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First published online August 22, 2008
Journal of Experimental Biology 211, 2859-2864 (2008)
Published by The Company of Biologists 2008
doi: 10.1242/jeb.017970
The effects of short-term antioxidant supplementation on oxidative stress and flight performance in adult budgerigars Melopsittacus undulatus
1 Division of Environmental and Evolutionary Biology, Institute of Biomedical
and Life Sciences, University of Glasgow, Glasgow, UK
2 WALTHAM® Centre for Pet Nutrition, Waltham-on-the-Wolds, Melton-Mowbray,
Leicestershire LE14 4RT, UK
* Author for correspondence (e-mail: k.arnold{at}bio.gla.ac.uk)
Accepted 8 July 2008
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Summary |
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 TOP Summary INTRODUCTIONMATERIALS AND METHODSFlight escape time recordingRESULTSDISCUSSIONReferences |
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Key words: exercise, carotenoids, oxidative stress, MDA, TBAR, comet assay
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INTRODUCTION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSFlight escape time recordingRESULTSDISCUSSIONReferences |
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). Levels of
oxidative stress are therefore likely to be important fitness determinants,
and identifying the factors influencing an individual's susceptibility to
oxidative stress is of great interest. Physical activity is likely to be one
factor influencing oxidative status because raising metabolism, as during
exercise, will increase the production of ROS
(Urso and Clarkson, 2003).
Indeed, increased ROS production during exercise has been demonstrated in both
humans and other animals (Kanter et al.,
1988; O'Neil et al., 1996). An endogenous antioxidant system, well
conserved across all taxa, controls and neutralises the ROS produced during
exercise; however, prolonged strenuous exercise may overwhelm this antioxidant
system (Sjodin et al., 1990).
In this case dietary antioxidants may assist in removing free radicals and
reducing oxidative stress. In birds, take-off is one of the most energetically
demanding aspects of flight (Swaddle et
al., 1999) and is likely to be associated with a burst of ROS
production.
Since oxidative stress may cause damage to tissue
(Bailey et al., 2007), there is
growing interest in the possible role of dietary antioxidants in preventing
exercise-induced oxidative stress, and improving performance
(Powers et al., 2004). Much of
the interest in this area has focused on the effects of antioxidant
supplementation in human athletes, though the results are far from clear
(Urso and Clarkson, 2003).
Data from other, particularly non-model, taxa have the potential to improve
our understanding of these links between dietary antioxidants and exercise. In
birds high velocity initial vertical take-off, regardless of other escape
strategies, is also vital in avoiding predation
(Kenward, 1978). Although
morphological traits such as wingtip shape
(Swaddle and Lockwood, 2003)
and fat load (Kullberg et al.,
1996) have previously been demonstrated as important in
determining flight performance in birds, it is possible that antioxidant
status may also mediate flight performance by limiting oxidative damage
associated with exercise. The extent to which flight exercise affects
oxidative stress in birds, and how dietary antioxidants may ameliorate this,
is unclear. Recently, Costantini and colleagues demonstrated that oxidative
stress was increased with long flights in homing pigeons Columba
livia, the first direct evidence of an oxidative cost to flight in birds
(Costantini et al., 2008). In
birds, evidence suggests that short flights tend to use glycogen stores for
energy metabolism, whereas during long flights free fatty acids, produced by
hydrolysis of adipose tissue, are oxidised by flight muscles
(Jenni-Eiermann and Jenni,
1991; Schwilch et al.,
1996). Recent evidence suggests that anaerobic exercise may lead
to increased ROS production through different pathways from aerobic exercise
(Shi et al., 2007); thus
take-off flight may have different oxidative costs than endurance flight. When
fed on an antioxidant-rich diet, an individual should have a greater supply of
available antioxidants and will be better equipped to remove free radicals
associated with flight activity than when receiving a reduced antioxidant
diet. Indeed, it has recently been demonstrated that male zebra finches
Taeniopygia guttata fed supplementary carotenoids (nutrients
displaying antioxidant properties) flew faster than controls, although
oxidative stress was not measured (Blount
and Matheson, 2006).
