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Supplement: Waltham International Symposium

Voluntary Exercise Has Only Limited Effects on Activity of Antioxidant Enzymes and Does Not Cause Oxidative Damage in a Small Mammal

Colin Selman^*,3, Jane S. McLaren^*, Andrew R. Collins and John R. Speakman^*,

^* Aberdeen Centre for Energy Expenditure and Obesity (ACERO), Department of Zoology, Aberdeen University, Aberdeen, UK; Division of Cellular Integrity and ACERO, Division of Appetite and Energy Balance, Rowett Research Institute, Bucksburn, Aberdeen, UK

³To whom correspondence should be addressed. E-mail: c.selman{at}abdn.ac.uk.

KEY WORDS: • voluntary exercise • reactive oxygen species • antioxidant • enzymes • oxidative DNA damage • comet assay • vole

EXPANDED ABSTRACT

Regular physical exercise has a number of beneficial effects, including the reduction in the risk of cancer, osteoporosis, obesity and cardiovascular disease (1,2). Voluntary exercise through wheel running has also been shown to increase average life expectancy in rats by nearly 10% (3). However, physical exercise also considerably increases total oxygen consumption relative to resting levels, which may, in turn, increase the generation of reactive oxygen species (ROS). If ROS generation exceeds the antioxidant protection and repair mechanisms, oxidative stress will occur and this process is thought to be intimately involved in the aging process (4) and as a causative factor in lipid, protein and DNA damage (5–8). Exercise-induced oxidative stress is also implicated in muscle contractile dysfunction possibly by impaired Ca²⁺ metabolism and apoptosis of muscle cells (7,9).

Considerable debate exists in the literature [e.g., Powers & Sen (10)] on how exercise affects the balance between ROS production, antioxidant protection and repair. During endurance training, in particular, increases occur in both enzymatic and nonenzymatic antioxidants (11,12), although these responses appear highly tissue specific (13,14). Repeated bouts of exercise may also increase resistance to oxidative stress (15), primarily through the induction of various stress proteins (16). Strenuous exercise has been shown to elevate urinary 8-hydroxy-deoxyguanosine (8-oxodGuo) excretion, which may be interpreted as an increase in oxidative DNA damage or in DNA repair (6,17). Endurance exercise in dogs decreased the level of 8-oxodGuo in the DNA of colonocytes and lymphocytes, indicating an increase in DNA repair capacity (17), or in antioxidant activity. However, the response of the various antioxidant and repair mechanisms to exercise appears dependent on many factors, including exercise bout duration, exercise intensity, previous exercise exposure, subject species, subject age and assay technique employed (11–13).

The majority of studies examining the relationship between exercise, ROS production and oxidative stress have exposed subjects to bouts of acute and/or exhaustive exercise, or examined the effects of endurance training (10), with fewer studies investigating the effects of voluntary exercise on oxidative stress parameters [e.g., Leeuwenburgh et al. (18)]. In the following study, we used a small (15–30 g) mammalian model, the short-tailed field vole (Microtus agrestis) to examine whether short-term (i.e., 1- or 7-d) voluntary wheel running, with or without an 8-h recovery period, had any effect on the activities of the antioxidant enzymes catalase (Cat), glutathione peroxidase (Gpx) and total superoxide dismutase (total-SOD) or DNA oxidation. We measured oxidative DNA damage in lymphocytes and hepatocytes, employing the comet assay and lesion-specific enzymes endonuclease III (endo III) and formamidopyrimidine DNA glycosylase (FPG) (19–21). Antioxidant enzyme activities were measured in skeletal muscle (hind- and forelimb) and heart because these tissues experience a large increase in oxygen consumption during exercise (18) and are thought to be relatively susceptible to oxidative stress (22). Using the doubly labeled water technique (23), we previously showed that the daily energy expenditure, and hence oxygen consumption, is over 40% higher in voles with access to running wheels compared to that in nonrunning sibling-matched controls (24).

	MATERIALS AND METHODS

TOP MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

 
Animals

Short-tailed field voles Microtus agrestis, derived from a captive breeding population at Aberdeen, UK, were maintained at 22 ± 3°C. Individuals ( 6 wk old) were exposed to a 16:8 light regime (lights on 0500 h GMT) and, when given running wheels, chose to run primarily during darkness. No individual had access to running wheels before the experiment started. Voles were weaned at d 18, individually housed in shoebox cages containing sawdust and provided, ad libitum, with water and a pelleted rodent diet [rat and mouse breeder and grower diet; Special Diets Services, BP Nutrition, UK), which included vitamin E (103.2 mg/kg), -tocopherol (93.8 mg/kg), ß-carotene (0.9 mg/kg) and vitamin C (8.0 mg/kg)]. All voles were killed by cervical dislocation, complying with a local ethical committee and the U.K. Home Office.

