Antioxidant Properties of Astaxanthin
What is oxidation and how does it play a role in disease?
How do carotenoids prevent oxidation?
How does astaxanthin compare as an antioxidant with other carotenoids?
In what diseases has oxidation been implicated?
What is the evidence that dietary astaxanthin acts as a potent antioxidant? What is oxidation and how does it play a role in disease?
Technically, oxidation is the chemical process by which an atom,
molecule, or ion robs another of one or more of its electrons. Chemicals exhibiting this tendency for stealing electrons are referred to as oxidizing agents. Perhaps the most familiar oxidizing agent is oxygen itself. We can see many examples of oxygen doing its electron stealing in our everyday lives: the browning of an apple, the rusting of an iron nail, the slow fading of blue jeans. When a material is oxidized, its chemical structure is altered, often irreversibly. The human body is no exception.
We are constantly exposed to oxidative stress. This stress is partly brought on by environmental
parameters, such as air pollution, tobacco smoke, exposure to chemicals, and exposure to ultraviolet
(UV) light or other forms of ionizing radiation (Møller et al. 1996; Papas 1999). Partly, however,
oxidative stress in animals, including humans, arises as a natural result of the body sustaining
itself by aerobic (oxygen-requiring) metabolism (Ames et al. 1993; Davies 1995). Normal aerobic
metabolism produces as its by-products various highly reactive molecules, collectively termed
"oxidants". These oxidants include a variety of electron-stealing molecules known as free radicals,
as well as the highly reactive singlet form of oxygen (Darley-Usmar and Halliwell 1996). Some of
these reactive molecules (e. g., superoxide, hydrogen peroxide, and nitric oxide) are physiologically
useful and, in fact, are necessary for life, but can also be harmful if present in excess or in
inappropriate situations. All of these oxidants can react with various components of a living cell,
such as proteins, DNA, or lipids (fats), thus causing damage by changing the chemical structure of
these components. Such damage has been linked to a number of pathological conditions including
aging (Harman 1981; Ames and Shigenaga 1992), atherogenesis (Steinberg et al. 1989; Esterbauer et al.
1992), ischemia-reperfusion injury (Simpson and Lucchesi 1987; Takayama et al. 1992), infant
retinopathy (Phelps 1987), age-related macular degeneration (Gerster 1991), and carcinogenesis
(Moody and Hassan 1982; Marnett 1987; Breimer 1990). For us, oxygen is therefore both necessary
and harmful; this sobering conclusion has been referred to as the "paradox of aerobic life" (Davies
1995).
The human body has evolved a large array of endogenous antioxidant defenses against oxidative
stress, including antioxidant enzymes such as superoxide dismutase, catalase, and various peroxidases,
as well as the ability to use small molecules with antioxidant activity such as glutathione
(Fahey and Sundquist 1991), the hormone melatonin (Reiter et al. 1997; Reiter 1998), and uric acid
(Yu et al. 1998). However, these endogenous antioxidants do not completely protect against the sum
of oxidative stresses challenging the body, and thus there is net oxidative damage that in the long
term contributes to aging and various diseases. In addition to the body's endogenous defenses
against oxidative stress, diet-derived antioxidants--including ascorbic acid (Vitamin C),
alpha-tocopherol (Vitamin E), and the carotenoids--may be important in protecting against disease
and age-related phenomena (Ames et al. 1993; Davies 1995; Halliwell 1996). Diet-derived
antioxidants may be classified on the basis of their solubility as either lipid-soluble
(i. e., soluble in fats), or water-soluble. Lipid-soluble antioxidants include vitamin E and the carotenoids, while vitamin C is a common water-soluble antioxidant. A more detailed discussion of free radicals and the chemistry of oxidation can be found
in the oxidation properties. References: Ames, B. N. and Shigenaga, M. K. (1992) Oxidants are a major contributor to aging.