In this study, we fed individual budgerigars Melopsittacus
undulatus (Shaw 1805) both an enhanced and a reduced quality diet. The
main nutritional difference between these diets was in antioxidant
concentration. In all cases, each bird received the two diets consecutively,
and acted as its own control. After receiving each diet, we measured
post-flight oxidative stress. We examined two indices of oxidative stress;
malondialdehyde (MDA) level and comet assay. MDA is one of the major products
of lipid peroxidation, after transition metal decomposition of lipid
peroxides. High performance liquid chromatography (HPLC) can be used to
examine the prevalence of MDA in its free form. The comet assay was developed
by Collins and colleagues for measuring breaks in the DNA of lymphocytes and
other single cells (Collins et al.,
1997). We also calculated an average flight escape time across 4
days, in order to assess whether dietary antioxidants were capable of limiting
flight performance. Our specific aims were to determine whether manipulating
supplementary dietary antioxidants affected (1) post-flight oxidative stress
levels and (2) take-off flight escape time.
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MATERIALS AND METHODS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSFlight escape time recordingRESULTSDISCUSSIONReferences |
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At the WALTHAM® Centre for Pet Nutrition, 12 male and 12 female green
and yellow (wild-type colour) budgerigars were selected from stock aviaries.
These domesticated budgerigars have been selected for large body size, so
skeletally are approximately 80% bigger than wild budgerigars. Each bird was
weighed, health checked and randomly caged with a member of the opposite sex
before being placed together in cages measuring 1002 mmx545 mmx410
mm. These experimental cages were smaller than the stock aviaries, though they
had multiple perches, allowing short flights between them. A previous
observational study showed that birds did fly in these cages, with a mean
frequency of 11.8±2.7 short flights per hour, when undisturbed (S.D.L.,
unpublished observation). However, the cages did not allow long, uninterrupted
flights, so the birds were relatively sedentary. Throughout this experiment
birds were not breeding, and temperature and day length were held constant.
Birds had ad libitum access to water and food throughout the
experiment, except during intake trials. Grit was provided in a separate
container. Birds were given 
10g of seed each per day, which was weighed
in and out of the cage on a daily basis. Water and cage lining were also
changed daily.
Diet manipulations
In this experiment we manipulated the level of an antioxidant-rich diet
supplement within a standard seed mix for adult budgerigars. Nutrivit® is
a nutritional supplement in the form of a small seed-like grain that is mixed
into the seed mix Trill® produced by Mars® (Mars, Csongrad, Hungary).
The main nutritional effect of Nutrivit® is to provide a higher
concentration of antioxidants than is present in seed alone. Thus, any
differences between birds on the two diets are likely to be mediated by
antioxidants. Every bird on the trial received a baseline diet consisting of
seed mix (Trill®) with a standard inclusion of Nutrivit® for 4weeks
prior to the start of the experiment. This was the same diet that the birds
usually received in their home aviaries. This ensured the birds were used to
the Nutrivit® supplement before beginning the experiment. Then, two
experimental diets were made up using identical proportions of seeds, but
differing in the percentage inclusion of Nutrivit®. The enhanced quality
diet (EQ) contained a 10% inclusion (by mass) of Nutrivit®. The reduced
quality diet (RQ) contained a 1% inclusion (by mass) of Nutrivit®.
Concentrations of antioxidants in the EQ diet were: 
-tocopherol
1675i.u.g–1; retinol 220,000i.u.g–1;
β-carotene 1.14µgg–1; lutein
41.7µgg–1; zeaxanthin 14.75µgg–1; and
in the RQ diet were: -tocopherol 174i.u.g–1; retinol
22,000i.u.g–1; β-carotene
0.654µgg–1; lutein 40.5µgg–1;
zeaxanthin 13.65µgg–1. The birds were retained in their
caged pairs and were randomly assigned to one of two groups. Half the pairs
received the EQ diet for the first experimental block, followed by the RQ diet
for the second block. The other half of the birds received the RQ diet for the
first experimental block, followed by the EQ diet for the second block.
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Flight escape time recording |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSFlight escape time recordingRESULTSDISCUSSIONReferences |
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) with
some modifications. The cage used was 2 m high by 70 cm wide by 70 cm deep.
