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First published online April 18, 2006
Journal of Experimental Biology 209, 1651-1661 (2006)
Published by The Company of Biologists 2006
doi: 10.1242/jeb.02195
Metabolic scaling associated with unusual size changes during larval development of the frog, Pseudis paradoxus
Departamento de Fisiologia, Instituto de Biociências, Universidade de São Paulo, Rua do Matão, Travessa 14, no 321, Cidade Universitária, CEP 05508-900, São Paulo, SP, Brazil
* Author for correspondence (e-mail: scrsouza{at}ib.usp.br)
Accepted 2 March 2006
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O2) and
partitioning between aquatic
(wO2) and aerial
O2 uptake
(aO2) were
measured on tadpoles and froglets by closed system respirometry, using water
of PO2 ranging from 145 to 40 mmHg. Correlative
changes in body glycogen and lactate were examined by standard enzyme assays.
Scaling patterns in the growth and degrowth stages were analysed on
whole-body, log-transformed data using linear regressions. In normoxia,
O2 was
2.1–2.5 µmol g–1 h–1 in the early
larvae, increasing more than twofold on forelimb emergence and decreasing
sharply in the froglets;
O2 varies in
strict proportion to body mass (Mb), both in the growth
(b=1.02) and degrowth (b=0.97) phases, according to the
equation
O2=aMbb,
where b is the scaling coefficient.
wO2 constitutes
>90% of total uptake in the growth stages, increasing with b=1.02
while aO2
increases with b=1.13; during degrowth there is a change in the
pattern related to intensification of metamorphosis. Hypoxic water did not
affect O2;
however, in all larval stages
wO2 and
aO2 changed with
a decrease in PO2. At 60 mmHg, rates are more
severely affected in the largest tadpoles, causing the b values for
wO2 and
aO2 to change to
0.11 and 1.44, respectively, in the growth phase. Glycogen and lactate levels
increase out of proportion with body mass increase (b=2.05 and 1.47,
respectively) in the growth stages, and increase anaerobic capacity in late
metamorphosis. In hypoxic water, glycogen levels decrease in the growth stages
and the largest tadpoles accumulate surplus lactate, possibly related to
surfacing activity. Our results may reveal the consequences of size on energy
demand at the tissue level in P. paradoxus larvae, indicating that
air breathing must subsidise energy expenditure during larval development.
Key words: metabolic rate, oxygen uptake, metamorphosis, scaling, hypoxia, glycogen, lactate, Amphibia, anuran, Pseudis paradoxus
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;
Ultsch, 1976). Amphibians
spend a large part of their daily cycle at rest, and many of their routine
behaviours seem to use only a fraction of their aerobic capacity
(Gatten, Jr et al., 1992). The
scaling of resting metabolic rates
(O2) with body
mass Mb in intra-specific comparisons with adult
individuals, described by the allometric equation
O2=aMbb,
has not disclosed any particular tendency towards a 2/3 exponent, and scaling
coefficient values (b) on average express an intermediate proportion
in the surface area:body mass relationship
(Withers, 1992). However,
surface limitation may be significant and may restrain metabolic capacity to
grow and sustain activity, particularly in those species that rely heavily on
cutaneous gas exchange and during larval life stages.
The issue is of interest owing to the recent elucidation of processes
contributing to metabolic rate in organisms, and of how body size exerts its
influence on energy expenditure at the whole-body level
(Hochachka et al., 2003;
Darveau et al., 2002;
Hulbert and Else, 2000;
Rolfe and Brown, 1997). It has
become clear that, as organisms increase in size, they adjust their structure
and function at all levels of organization, from the external surface for
O2 transfer to the composition of cell membranes and protein
function, each with their own characteristic scaling coefficient and control
contribution, which in turn, depend on metabolic state. These ideas have been
largely developed from inter-specific comparisons of adult organisms, under
low and high activity levels; in the ontogenetic context, energy utilization
for growth and organogenesis may have a great influence on overall metabolic
scaling according to the developmental stage. In the few mammals and fishes
examined, metabolic rates change in direct proportion to mass during the early
stages (the period of greatest growth), bringing the mass exponent to close to
1.0; thereafter, rates tend to follow the surface rule with the two
regressions intersecting after a given proportion of adult body mass is
reached (reviewed by Hulbert and Else,
2000; Wieser,
1995; Wieser,
1984).
