, Inc., Chicago, IL, USA). P<0.05 was considered to indicate a statistically significant difference.

Results <sec> <title>Effect of selenium on MDA concentration

The effect of selenium on MDA concentration in the male albino rats is demonstrated in Fig. 1. The MDA concentration in the control rats (group I) was 33±1 nmol/g, whereas it increased to 58±1.1 nmol/g in the cisplatin-induced rats (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly reduced (49±1.2 nhmol/g) the concentration of MDA in the rats compared to the control group (group I) (P=0.02132; Fig. 1). The administration of 20 µg/ml selenium with 20 µg/ml cisplatin (group IV) also significantly reduced the concentration of MDA (37±1.3 nmol/g) in the rats compared to the control group (group I) (P=0.03562; Fig. 1).

Effect of selenium on level of GSH

The effect of selenium on GSH content in the male albino rats is demonstrated in Fig. 2. The level of GSH in the control rats (group I) was 67±2 mg/g, whereas it decreased to36±1.1 mg/g in the cisplatin-induced rats (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly increased (46±1.2 mg/g) the level of GSH in the rats compared to the control group (group I) (P=0.4329; Fig. 2). The administration of 20 µg/ml selenium with 20 µg/ml cisplatin (group IV) also significantly increased the level of GSH (58±1 mg/g) in the rats compared to the control group (group I) (P=0.02147; Fig. 2).

Effect of selenium on SOD activity

The effect of selenium on SOD activity in the male albino rats is demonstrated in Fig. 3. The SOD activity in the control rats (group I) was 3.1±0.1 U/mg, whereas it decreased to 2.1±0.02 U/mg in the cisplatin-induced rats (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly increased the SOD activity in the rats compared to the control group (group I) (P=0.03253; Fig. 3). The administration of 20 µg/ml of selenium with 20 µg/ml of cisplatin (group IV) also significantly increased the SOD activity (58±1 mg/g) in the rats compared to the control group (group I) (P=0.03821; Fig. 3).

Effect of selenium on catalase activity

The effect of selenium on catalase activity in the male albino rats is demonstrated in Fig. 4. The catalase activity in the control rats (group I) was 9.2±0.1 U/g, whereas it decreased to 5.2±0.2 U/g in the cisplatin-induced rats (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) (P=0.02225; Fig. 4) significantly increased (6.4±0.1 U/g) the catalase activity in the rats compared to the control group (group I). The administration of 20 µg/ml selenium with 20 µg/ml cisplatin (group IV) also significantly increased the catalase activity (7.9±0.2 U/g) in the rats compared to the control group (group I) (P=0.03312; Fig. 4).

Effect of selenium on LDH activity

The effect of selenium on LDH activity in the male albino rats is demonstrated in Fig. 5. The LDH activity in the control rats (group I) was 90±2 U/l, whereas it increased to 152±3 U/l in the cisplatin-induced rats (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly decreased (124±2 U/l) the LDH activity in the rats compared to the control group (group I) (P=0.02412; Fig. 5). The administration of 20 µg/ml selenium with 20 µg/ml cisplatin (group IV) also significantly decreased LDH activity (107±2 UL-1) in the ratscompared to the control group (group I) (P=0.04412; Fig. 5).

Effect of selenium on mRNA expression

The effect of selenium on mRNA expression in the male albino rats is shown in Fig. 6. The mRNA expression of p53, bax and caspase 3 decreased 0.53-, 0.39 and 0.48-fold, in the cisplatin-induced rats (group I) compared with their respective controls (group I). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly increased mRNA expression of p53, bax and caspase 3 (0.42-, 0.27- and 0.36-fold, respectively) in the rats compared to the control group (group I) (P=0.03312; Fig. 6). The administration of 20 µg/ml of selenium with 20 µg/ml of cisplatin (group IV) significantly increased mRNA expression (0.13-, 0.11- and 0.22-fold, respectively) in the rats compared towith the control group (P=0.05113; Fig. 6).

Effect of selenium on caspase 3 activity

The effect of selenium on caspase 3 activity in the male albino rats is shown in Fig. 7. The caspase 3 activity decreased to 11% of the control in the cisplatin-induced rats (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly increased (17.4%) the caspase 3 activity in the rats compared to the control group (group I) (P=0.04451; Fig. 7). The administration of 20 µg/ml selenium with 20 µg/ml cisplatin (group IV) also significantly increased the caspase 3 activity (28.2%) in the rats compared to the control group (group I) (P=0.04123; Fig. 7).

Effect of selenium on apoptosis

Microscopy was performed to determine whether the anticancer activity of selenium is associated with the induction of apoptosis, a morphological feature of cell death. Chromatin condensation in the stained nucleus was used to differentiate viable, apoptotic and necrotic cells. The anticancer activity of cisplatin in the HK1 cells is shown in Figs. 8 and 9. The analysis revealed normal cell size and morphology in the control cells (group I), whereas the cisplatin-incubated HK1 cells demonstrated altered cell morphology, including apoptosis and necrosis (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly reduced the apoptosis and necrosis of the cells compared to the control group (group II). The administration of 20 µg/ml selenium with 20 µg/ml cisplatin (group IV) (P=0.03421; Figs. 8 and 9) significantly reduced the occurrence of apoptosis and necrosis towards normal levels compared to the control group (group II) (P=0.03411; Figs. 8 and 9).