The front wall of the cage was made of transparent Perspex. Coloured masking
tape was taped horizontally across the cage at 10 cm increments above the
floor, on both the transparent front panel and the back wall. A hinged 20
cm3 holding box was used to release the birds. The lid of the box
was transparent, and was attached to a string. When pulled sharply this
collapsed the side panels, and stimulated escape from ground level to a perch
situated at the top of the cage. The loud sound of the sides hitting the
ground meant each bird exhibited a standardised vertical escape flight.
On day 22 all birds were allowed to acclimate to the flight apparatus in
groups of six. On day 23 of each experimental block, the flight cage was
positioned at a fixed location in an enclosed procedures room, and video
recording apparatus was fixed on a tripod 3 m from the cage. Birds were then
placed in the holding box and flown individually as described previously
(Veasey et al., 2001);
however, in this study we calculated escape time from 10 to 50 cm height.
Following this, the birds were given two trial flights each day between day 23
and day 26, and three flights on day 27 (11 flights in total). Each bird had a
10 min break between flights. By watching videos back frame-by-frame we could
calculate escape time in 0.04 s intervals. Because of the holding cup design,
the bird could not be observed flying over the first few centimetres. Thus,
the escape time measurement started when the head passed a line 10 cm from the
ground, and finished when the head passed a line 50 cm high. We used a mean
escape time across all 11 flights in our analysis.
Blood and plasma analysis
We blood sampled every bird prior to the experimental phase, after 28 days
of receiving their baseline diet, then on day 28 of each experimental block,
around 24 h after the final exercise trial. Individual birds were weighed and
tarsus, wing and mass measurements were taken. A small blood sample
(250µl) was taken from the jugular vein via a syringe; 50
µl of the whole blood was diluted in 1 ml PBS immediately in a sodium
citrate tube for comet assay. The rest of the blood was transferred to 75
µl capillary tubes. The capillary tubes of blood for antioxidant and MDA
analysis were centrifuged and haematocrit readings were taken from each.
Plasma was stored at –70°C, prior to antioxidant and MDA
analysis.
Antioxidant extraction and analysis
At the University of Glasgow, we analysed levels of -tocopherol,
lutein, zeaxanthin and retinol in order to uncover any effect of feeding
treatment or exercise on plasma antioxidant profile. To extract the
antioxidants, 40µl of ethanol was added to 20µl of plasma and vortexed
thoroughly; 50 µl of hexane was then added and vortexed before the hexane
layer, containing the antioxidants was drawn off. This was repeated with 40
µl of hexane before the hexane extract was placed in a SpeedVac model SPD
111V (Thermo Electron Corp., San Jose, CA, USA) for 20min. The final
antioxidant extract was then dissolved in 20 ml of methanol.
A Spectra model 8800 HPLC pump system with a Phenomenex 250mmx2mm
i.d. column (Phenomenex, Macclesfield, UK) was employed to determine the
antioxidant composition of each sample. We used HPLC at a flow rate of
0.2mlmin–1 with a mobile phase of water/acetonitrile
(2.5:97.5), and water/ethyl acetate (2.5:97.5) in a gradient elution. Using a
Diode array absorbance detector type Thermo SPECTRAsystem UV6000LP (Thermo
Electron Corp.), we detected carotenoids by absorbance at 445nm,
-tocopherol at 295nm and retinol at 325 nm. Peaks were identified by
comparison with chromatography and retention times of several standards
(Sigma, Poole, UK; Fluka, Gillingham, UK).
MDA analysis
The MDA method was based on that of Young and Trimble
(Young and Trimble, 1991).
