+Bioline International Official Site (site up-dated regularly)

search
for

Indian Journal of Dermatology, Venereology and Leprology
Medknow Publications on behalf of The Indian Association of Dermatologists, Venereologists and Leprologists (IADVL)
ISSN: 0378-6323 EISSN: 0973-3922
Vol. 75, Num. 3, 2009, pp. 268-271

Indian Journal of Dermatology, Venereology and Leprology, Vol. 75, No. 3, May-June, 2009, pp. 268-271

Original Article

Determination of oxidative stress in vitiligo by measuring superoxide dismutase and catalase levels in vitiliginous and non-vitiliginous skin

Sravani PV, Babu NKishore, Gopal K.V.T, Rama Rao GRaghu, Rao AthotaRama, Moorthy Bhagavatula, Rao TRaghava

Department of Dermatology, King George Hospital, Andhra University, Visakhapatnam, AP
Correspondence Address:Gopal Sadan, D. No: 15-1-2C, Naoroji Road, Maharanipeta, Visakhapatnam - 530 002
graghuramarao@hotmail.com

Code Number: dv09080

PMID: 19439879
DOI: 10.4103/0378-6323.48427

Abstract

Background: Vitiligo is an acquired disorder characterized by circumscribed depigmented macules devoid of identifiable melanocytes. Complex genetic, immunological, neural and self destructive mechanisms interplay in its pathogenesis. According to autocytotoxic hypothesis, oxidative stress has been suggested to be the initial pathogenic event in melanocyte degeneration.
Aims: The aim of our investigation was to evaluate the role of oxidative stress by measuring levels of the antioxidant enzymes superoxide dismutase (SOD) and catalase (CAT) in lesional and normal skin of patients with vitiligo and in the skin of normal controls.
Methods: We determined the activity of SOD in lesional and non-lesional skin and CAT in lesional skin only of 25 vitiligo patients and 25 controls by using the spectrophotometric assay and Aebi's method, respectively.
Results: There was statistically significant increase in the levels of SOD in vitiliginous and non vitiliginous skin of patient group compared to the control group ( P < 0.001). No significant difference was found between the levels of SOD in lesional skin and non-lesional skin of vitiligo patients. The levels of CAT in the skin of patients were found to be significantly lower than those of controls ( P < 0.001).
Conclusions: There is increased oxidative stress in vitiligo as is indicated by high levels of SOD and low levels of CAT in the skin of vitiligo patients.

Keywords: Catalase, Oxidative stress, Superoxide dismutase, Vitiligo

Introduction

Vitiligo is an acquired disorder characterized by well-circumscribed milky white cutaneous macules devoid of identifiable melanocytes.^[1] Across the globe, vitiligo is the most common pigmentary disorder affecting 0.1%-2% of the world′s population irrespective of race and gender.^[2]

Although the precise etiology of vitiligo is not known, it has become quite clear in recent times that complex genetic, immunological, neural and self-destructive mechanisms interplay in its pathogenesis.^[2],[3] According to autocytotoxic hypothesis, oxidative stress has been suggested to be the initial pathogenic event in melanocyte degeneration with H₂ O₂ accumulation in the epidermis of patients with active disease.^[4] In recent studies, the involvement of oxidative stress in the pathophysiology of vitiligo has been investigated. An alteration in the antioxidant pattern, with significantly higher levels of superoxide dismutase (SOD) has been observed in the skin,^[5] erythrocytes,^[6],[7],[8] peripheral blood mononuclear cells^[6],[9] and serum^[10],[11] of vitiligo patients. Reduction in catalase (CAT) activity has been demonstrated in the epidermis,^[12],[13] peripheral blood mononuclear cells^[6] and in melanocytes.^[4] These findings support the concept of possible systemic oxidative stress in vitiligo.

As there are very few studies showing the extent of oxidative stress at tissue level, the present study has been undertaken to determine the status of oxidative stress by measuring levels of antioxidant enzymes, i.e., SOD and CAT, in lesional and normal skin of patients with vitiligo and in the skin of normal controls.

Methods

The study was conducted in the Departments of Dermatology, Andhra Medical College, and Biochemistry, Andhra University, Visakhapatnam. The study group included 25 cases of generalized and localized vitiligo. Patients with diabetes mellitus, thyroid disease, any autoimmune disorder or concomitant dermatological diseases were excluded. Patients who had taken systemic or topical treatment within three months before the present study were also excluded. Patients with a history of smoking or alcoholism or taking drugs for any other reason were not included. Twenty-five age- and sex-matched healthy individuals, who were non-smokers and non- alcoholics, were included as controls.