Wheel-running apparatus

The wheel-running apparatus was designed by Dr. Phil Bagley (University of Aberdeen, UK) and consisted of 40 individual cages with attached running wheels. Each wheel was connected to a nonconcentric disc, which operated a microswitch on each complete rotation. Data collected on the microswitch and activity were transmitted to a PC-based acquisition system by an optically isolated logic level converter. The number of revolutions run by each individual was recorded during each 10-min period, over 24 h per day, and downloaded directly onto a spreadsheet package (Microsoft Excel).

Assays

The activities of the antioxidant enzyme catalase (Cat), selenium-dependent glutathione peroxidase (Gpx) and total superoxide dismutase (total-SOD) were measured in six experimental groups: control (no running wheel), 1-d (access to wheel) or 7-d (access to wheel), killed at 0500 h (no rest period after running) or 1300 h (8-h rest period after running). Sixty individuals (30 male, 30 female: 10 per group) were used to determine antioxidant enzyme activity in skeletal muscle (hind- and forelimb) and in the heart. The protocols employed are described fully elsewhere (25).

Oxidative DNA damage was determined in lymphocytes and hepatocytes in three groups, all killed at 1300 h after 8-h rest: control (no wheel), 1 d (access to wheel) and 7 d (access to wheel).

The comet assay, with the modification of an extra step after lysis in which DNA is digested with lesion-specific enzymes, has been described previously (26). Cells are embedded in agarose on a microscope slide and lysed in detergent and high salt to form nucleotides. During electrophoresis at high pH, the relaxed DNA extends out from the nucleoid to form a "comet" tail, and the relative amount of DNA in the tail indicates the frequency of breaks. In the modified comet assay, the nucleoid DNA is digested with endo III, which converts oxidized pyrimidines to strand breaks, or formamidopyrimidine DNA glycosylase (FPG), which recognizes and breaks altered purines, thus increasing both the number of breaks and the intensity of the comet tail.

Statistical analyses

All values reported are means ± SEM, except where indicated. Data were analyzed employing SPSS (Version 9) statistical software and one-way analysis of variance. Significance was indicated by values of P < 0.05.

	RESULTS

TOP MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

 
Body mass did not differ between the experimental groups (Table 1). The mean ± SEM distance run per day was 7.8 ± 1.2 km, with voles running almost exclusively during the 8 h of darkness (lights on 0500 h GMT). No differences were observed between the experimental groups in the activities of Cat, Gpx or total-SOD in either hind- or forelimb skeletal muscle. The activities of heart Cat and Gpx between groups were also not significantly different, although heart total-SOD was, with the lowest levels observed in 1- and 7-d runners killed immediately after exercise (0500 h).

View larger version (15K): [in this window] [in a new window]   FIGURE 1 Oxidative DNA damage (arbitrary units) using the comet assay and lesion-specific enzymes endo III and FPG in lymphocytes of nonrunning control, 1- and 7-d runners killed at 1300 h. Values are means ± SEM, n = 6 in each group. No significant differences were observed between groups using either endo III (P = 0.712) or FPG (P = 0.793).

View larger version (12K): [in this window] [in a new window]   FIGURE 2 DNA oxidative damage (arbitrary units) in hepatocytes of nonrunning controls, 1- and 7-d runners killed at 1300 h. Values are means ± SEM, n = 6 in each group. No significant differences were observed between groups in strand breaks (P = 0.726), with no increase in oxidized bases using the lesion-specific enzymes endo III and FPG.

	DISCUSSION

TOP MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

Forced, endurance and exhaustive exercise generally induce an increase in both enzymatic and nonenzymatic antioxidants in heart and skeletal muscle (11,12,22,27,28). Rats with access, over 20 mo, to voluntary running wheels exhibited elevated activities in skeletal muscle of mitochondrial SOD and cytosolic Gpx, but not Cat or cytosolic SOD compared with that of sedentary controls (18). It has been proposed that the basal levels of antioxidant enzymes, particularly skeletal muscle SOD, are sufficient during moderate oxidative stress (13), although by measuring total-SOD activity we cannot be certain that the activities of the different isoenzymes of SOD did not alter during this exercise protocol.

Moderate-intensity exercise has been shown to increase heart SOD activity in some (27) but not all studies (13). In our study, a significant difference was observed between groups in heart total-SOD activity, although there was no clear pattern of difference between the sedentary and running groups, with the lowest levels of SOD actually observed in the exercise groups killed without any period of rest. A reduction in heart Mn-SOD was observed in rats after exhaustive exercise, although the reason for this appears unresolved (30). It has been suggested that, whereas exercise, particularly to exhaustion, leads to a ROS-induced oxidation of DNA (6,7), nonexhaustive exercise may also enhance DNA repair mechanisms, leading to a decrease in lymphocyte and colonocyte DNA damage (5,17). However, in the present study we found no decrease in either lymphocyte or hepatocyte DNA damage after voluntary exercise.