Thiobarbituric acid (0.044 mol l–1,100 µl) and phosphoric
acid (1.22moll–1, 100µl) were mixed together and added to
50 µl of plasma (per bird) in a test tube. An inert atmosphere was created
by applying a nitrogen blanket, and the test tubes were sealed and vortexed
prior to heating (60 min, 70–75°C). Samples were cooled in water,
then 200 µl was transferred to a centrifuge tube containing sodium
hydroxide (1 mol l–1, 100 µl). Methanol (500 µl) was
added and mixed. Samples were centrifuged (10 min, 12,000 g)
and the supernatant analysed on a Summit HPLC system (Dionex, Idstein,
Germany) using Chromeleon software (Dionex). An Acclaim 120 C18 5 µm 4.6
mmx250 mm column (Dionex) and guard were used with fluorescence
detection (excitation 532 nm and emission 553 nm). The mobile phase was
isocratic, 40:60 methanol:phosphate buffer (40 mmol l–1, pH
6.5), with a flow rate of 1 ml min–1, and a run time of 7
min. Samples were assayed against a standard of malonaldehyde bis(dimethyl
acetal; Sigma Aldrich) that was simultaneously taken through the same
procedure.
Comet assay
We performed the alkaline comet assay procedure according to Tice and
colleagues at two different pH values for each bird
(Tice et al., 2000):
electrophoresis at low pH (0.03 mol l–1 NaOH) to reveal
single stranded breaks and electrophoresis at high pH (0.3 mol
l–1 NaOH), which converts alkali labile sites into single
strand breaks. Slides were made and analysed on the same day as blood
sampling. We used 50 µl SYBR Gold in each gel for visualisation of comets.
Slides were viewed by epifluorescence microscopy using an Olympus BX-51
(Olympus Optical Co., Tokyo, Japan) with a 460 nm UV filter for SYBR Green.
Komet software (v.6, Kinetics Imaging, Nottingham, UK) was used for image
analysis on 100 randomly selected cells for each bird and treatment. Cells
were scored according to the percentage DNA in the comet head, as a measure of
DNA intactness.
Intake trials
In order to ensure that the birds were eating the Nutrivit® supplement,
and also to assess selection or otherwise of the high antioxidant food, we
performed an intake trial during each experimental block. Each morning at
08:00 h on days 24, 25 and 26 of each experimental block, feeding dishes were
removed from each cage for a period of 2 h to standardise hunger, and cages
were cleaned. After 2 h without food, pairs were separated with the female on
the left of the cage in all cases. Individual budgerigars were presented with
a food bowl containing a prepared 10 g sample of their experimental diet
containing very precisely weighed seed, and known numbers of Nutrivit®
pieces. The dish and tray were removed after 2 h, along with any spilled seed.
The contents of the dish and cage floor were then sorted and weighed, and the
number of uneaten Nutrivit® particles was counted and subtracted from the
original total.
Statistical analysis
Data from the EQ and RQ diet experiments were analysed using generalised
linear mixed models (GLMM; Proc Mixed in SAS version 9; Cary, NC, USA) with a
normal error distribution. Individual identity was entered as a random factor
into the model to control for the non-independence of repeated measures from
the same individual. The order in which each bird received the diets, the diet
and sex were entered into the models as factors, and morphometric, escape time
and blood measurements were entered as covariates. All models used a
Satterthwaite correction, which can result in degrees of freedom that are not
integers. Models were developed using backward elimination starting with the
highest order interaction term. We tested for all two-way interactions between
main effects and covariates, and removed non-significant factors stepwise from
the full model beginning with the interaction terms. We used
P<0.05 for statistical significance. All significance tests were
based on the F distribution. Comet data were proportions and so were
arcsine square-root transformed. Count data were square-root transformed prior
to analysis. Means with standard errors (s.e.m.) are reported throughout the
text. In some cases problems during blood sampling or repeated failure to fly
in some birds resulted in a sample size unequal to 24 birds. One bird was
omitted from all analyses because it was observed to exhibit abnormal
behaviour throughout the experiment and subsequently had atypical results.
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RESULTS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSFlight escape time recordingRESULTSDISCUSSIONReferences |
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When individuals were maintained on the RQ diet they had significantly higher levels of MDA than when on the EQ diet (GLMM F1,37=8.37, P=0.0064, see Fig. 1A). Birds had a higher proportion of intact DNA, measured by high pH comet assay, which assesses strand breaks and alkali labile sites, on the enhanced antioxidant diet than on the reduced antioxidant diet (GLMM F1,35=5.3, P=0.0273, see Fig. 1B). There was no effect of diet on the low pH comet (P>0.5, see Fig. 1C). There was no significant effect of diet order on any measure of oxidative stress, showing there were no carry-over effects between experimental blocks.