After obtaining consent from the participants, split-thickness skin specimens were obtained from lesional and non-lesional skin of 18 patients, from only vitiliginous skin of 7 patients and from normal skin of 25 controls. Split-thickness skin specimens were obtained from the middle of the lesional skin and from the normal skin at least 10 cm away from the lesional skin in the patient group. The control skin specimens were taken from the inner aspect of the forearm in healthy volunteers. After the desired amount of specimen was obtained, it was washed in ice-cold saline and was immediately carried in an ice box to the Department of Biochemistry.

Tissue samples were blotted on paper, weighed and minced in ice-cold 0.25 M sucrose solution. The resulting pieces were homogenized and diluted with ice-cold 0.25 M sucrose solution to reach a final dilution of 10% (w/v) for tissues. The resulting homogenates were centrifuged at an average speed of 8500 g for 10 min (at 2°C) to spin down tissue fragments, nuclei and mitochondria. The resulting supernatant samples were obtained for enzyme assays^[14] and measured by UV-visible spectrophotometer.

Measurement of Cu/Zn Superoxide Dismutase Activity
The Cu/Zn superoxide dismutase (E.C.1.15.1.1) enzyme activity was determined by the spectrophotometric assay using Oxford Biomedical Research kit.^{[14],[15],[16]} This method is based on the superoxide-mediated increase in the rate of autoxidation of 5, 6, 6a,11b-tetrahydroxybenzo (c) fluorine R1 in aqueous alkaline solution to yield a chromophore with maximum absorbance measured at 525nm. Results were expressed as units (U) of SOD activity/mg protein.

Measurement of Catalase Activity
Catalase (E.C.1.11.1.6) activity was measured by Aebi′s method.^[17] This method is based on the principle that the absorbance will decrease due to dismutation of H₂ O₂ at 240 nm. (UV-visible spectrophotometry). The amount of H₂ O₂ converted into H₂ O and 0.5 O in 1minute under standard conditions is accepted as the enzyme reaction velocity. Results were expressed as micromoles H₂ O₂ metabolized/min/mg protein.

SOD was estimated in both lesional and non-lesional skin of patients and skin of controls, whereas CAT was measured only in lesional skin of patients and skin specimens of controls.

Statistical Analysis
The statistical analysis was performed by using Student t test . The differences were considered significant when P < 0.05.

Results

The study group included 25 cases of generalized and localized vitiligo (14 men and 11 women). The age of the patients varied from 18 to 53 years (mean age = 33.32 years). Duration of vitiligo ranged from 4 months to 40 years, with a mean duration of 11.3 years. Twenty patients had generalized vitiligo and 5 had focal vitiligo. Five patients had progressive vitiligo and 20 had stable vitiligo.

In this study, the levels of SOD in vitiliginous skin of vitiligo patients (2,474 + 966 U/mg of protein) were found to be higher than the levels of SOD in normal skin of controls (969.15 + 388.56U/mg of protein). The difference was found to be statistically significant ( P < 0.001). Similarly, it was also observed in our study that the levels of SOD in non-vitiliginous skin of vitiligo patients (2351.97 + 984.37U/mg of protein) were significantly higher than the levels of SOD in normal skin of controls (969.15 + 388.56U/mg of protein) ( P < 0.001). No significant difference was found between the levels of SOD in vitiliginous skin and non-vitiliginous skin of patients ( P > 0.05).

The levels of CAT in the lesional skin of patients (5.36 + 0.83µM/min/mg protein) were found to be significantly lower than those of controls (13.18 + 0.53µM/min/mg protein) ( P < 0.001). There was no significant difference in the levels of SOD and CAT in the skin of vitiligo patients in relation to sex, age, duration or clinical type of vitiligo.

Discussion

One of the hypotheses to explain vitiligo is the self- destructive theory of melanocytes, which suggests a role for oxidative stress. Oxidative stress is thought to be the initial pathogenic event in melanocyte destruction.^[3],[4] Free radicals such as superoxide (O2⁻ ), hydrogen peroxide (H₂ O₂ ) and nitric oxide are molecules that occur during several physiological and pathological processes.^[18] These free radicals are scavenged continuously by antioxidant enzymes such as SOD, CAT, glutathione peroxidase, glutathione reductase, beta carotene, vitamin C, vitamin E and other trace elements.^[18] In oxidative stress, there is insufficient antioxidant activity leading to excessive accumulation of free radicals, which damage cellular compounds such as protein, carbohydrate, DNA and lipid.^[19] In normal conditions, SOD, an antioxidant enzyme catalyzes the dismutation of superoxide anion (O2⁻ ) into O₂ and H₂ O2^[15],[16] and CAT converts H₂ O₂ to O₂ and H₂ O. In oxidative stress, to counteract or scavenge increased levels of superoxide anions (O2⁻ ), SOD, an antioxidant enzyme, is increased, whereas CAT levels are decreased.^[20] Hydrogen peroxide, thus produced from superoxide anion (O2⁻ ), can readily cross cell membranes, causing much of the damage. Hence, measuring the levels of SOD and CAT in the skin, melanocytes, erythrocytes, peripheral blood mononuclear cells and blood indicates the status of oxidative stress in vitiligo patients.