In conclusion, it would appear that, although voluntary wheel running increased energy expenditure significantly compared to that of sedentary controls (24), this did not appear to induce oxidative stress responses. The fact that, despite the absence of a response, there was no evidence of oxidative DNA damage may be because during voluntary exercise the antioxidant protection and repair mechanisms are sufficient to cope with any accompanying increase in ROS production. The exercise regime employed in this study may also have been insufficient in intensity and/or duration to cause a significant increase in oxidative damage (29) or, perhaps, the antioxidant levels of the rodent diet used were fortified with respect to requirements in voles.

	ACKNOWLEDGMENTS

 
We are grateful to the animal house staff, Dr. Phil Bagley and Suzanne Lumsden for help during this study.

	FOOTNOTES

 
¹ Presented as part of the Waltham International Symposium: Pet Nutrition Coming of Age held at Vancouver, Canada, August 6–7, 2001. This symposium and the publication of symposium proceedings were sponsored by the Waltham Centre for Pet Nutrition. Guest editors for this supplement were James G. Morris, University of California, Davis, Ivan H. Burger, consultant to Mars UK Limited, Carl L. Keen, University of California, Davis, and D’Ann Finley, University of California, Davis.

² Supported, in part, by a grant to J.R.S. from the Biotechnology and Biological Sciences Research Council (SAGE-1 initiative).

⁴ Abbreviations used: cat, catalase; endo III, endonuclease III; FPG, formamidopyrimidine DNA glycosylase; Gpx, glutathione peroxidase; ROS, reactive oxygen species; total-SOD, total superoxide dismutase.

	LITERATURE CITED

TOP MATERIALS AND METHODS RESULTS DISCUSSION LITERATURE CITED

 

1. Paffenberger, R. S., Hyde, R. T., Wing, A. L., Lee, I. M., Jung, D. L. & Kampert, J. B. (1993) The association of changes in physical-activity level and other lifestyle characteristics with mortality among men. N. Engl. J. Med. 328:538-545.[Abstract/Free Full Text]

2. Shephard, R. J. & Shek, P. N. (1998) Associations between physical activity and susceptibility to cancer-possible mechanisms. Sports Med 26:293-315.[Medline]

3. Holloszy, J. O. (1998) Longevity of exercising male rats: effect of an antioxidant supplemented diet. Mech. Ageing Dev. 100:211-219.[Medline]

4. Beckman, K. B. & Ames, B. N. (1998) The free radical theory of ageing. Physiol. Rev. 78:547-201.[Abstract/Free Full Text]

5. Inoue, T., Mu, Z., Sumikawa, K., Adachi, K. & Okochi, T. (1993) Effect of physical exercise on the content of 8-hydroxydeoxyguanosine in nuclear DNA prepared from human lymphocytes. Jpn. J. Cancer Res. 84:720-725.[Medline]

6. Alessio, H. M. (1993) Exercise-induced oxidative stress. Med. Sci. Sports Exerc. 25:218-224.[Medline]

7. Mars, M., Govender, A., Weston, A., Naicker, V. & Chuturgoon, A. (1998) High intensity exercise: a cause of lymphocyte apoptosis. Biochem. Biophys. Res. Commun. 249:366-370.[Medline]

8. Leichtweis, S. B., Leeuwenburgh, C., Parmelee, D. J., Fiebig, R. & Ji, L. L. (1997) Rigorous swim training impairs mitochondrial function in post-ischaemic heart. Acta Physiol. Scand. 160:139-148.[Medline]

9. Phaneuf, S. & Leeuwenburgh, C. (2001) Apoptosis and exercise. Med. Sci. Sports Exerc. 33:393-396.[Medline]

10. Powers, S. K. & Sen, C. K. (2000) Physiological antioxidants and exercise training. Sen, C. K. Packer, L. Hänninen, O. eds. Handbook of Oxidants and Antioxidants in Exercise 2000:221-242 Elsevier Science Amsterdam, The Netherlands. .

11. Leeuwenburgh, C., Hollander, J., Leichtweis, S., Griffiths, , Gore, M. & Ji, L. L. (1997) Adaptations of glutathione antioxidant system to endurance training are tissue and muscle fiber specific. Am. J. Physiol. 272:363-369.