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There was no effect of diet on flight escape time (EQ, 0.58±0.1 s;
RQ, 0.57±0.1 s). There was a significant, positive relationship between
mass and flight escape time (GLMM F1,32=7.39,
P=0.011, see Fig. 2)
but no interaction between diet and mass affecting escape time (GLMM
F1,17.7=2.81, P=0.112). There was no relationship
between comet assay, plasma MDA or plasma antioxidant concentration and flight
escape time. There was no effect of diet on blood plasma concentration of
-tocopherol, lutein, zeaxanthin or retinol (P>0.1 in all
cases), and no significant effect of diet order on plasma levels of the
different antioxidants (P>0.1 in all cases), demonstrating that
there were no carry-over effects of antioxidant supplementation (see
Fig. 3).
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Birds consumed significantly more Nutrivit® on the EQ diet (1.07±0.23 pieces per 2 h) than on the RQ diet (0.08±0.039 pieces per 2 h; GLMM F1,44=19.32, P<0.0001). However, there were no differences in the mass of seed eaten.
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DISCUSSION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSFlight escape time recordingRESULTSDISCUSSIONReferences |
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;
Aniagu et al., 2006). Increases
in MDA after exercise have also been shown in other taxa (for a review, see
Vollaard et al., 2005). The
high pH comet assay is thought to reveal alkali labile sites in DNA,
representing several different forms of oxidative damage, rather than just
single stranded breaks as found in low pH comet
(Rojas et al., 1999). Although
we found no difference between EQ and RQ diet in our low pH comet assay, the
higher abundance of alkali labile sites on a reduced antioxidant diet suggests
that dietary antioxidants prevented some exercise-induced oxidative damage of
DNA.
Although in a short-term study it is difficult to assess the biological
importance of exercise-induced damage, we suggest that increases in DNA damage
may have long-term consequences. Lymphocytes are the most prevalent cells used
in comet assays of avian blood (C.A.T., unpublished data). Avian lymphocytes
are only produced early in development, so can be repaired but not replaced
during adulthood, and circulate for a high proportion of an animal's life
(Glick, 1979). Increases in DNA
damage, including alkali labile sites, can eventually lead to apoptosis
(Monti et al., 1992).
Long-term DNA damage may induce a reduction in lymphocyte number and therefore
immunocompromise an individual. The preventative action of dietary
antioxidants on exercise-induced oxidative stress may thus have important
effects besides those pertaining to exercise performance. Hartmann and
colleagues previously reported that dietary vitamin E prevented oxidative
damage of DNA in human subjects after treadmill running
(Hartmann et al., 1995), though
to our knowledge, ours is the first study to report dietary antioxidants
preventing exercise-induced DNA damage in birds.
Increased oxidative stress was predicted to be one of the factors involved
in limiting strenuous exercise in animals, where there may be a trade-off
between minimising damage to tissue, yet maximising the chances of escape from
a predator. Over 4 days we calculated average take-off escape time, an
important aspect of fitness, for each bird when on EQ and RQ diets. We found
that there was no effect of dietary antioxidant intake on escape time. In
contrast, Blount and Matheson reported that zebra finches Taeniopygia
guttata, a small passerine bird, receiving a carotenoid-enhanced diet
flew faster than controls (Blount and
Matheson, 2006). In their study oxidative stress was not measured,
and it is possible that the difference was due to an effect of carotenoids
aside from antioxidative protection. Indeed, carotenoids are useful in their
role in immune signalling and as precursors for retinoids
(Hartley and Kennedy, 2004). Of
course, the difference may also represent a species-specific difference in
behaviour.
In our experiment it is possible, though hard to prove, that the birds
always flew as fast as possible, but they paid a price for this through
increased oxidative stress. The consequences of this increased oxidative
stress are unclear from a short-term experiment; although there is some
evidence that oxidative stress can cause muscle damage
(Bailey et al., 2007), other
studies have found no effect of oxidative stress on muscle performance.