In this study, the levels of SOD in vitiliginous and non-vitiliginous skin of vitiligo patients were found to be higher than the levels in normal skin of controls ( P < 0.001). A lower level of CAT activity was found in vitiligo patients when compared with controls ( P < 0.001). These high SOD levels and low levels of CAT in vitiligo patients support the concept of oxidative stress in the pathogenesis of vitiligo. In the present study, SOD levels were measured not only in lesional skin but also in non-lesional skin of patients to know whether the oxidative stress is localized or generalized. It was found that high levels of SOD were present both in lesional and non-lesional skin of patients. Schallreuter et al. ,^[12] reported higher levels of glutathione reductase and low levels of CAT in both lesional and non-lesional skin of vitiligo patients. These findings, inclusive of ours, suggest that oxidative stress is not a localized phenomenon but a more generalized process. This may be one of the explanations for developing newer lesions in vitiligo patients in the course of the disease.

Very few studies have been done to measure antioxidant enzymes at tissue level. Yildirim et al. ,^[5],[11] found significantly increased levels of SOD not only in lesional skin but also in erythrocytes of patients with generalized vitiligo. They supported the concept of free radical-mediated damage to melanocytes in generalized vitiligo. Similar higher levels of SOD were reported not only at tissue level (epidermis) but also in erythrocytes,^[6],[7],[8] peripheral mononuclear cells,^[6],[9] serum^[10],[11] and whole blood.^[21] These findings are in agreement with the results of the present study. However, Passi et al. ,^[13] Picardo et al.^[22] and Maresca et al. ,^[4] reported no significant difference, whereas Koca et al. ,^[21] reported decreased levels of superoxide dismutase in vitiligo patients compared with controls. Schallreuter et al.^[12] have demonstrated epidermal H₂ O₂ accumulation in association with low CAT levels in both involved and uninvolved skin of vitiligo patients. Decreased CAT levels in vitiligo patients compared with healthy controls have also been reported in other studies.^{[4],[9],[10],[13]} Recently, a study on the catalase gene ( CAT ) and its mutations leading to quantitative deficiency of CAT activity in the epidermis and accumulation of excess H₂ O₂ and susceptibility to develop vitiligo has been reported.^[23]

Our findings and several studies demonstrate that there is impairment in the antioxidant system in vitiligo, leading to free radical-mediated damage to melanocytes. Our findings revealed that this oxidative stress is not a localized phenomenon but a generalized process and may be one of the reasons for the progressive nature of the disease. In view of these findings, antioxidants may play an adjuvant role in the management of vitiligo in addition to specific therapies.