Effect of selenium on reactive oxygen species (ROS) level

ROS play a vital role in facilitating signal transduction processes within the intracellular region (10). The fluorescent probe, DCFH-DA, determined the intracellular ROS generation. Fluorescence studies indicated no green fluorescence intensity of DCF in the control cells (group I), whereas increased levels were found in the cisplatin-incubated cells (group II). The administration of 10 µg/ml selenium with 10 µg/ml cisplatin (group III) significantly increased the levels of ROS compared with the control group (II). The administration of 20 µg/ml selenium with 20 µg/ml cisplatin (group IV) also increased the levels of ROS in the cells compared with the control group (P=0.04612; Fig. 10).

Discussion

Recently, several studies have been focused on cisplatin due to its wider uses. Cisplatin induces neurotoxicity, nephrotoxicity, ototoxicity, myelotoxicity, nausea, vomiting, hemolytic anemia and electrolyte disturbances (6,11). Chronic exposure to cisplatin could cause drug resistance and nasopharyngeal cancer. Selenium has attracted attention from several researchers due its anticancer potential (11). The present study demonstrated that chronic exposure to cisplatin could produce nasopharyngeal cancer in adult rats and that the use of selenium could reduce the effect of cisplatin.

The accumulation of free radicals and oxidative stress induction have been reported as the toxic effects of cisplatin (6). It is well known that oxidative stress plays a crucial role in cell apoptosis and death. Increased lipid peroxidation is the primary consequence of this oxidative stress, mainly involving polyunsaturated fatty acids (12). In the present study, cisplatin significantly increased lipid peroxidation in the male albino rats. This is evidence for the role of free radicals and oxidative damage in the reduction of cisplatin-induced nasopharyngeal cancer. Cell membranes may readily bind to cisplatin and cause lipid peroxidation via the increased generation of free radicals (13). Treatment of selenium with cisplatin reduced the concentration of MDA, indicating the anti-cancer activity of selenium (14). It has been reported that the use of selenium has a protective effect against myocardial injury (14).

Cell and tissue integrity and function have been shown to be safeguarded by the protective action of selenium against oxidative damage. ROS may also bind to cellular proteins and can initiate the formation of side chain and readily susceptible (degradative) amino acids (15). Impairment of cell function may occur due to the accumulation of oxidized proteins. Yuan and Tang (16) demonstrated that selenium can counteract the free radicals and oxidative damage in chickens.

The accumulation of free radicals may affect DNA structure and stability, leading to DNA damage and cell death (17). It has been reported that several toxic compounds can induce DNA damage (18), and the lipid peroxidation product MDA could bind to DNA (19). It has been shown that selenium could reduce DNA damage in cells (20). Kara et al (21) have demonstrated the antioxidant properties of selenium. Antioxidant enzymes are the first line of cell defense that safeguards cells from oxidative damage. In the present study, SOD, catalase and LDH activities all significantly increased following selenium treatment.

GSH is a well-known non-enzymatic antioxidant that provides a second line of defense against oxidative damage (22). GSH acts as a substrate for the glutathione peroxidase and glutathione S-transferase enzymes, and is involved in the reduction/removal of ROS from cells (23). Reduced levels of GSH occur during oxidative stress, which results in the impairment of cell function and metabolism (24).

In conclusion, in the present study, cisplatin exhibited carcinogenicity in male albino rats and HK1 cells. Cellular architecture also returned to normal following treatment. Morphological and apoptotic changes confirmed that a reduction in apoptosis occurs following selenium treatment. From these experimental results, it can be concluded that cisplatin could exert carcinogenicity, but that treatment with selenium could significantly reverse this toxicity.

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Figure 1.

Effect of selenium on lipid peroxidation in nasopharyngeal cancer of male albino rats, as determined by MDA, malondioldehyde, level. The results are presented as nmol/g compared with the control. Values are expressed as the mean ± standard deviation. *P<0.05 vs. control.

Figure 2.

Effect of selenium on GSH, glutathione, levels in the nasopharyngeal cancer of male albino rats. The results are presented as mg/g compared with the control. Values are expressed as the mean ± standard deviation. *P<0.05 vs. control.

Figure 3.

Effect of selenium on SOD, superoxide dismutase, activity in the nasopharyngeal cancer of male albino rats. The results are presented as U/mg compared with the control. Values are expressed as the mean ± standard deviation. *P<0.05 vs. control.

Figure 4.

Effect of selenium on catalase activity in the nasopharyngeal cancer of male albino rats. The results are presented as U/g compared with the control. Values are expressed as the mean ± standard deviation. *P<0.05 vs. control.

Figure 5.

Effect of selenium on LDH, lactate dehydrogenase, activity in the nasopharyngeal cancer of male albino rats. The results are presented as UL-1 compared with the control. Values are expressed as the mean ± standard deviation. *P<0.05 vs. control.

Figure 6.

Effect of selenium on apoptotic-related gene mRNA expression in the nasopharyngeal cancer of male albino rats. The results are presented as fold increase compared with the control. Values are expressed as the mean ± standard deviation. *P<0.05 vs. control.

Figure 7.

Effect of selenium on caspase 3 activity in the nasopharyngeal cancer of male albino rats. The results are presented as percentage compared with the control. Values are expressed as the mean ± standard deviation. *P<0.05 vs. control.

Figure 8.

Effect of selenium on apoptosis in nasopharyngeal cancer cells. AO, acridine orange and EB, ethidium bromide, stains are shown. The respective images from three independent fluorescence experiments.

Figure 9.

Effect of selenium on apoptosis in the nasopharyngeal cancer cells. The respective images from three independent confocal experiments.

Figure 10.

Effect of selenium on ROS, reactive oxygen species, in the nasopharyngeal cancer cells. The respective images from three independent experiments.