Ann. N. Y. Acad. Sci., 663:85-96. Breimer, L.H. (1990) Molecular mechanisms of oxygen radical carcinogenesis and mutagenesis:
the role of DNA base damage. Mol. Carcinog., 3:188-197. Darley-Usmar, V. and Halliwell, B. (1996) Blood radicals: reactive nitrogen species,
reactive oxygen species, transition metal ions, and the vascular system. Pharm. Res., 13(5):649-662. Davies, K. J. (1995) Oxidative stress: the paradox of aerobic life. Biochem. Soc. Symp., 61:1-31. Esterbauer, H., J. Gebicki, H. Puhl, and G. Jurgens. (1992) The role of lipid peroxidation and
antioxidants in oxidative modification of LDL. Free Radic. Biol. Med., 13:341-390. Fahey, R. C. and Sundquist, A. R. (1991) Evolution of glutathione metabolism.
Adv. Enzymol. Related Areas Mol. Biol., 64:1-53. Gerster, H. (1991) Antioxidant protection of the ageing macula. Age Ageing, 20:60-69. Halliwell, B. (1996) Oxidative stress, nutrition, and health. Experimental strategies for
optimization of nutritional antioxidant intake in humans. Free Radic. Res., 25(1):57-74. Harman, D. (1981) The aging process. Proc. Natl. Acad. Sci. USA 78:7124-7128. Marnett, L.J. (1987) Peroxyl free radicals: potential mediators of tumor initiation and
promotion. Carcinogenesis, 8:1365-1373. Møller, P., Wallin, H., and Knudsen, L. E. (1996) Oxidative stress associated with exercise,
psychological stress, and life-style factors. Chem. Biol. Interact., 102(1):1-36. Moody, C.S., and H.M. Hassan. (1982) Mutagenicity of oxygen free radicals.
Proc. Natl. Acad. Sci. USA, 79:2855-2859. Papas, A.M. (1999) Determinants of antioxidant status in humans. In: Papas, A.M. [ed],
Antioxidant Status, Diet, Nutrition, and Health. Boca Raton: CRC Press. Phelps, D.L. (1987) Current perspectives on vitamin E in infant nutrition. Am. J. Clin. Nutr., 46(suppl.):187-191. Reiter, R. J. (1998) Oxidative damage in the central nervous system: protection by melatonin.
Prog. Neurobio.,l 56(3):359-384. Reiter, R. J., Carneiro, R. C., and Oh, C. S. (1997) Melatonin in relation to cellular
antioxidative defense mechanisms. Horm. Metab. Res., 29(8):363-372. Simpson, P.J., and B.R. Lucchesi. (1987) Free radicals and myocardial ischemia and reperfusion
injury. J. Lab. Clin. Med., 110:13-30. Steinberg, D., S. Parthasarathy, T.E. Carew, J.C. Khoo, and J.L. Witztum. (1989)
Beyond cholesterol. Modifications of low-density lipoprotein that increase its atherogenicity.
N. Eng. J. Med., 320:915-924. Takayama, F., T. Egashira, Y. Kudo, and Y. Yamanaka. (1992) Chemiluminescence-HPLC assay of
phosphatidylcholine hydroperoxide generated by ischemia-reperfusion in the liver of rats.
Biochem. Pharmacol., 44:2412-2414. Yu, Z. F., Bruce-Keller, A. J., Goodman, Y., and Mattson, M. P. (1998) Uric acid protects
neurons against excitotoxic and metabolic insults in cell culture, and against focal ischemic brain
injury in vivo. J. Neurosci. Res., 53(5):613-625. How do carotenoids prevent oxidation? All carotenoids share a structural feature termed "polyunsaturation",
that is to say, they have several "unsaturated" or "double" bonds (double bonds between two adjacent
carbon atoms). This is in contrast to "saturated" or "single" bonds. When double bonds are
arranged in a series alternating with single bonds, they are termed "conjugated"--this means that the
electrons that make up the double bonds in the linear chain are "delocalized", or shared evenly over
the whole chain. This makes the whole chain relatively electron-rich. This conjugated double bond
structure is responsible for the characteristic yellow, orange, or red colors typical of carotenoids.