12. Hollander, J., Fiebeg, R., Gore, M., Bejma, J., Ookawara, T., Ohno, H. & Ji, L. L. (1999) Superoxide dismutase gene expression in skeletal muscle: fiber-specific adaption to endurance training. Am. J. Physiol. Regulatory Integrative Comp. Physiol. 277:R856-R862.[Abstract/Free Full Text]

13. Ji, L. L. (1993) Antioxidant enzyme response to exercise and aging. Med. Sci. Sports Exerc. 25:225-231.[Medline]

14. Kretzschmar, M. U. & Muller, D. (1993) Aging, training and exercise: a review of effects of plasma glutathione and lipid peroxidation. Sports Med 15:196-209.[Medline]

15. Radák, Z., Sasvári, M., Nyakas, C., Pucsok, J., Nakamoto, H. & Goto, S. (2000) Exercise preconditioning against hydrogen peroxide-induced oxidative damage in proteins of rat myocardium. Arch. Biochem. Biophys. 376:248-251.[Medline]

16. Salo, D. C., Donovan, C. M. & Davies, K. J. A. (1991) HSP70 and other possible heat shock or oxidative proteins are induced in skeletal muscle, heart and liver during exercise. Free Radical Biol. Med. 11:239-246.[Medline]

17. Okamura, K., Doi, T., Sakarai, M., Hamada, K., Yoshioka, Y., Sumida, S. & Sugawa-Katayama, Y. (1997) Effect of endurance exercise on the tissue 8-hydroxy-deoxyguanosine content in dogs. Free Radical Res. Commun. 26:523-528.

18. Leeuwenburgh, C., Hansen, P. A., Holloszy, J. O. & Heinecke, J. W. (1999) Hydroxyl radical generation during exercise increases mitochondrial protein oxidation and levels of urinary dityrosine. Free Radical Biol. Med. 27:186-192.[Medline]

19. McKelvey, M. V. J., Green, M. H. L., Schmezer, P., Poolzobel, B. L., De Meo, M. P. & Collins, A. (1993) The single-cell gel-electrophoresis assay (Comet assay): a European review. Mutat. Res. 288:47-63.[Medline]

20. Duinská, M. & Collins, A. R. (1996) Detection of oxidised purines and UV-induced photoproducts in DNA of single cells, by inclusion of lesion-specific enzymes in the comet assay. Altern. Lab. Anim. 24:405-411.

21. Collins, A. R. & Horváthová, E. (2001) Oxidative DNA damage, antioxidants and DNA repair: applications of the comet assay. Biochem. Soc. Trans. 29:337-342.[Medline]

22. Lawler, J. M., Powers, S. K., Visser, T., Dijk, H. V., Kordus, M. J. & Ji, L. L. (1993) Acute exercise and skeletal muscle antioxidant and metabolic enzymes: effects of fiber type and age. Am. J. Physiol. Regulatory Integrative Comp. Physiol. 265:R1344-R1350.

23. Speakman, J. R. (1997) Doubly Labelled Water: Theory and Practice 1997 Chapman & Hall London, UK.

24. Selman, C., McLaren, J. S. & Speakman, J. R. (2001) The effects of voluntary exercise on antioxidant enzymes and DNA oxidative damage in a small mammal [unpublished abstract] 2001 Second International Conference on Oxidative Stress and Aging Maui, Hawaii.

25. Selman, C., McLaren, J. S., Himanka, M. J. & Speakman, J. R. (2000) Effect of long-term cold exposure on antioxidant enzyme activities in a small mammal. Free Radical Biol. Med. 28:1279-1285.[Medline]

26. Collins, A. R. (2000) Measurement of oxidative DNA damage using the comet assay. Lunec, J. Griffiths, H. R. eds. Measuring In Vivo Oxidative Damage: A Practical Approach 2000:83-94 Wiley Chichester, UK. .

27. Powers, S., Criswell, D., Lawler, J., Ji, L. L., Martin, D., Herb, R. & Dudley, G. (1994) Rigorous exercise training increases superoxide dismutase activity in the ventricular myocardium. Am. J. Physiol. 266:375-380.

28. Leeuwenburgh, C., Fiebeg, R., Chandwaney, R. & Ji, L. L. (1994) Aging and exercise training skeletal muscle. Responses of glutathione and antioxidant enzyme systems. Am. J. Physiol. Regulatory Integrative Comp. Physiol. 267:R439-R445.

29. Caillaud, C., Py, G., Eydoux, N., Legros, P., Prefaut, C. & Mercier, J. (1999) Antioxidants and mitochondrial respiration in lung, diaphragm, and locomotor muscles: effect of exercise. Free Radical Biol. Med. 9/10:1292-1299.

30. Quintanilha, A. T. & Packer, L. (1983) Biology of vitamin E. Porter, R. Whelan, J. eds. Ciba Foundation Symposium 101 1983:56-69 Pitman London, UK. .

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