References

1.	Hann SK, Nordlund JJ. Definition of vitiligo. In: Hann SK, Nordlund JJ, editors. Vitiligo. A monograph of the basic and clinical science. Oxford: Blackwell Science Ltd; 2000. p. 3-5. Back to cited text no. 1
2.	Ortonne JP, Bahodoran P, Fitzpatrick TB, Mosher DB, Hori Y. Hypomelanoses and hypermelanoses. In: Freedberg IM, Eisen AZ, Wolff K, Austen KF, Goldsmith LA, Katz SI, editors. Fitzpatrick's Dermatology in General Medicine. 6^th ed. New York: McGraw Hill; 2003. p. 839-47. Back to cited text no. 2
3.	Kovacs SO. Vitiligo. J Am Acad Dermatol 1998;38:647-66. Back to cited text no. 3 [PUBMED] [FULLTEXT]
4.	Maresca V, Roccella M, Roccella F, Camera E, Del Porto G, Passi S, et al . Increased sensivity to peroxidative agents as a possible pathogenic factor of melanocyte damage in vitiligo. J Invest Dermatol 1997;109:310-3. Back to cited text no. 4 [PUBMED]
5.	Yildirim M, Baysal V, Inaloz HS, Can M. The role of oxidants and antioxidants in generalized vitiligo at tissue level. J Eur Acad Dermatol Venereol 2004;18:683-6. Back to cited text no. 5 [PUBMED] [FULLTEXT]
6.	Dell'Anna ML, Maresca V, Briganti S, Camera E, Falchi M, Picardo M. Mitochondrial impairment in peripheral mononuclear cells during the active phase of vitiligo. J Invest Dermatol 2001;117:908-13. Back to cited text no. 6 [PUBMED] [FULLTEXT]
7.	Agarwal D, Shajil EM, Marfatia YS, Begum R. Study on the antioxidant status of vitiligo patients of different age-groups in Baroda. Pigment Cell Res 2004;17:289-94. Back to cited text no. 7
8.	Hazneci E, Karabulut AB, Ozturk C, Batcioglu K, Dogan G, Karaca S, et al . A comparative study of superoxide dismutase, catalase and glutathione peroxidase activities and nitrate levels of vitiligo patients. Int J Dermatol 2005;44:636-40. Back to cited text no. 8
9.	Dell'Anna ML, Urbanelli S, Mastrofrancesco A, Camera E, Iacovelli P, Leone G, et al . Alterations of mitochondria in peripheral blood mononuclear cells of vitiligo patients. Pigment Cell Res 2003;16:553-9. Back to cited text no. 9 [PUBMED] [FULLTEXT]
10.	Chakraborty DP, Roy S, Chakraborty AK. Vitiligo, psoralen and melanogenesis: Some observations and understanding. J Invest Dermatol 1990;95:441-5. Back to cited text no. 10
11.	Yildirim M, Baysal V, Inaloz HS, Kesici D, Delibas N. The role of oxidants and antioxidants in generalized vitiligo. J Dermatol 2003;30:104-8. Back to cited text no. 11 [PUBMED] [FULLTEXT]
12.	Schallreuter KU, Wood JM, Berger J. Low catalase levels in epidermis of patients with vitiligo. J Invest Dermatol 1991;97:1081-5. Back to cited text no. 12 [PUBMED]
13.	Passi S, Grandinetti M, Maggio F, Stancato A, DeLuca C. Epidermal oxidative stress in vitiligo. Pigment Cell Res 1998;11:81-5. Back to cited text no. 13
14.	Nebot C, Moutet M, Huet P, Xu JZ, Yadan J, Chaudiere J. Spectrophotometric Assay of superoxide dismutase activity based on the activated autoxidation of a tetracyclic catechol. Anal Biochem 1993;214:442-51. Back to cited text no. 14
15.	Beyer W, Imlay J, Fredovich I. Superoxide dismutase. Progr Nucl Acid Res Mole Biol 1991;40:221-53. Back to cited text no. 15
16.	Stallings W, Pattridge K, Strong R, Ludwig M. Manganese and iron superoxide dismutases are structural homologs. J Biol Chem 1984;259:10695-9. Back to cited text no. 16
17.	Aebi H. Catalase in vitro . In: Packer L editor. Methods in Enzymology. Orlando FL: Academic Press; 1984. p. 121-6. Back to cited text no. 17
18.	Knight JA. Diseases related to oxygen-derived free radicals. Ann Clin Lab 1995;25:111-21. Back to cited text no. 18
19.	Beazley WD, Gaze D, Panske A, Panzig E, Schallreuter KU. Serum Selenium levels and blood glutathione peroxidase activities in vitiligo. Br J Dermatol 1999;141:301-3. Back to cited text no. 19 [PUBMED] [FULLTEXT]
20.	Koca R, Armutcu F, Altinyazar HC, Gurel A. Oxidant-Antioxidant enzymes and lipid peroxidation in generalized vitiligo. Clin Exp Dermatol 2004;29:406-9. Back to cited text no. 20
21.	Boisseau-Garsaud AM, Garsaud P, Lejoly-Boisseau H, Robert M, Quist D, Arveiler B. Increase in total blood antioxidant status and selenium levels in black patients with active vitiligo. Int J Dermatol 2002;41:640-2. Back to cited text no. 21 [PUBMED] [FULLTEXT]
22.	Picardo M, Passi S, Morrone A, Grandinetti M, Di Carlo A, Ippolito F. Antioxidant status in the blood of patients with active vitiligo. Pigment Cell Res 1994;7:110-5. Back to cited text no. 22 [PUBMED]
23.	Courtney BC, Jin-Xiong S, Wayne TM. Genetic association of the catalase gene (CAT) with vitiligo susceptibility. Pigment Cell Res 2002;15:2. Back to cited text no. 23

Home	Faq	Resources	Email Bioline
© Bioline International, 1989 - 2024, Site last up-dated on 01-Sep-2022. Site created and maintained by the Reference Center on Environmental Information, CRIA, Brazil System hosted by the Google Cloud Platform, GCP, Brazil