Indeed, there is some evidence that increasing ROS production is necessary to
optimise muscle performance (Reid,
2001). Measuring flight speed repeatedly over a longer course of
time on each diet may have revealed differences in performance, and it is
possible that oxidative damage accumulating in muscle tissue is more important
in affecting muscle stamina, rather than burst exercise. For example, one
recent study showed that the length of flight in homing pigeons Columba
livia was directly related to oxidative stress after flight
(Costantini et al., 2008). In
our study, although we expect the birds exerted maximal effort, the flight
procedure was quick, and birds were rested between each flight. It has been
shown that energy metabolism in short flights is quite different from that
during long flights (Schwilch et al.,
1996). Thus, flying birds for long periods, perhaps using a wind
tunnel, or flying birds more often without rest, would reveal further
differences in oxidative stress and flight performance.
In this study, resolution of different flight escape times was achieved
using a standard video camera. This meant flight duration could only be
measured to the nearest 0.04 s. Given the short flight distance, any
difference in within-individual flight performance may have required a more
sensitive filming technique. In order to properly assess flight take-off, a
high speed camera would attain a more effective measure of performance (e.g.
Williams and Swaddle, 2003).
This is especially true over the first few centimetres, potentially those most
important in predator evasion (Kenward,
1978). However, the flight protocol employed here was certainly
suitable to induce exercise, and there were differences in oxidative stress
apparently mediated by the flight procedure. In this context the design was
successful, and similar apparatus has been used previously to assess
differences in vertical flight escape times
(Veasey et al., 1998;
Veasey et al., 2001; Blount
and Matheson, 2005).
In spite of the effect of our dietary treatment on oxidative stress, we
found that there was no significant difference in plasma levels of lutein,
zeaxanthin, -tocopherol or retinol after each 4week block. However, we
do not believe this indicates a failure in the dietary treatment. We found
that during the 2 h intake trials, intake of Nutrivit®, but not seed, was
significantly increased on the EQ diet compared with the RQ diet. It is
possible that the EQ birds had greater levels of antioxidants in other organs,
though not in blood plasma. For example, it has been shown repeatedly (e.g.
Surai et al., 2002;
Karadas et al., 2005) that
birds are capable of storing antioxidants in their liver at levels far greater
than those seen in plasma. However, our experimental measurements indicated
oxidative damage was increased after the birds received the RQ diet,
regardless of the diet order. If antioxidants from the EQ diet were stored, we
may have expected a lesser effect of exercise on oxidative stress after the RQ
diet in birds that received the RQ diet in the second experimental block,
which was not the case. Indeed, there was no effect of diet order on any
plasma antioxidant we measured. Other recent studies of antioxidants in birds
have found no effect of increased dietary antioxidants on plasma antioxidant
levels (e.g. Biard et al.,
2006). They did, however, find effects of the supplementation on
other parameters, supporting the idea that although the antioxidants are not
evident in plasma, they may have been used in other physiological systems.
While retinol and -tocopherol are increased in Nutrivit® to
relatively high concentrations, other antioxidants, which we have not sampled,
are possibly more important in this species. By assessing other important
antioxidants perhaps we would attain a more effective estimate of antioxidant
status.
Given the apparent beneficial effects of antioxidants, it could be expected that animals may selectively choose antioxidant-rich food items. We found no evidence that birds were selectively eating the antioxidant supplement. On the RQ diet Nutrivit® was seldom eaten at all, whereas on the EQ diet the average number of pieces eaten was around one during the 2 h palatability trial. This suggests that rather than selecting Nutrivit®, the birds ate it by chance when it was mixed into their seeds. However, after a 2 h deprivation it is conceivable that the birds selected foods based on their calorific content, rather than their antioxidant status.
In our study, we found evidence for exercise-induced lipid peroxidation and DNA damage. We also found that dietary supplementation with an antioxidant supplement was capable of countering this increased oxidative stress. Although we found no evidence of dietary antioxidants modifying exercise performance, longer term studies will be crucial in elucidating the roles of both oxidative stress and dietary antioxidants in determining physical capabilities in animals. DNA damage may have implications for immune function, as well as exercise performance. Thus access to dietary antioxidants may be an important fitness determinant, through various physiological pathways.
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Acknowledgments |
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