The difference in colors depends primarily on how many double bonds are conjugated, or in other
words, over how long a chain the electrons can be delocalized. Conjugated double bonds are very
chemically stable, yet are capable of specific chemical reactions that require their electron-rich
yet stable structure. For example, if a carotenoid loses one electron and becomes a carotenoid
cation (positively charged ion), the resulting charge of +1 is distributed over the electron-rich
chain, a much more stable situation than if the charge were limited to a single location on the
compound. In mammalian and human cells, carotenoids protect from oxidative damage by two general mechanisms:
In photosynthetic cells (as in plants and algae), and perhaps in cells exposed to high light levels,
there are additional protective mechanisms, including:
A more detailed discussion of the radical-scavenging
and singlet oxygen-quenching mechanisms of carotenoids can be found in the mechanisms of carotenoid Antioxidant Behavior
Several studies have compared astaxanthin's antioxidant activity with that of other carotenoids.
It should be kept in mind when reviewing these studies that measurement of antioxidant activity is
highly dependent on the experimental system used, and one should be cautious in comparing results of
separate studies, or of extending the conclusions of a given study beyond its experimental limits.
As is the case with other carotenoids, astaxanthin is a potent quencher of singlet oxygen.
One comprehensive study found astaxanthin to be twice as effective as beta-carotene (and about 80
times more effective than vitamin E) in quenching singlet oxygen in chemical solution (Di Mascio et al
. 1991); lycopene was found to be about a third more effective than astaxanthin. Similar results
were found by researchers working with an in vitro system of human blood cells treated with
different carotenoids and then exposed to singlet oxygen; again, lycopene was found to be more
effective than astaxanthin, which in turn was more effective than beta-carotene (Tinkler et al.
1994). A second major antioxidant role of carotenoids is in the scavenging of free radicals. An elegant
study of carotenoid-radical reactions in chemical solution clearly demonstrated that reactivity
rates depend not only on the carotenoid but also on the nature of the radical (Mortensen et al. 1997).
In one study, astaxanthin was approximately as effective as canthaxanthin (a xanthophyll
structurally similar to astaxanthin), and about 50% more effective than beta-carotene and
zeaxanthin, in preventing fatty acid peroxidation in chemical solution (Terao 1989). In a
membrane model, astaxanthin was found to be more effective at scavenging peroxyl radicals than was beta-carotene (Palozza and Krinsky 1992). Another study using membrane models found similar
results, with astaxanthin better at delaying lipid peroxidation than zeaxanthin, canthaxanthin, or beta-carotene (Lim et al. 1992). A tissue culture model demonstrated that astaxanthin was superior to beta-carotene or vitamin E in protecting the cells from herbicide-induced oxidative stress (Lawlor and O'Brien 1995). References: Di Mascio, P., Murphy, M. E., and Sies, H. (1991) Antioxidant defense systems: the role of
carotenoids, tocopherols, and thiols. Am. J. Clin. Nutr., 53:194S-200S. Tinkler, J. H., Böhm, F., Schalch, W., and Truscott, T. G. (1994) Dietary carotenoids protect
human cells from damage. J. Photochem. Photobiol. B, 26:283-285. Mortensen, A., Skibsted, L. H., Sampson, J., Rice-Evans, C., and Everett, S. A. (1997)
Comparative mechanisms and rates of free radical scavenging by carotenoid antioxidants.
FEBS Letters, 418:91-97. Terao, J. (1989) Antioxidant activity of beta-carotene-related carotenoids in solution. Lipids, 24:659-661. Palozza, P. and Krinsky, N. I. (1992) Astaxanthin and canthaxanthin are potent antioxidants in
a membrane model. Arch. Biochem. Biophys., 297:291-295.
Lim, B. P., Nagao, A., Terao, J., Tanaka, K., Suzuki, T., and Takama, K. (1992) Antioxidant
activity of xanthophylls on peroxyl radical-mediated phospholipid peroxidation.
Biochim. Biophys. Acta, 1126:178-184. Lawlor, S. M. and O'Brien, N. M. (1995) Astaxanthin: antioxidant effects in chicken embryo
fibroblasts. Nutr. Res., 15:1695-1704.
Many human diseases and degenerative processes have been linked in some way to the action of free
radicals. Free radicals are not necessarily the only cause for these conditions, but may well make
the human body more susceptible to other disease-initiating factors, may enhance the progression of
diseases, and may inhibit the body's own defenses and repair processes. The following conditions
involving multiple organs have all been linked to free radicals (Cross et al. 1987):
In addition, a number of single-organ conditions have been related to free radicals
(Cross et al. 1987):
It is quite clear that human health depends to a large extent on the body's ability to control
free radicals and thus reduce oxidative damage to tissues, cells, and DNA. To that end, antioxidants
play an essential role in disease prevention, in longevity, and in overall well-being.
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References:
Cross, C. E., B. Halliwell, E.T. Borish, W.A. Pryor, B.N. Ames, R.L. Saul, J.M. McCord, and D. Harman. (1987) Oxygen radicals and human disease.
Ann. Intern. Med., 107:526-545.
Astaxanthin, like vitamin E, is a lipophilic (fat-soluble) antioxidant, and thus might be expected to exert its antioxidant properties in lipid-rich cell membranes and tissues. It was shown in two published studies that, in rats deprived of vitamin E, the resistance of lipids (fats) to oxidation was largely restored by feeding the animals astaxanthin (Kurashige et al. 1990; Miki 1991).
In the first study (Kurashige et al. 1990), rats were fed a vitamin E-deficient diet, with or without astaxanthin supplementation at 1 mg per 100 mg feed, for two to four months; control rats received a vitamin E-sufficient diet. Mitochondria were isolated from liver, and erythrocyte ghosts prepared from blood samples. Membrane preparations (intact mitochondria or erythrocyte ghosts) were subjected to oxidation by superoxide generated in situ by an iron-catalyzed xanthine oxidase system. An index of lipid peroxidation, the formation of thiobarbituric acid-reactive (TBA-reactive) substances, was measured colorimetrically. Mitochondria from vitamin E-deficient rats were preincubated with various concentrations of either astaxanthin or vitamin E, and then exposed to superoxide. The percent inhibition of TBA-reactant formation (as compared to controls with no added antioxidant) was measured. At all concentrations tested, astaxanthin inhibited the formation of TBA-reactants more effectively than did vitamin E, and the IC50 concentration was approximately 3 orders of magnitude lower for astaxanthin than for vitamin E. In this system, astaxanthin was a more effective antioxidant than was vitamin E. TBA-reactive metabolite levels were compared between erythrocyte ghost preparations from the three treatment groups. The amount of TBA-reactants was about 15-fold greater in the erythrocyte ghosts from vitamin E-deficient rats than in those from the control group. In erythrocyte ghosts from the astaxanthin-supplemented, vitamin E-deficient rats, the level of TBA-reactants was elevated only about 6-fold over that of the controls, i. e., 2.5-fold less than in the vitamin E-deficient, non-astaxanthin supplemented animals. This indicates that dietary administration of astaxanthin, in the absence of vitamin E, partially restored the in vitro oxidation resistance of erythrocyte membrane ghosts to the levels found in vitamin E-sufficient rats.
In the second study (Miki 1991), rats were fed a vitamin E-deficient diet, with or without astaxanthin supplementation at 1 mg per 100 mg feed, for four weeks; control rats received a vitamin E-sufficient diet. The susceptibility to oxidation of erythrocyte ghosts was assayed by a similar xanthine oxidase-generated superoxide system and measurement of TBA-reactants. Lipid peroxidation was high in the vitamin E-deficient rats and negligible in control animals. Rats that received the astaxanthin supplementation had peroxidation levels about half that of the vitamin E-deficient rats, again indicating that dietary astaxanthin restored much though not all of the vitamin E-dependent oxidative resistance of the erythrocyte membranes.
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References:
Kurashige, M., Okimasu, E., Inoue, M., and Utsumi, K. (1990) Inhibition of oxidative injury of biological membranes by astaxanthin. Physiol. Chem. Pys. & Med. NMR, 22:27-38. Miki, W. (1991) Biological functions and activities of animal carotenoids. Pure Appl. Chem., 63(1):141-146.
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