Interestingly, unlike the situation in mammal and fish species, there
appears to be no clear shift in the scaling pattern during the transition from
larval to adult life stages in anuran amphibians, the exponent varying from
0.65 to 0.88 (Gatten, Jr et al.,
1992; Feder,
1982), which suggests possible surface limitations to the increase
in cutaneous O2 transfer in direct proportion to body mass during
early development. In addition, experimental data with anuran larvae suggest
that the larger the larvae, the greater the contribution of air breathing to
the responses to severe aquatic hypoxia. The requirement of air breathing to
meet metabolic demands in developing tadpoles has long been controversial;
while cutaneous respiration provides 60% or more of overall oxygen uptake in
anuran larvae, air breathing does not seem to be essential for growth and
activity in their natural settings
(Burggren and Just, 1992;
Feder, 1984). However, since
post-metamorphic growth is usually responsible for 80% or more of body size in
anuran amphibians (Werner,
1986), it is plausible that growth processes may not influence
energy cost at the whole-body level during the larval phase in the species
examined, which might explain the apparent discrepancy in the scaling
patterns. In the present study, this hypothesis was examined in the frog
Pseudis paradoxus. The development of P. paradoxus is
unusual in several respects, such as the large larval size and small gain in
body mass after metamorphosis, leading to a large contrast in the maximum size
of the tadpole compared to the adult frog
(Emerson, 1988). Giantism in
P. paradoxus larvae may thus represent the anticipation of
post-metamorphic growth during the early stages of the life cycle, the
adaptive value of which is unknown.
P. paradoxus frogs are exclusively neotropical; in southern Brazil, newly hatched larvae are most abundant in late spring and become scarce by mid-summer, most tadpoles having metamorphosed by the early fall (S.C.R.d.S., unpublished observations). The large size at metamorphosis is attained during a relatively short period, implying use of a large fraction of the energy derived from aerobic sources to support growth processes in larval P. paradoxus. Further, O2 uptake might be severely affected in the largest tadpoles under hypoxic conditions, as is usual in the natural habitat. The present study is concerned with the question of how O2 uptake may be reconciled to growth and developmental changes in P. paradoxus tadpoles. We examined the relationship between body mass and aquatic and aerial O2 uptake in the growth and degrowth phases of the larval cycle, and the effects of aquatic hypoxia on the scaling patterns. In addition, we analysed correlative shifts in the levels of body glycogen and lactate as an indication of supplementary energy production from anaerobic sources. Our findings generally indicate that the scaling of metabolism in P. paradoxus may express the consequences of size on energy demand at the tissue level, suggesting that air breathing must subsidise energy expenditure in the largest individuals, and sustain the increase in metabolism during late metamorphosis.
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Experimental groups
Developmental stage was classified according to Cais after Gosner
(Cais, 1982;
Gosner, 1960). First stage
larvae were very vulnerable to handling and transportation and were not
included in the hypoxia experiments; partial data for larval stages
29–32 (body mass=3.7±1.2 g, mean ± s.d.) in normoxic water
are given in the Results. The individual data obtained for larvae from the
subsequent stages were combined into five developmental groups: the first
consisted of stages 33–37 (8.1±4.5 g), all larvae showing
inflated lungs; the second group consisted of stages 38–42
(17.0±7.3 g), the larvae showing well vascularized lungs, and stage 42
being marked by the emergence of the forelimbs; the fourth included stages
43–44 (14.8±8.2 g), and the fifth stage 45 alone (10.0±2.6
g); both these groups exhibit the most notable anatomical changes that
constitute the shape of the adult frog while maintaining a tail of
considerable proportions; the sixth group included stage 46 (7.1±2.4
g), corresponding to froglets up to 20 days of complete metamorphosis.
According to our observations, surfacing behaviour begins at low frequencies
during the early larval stages, and more regularly in tadpoles at stages
38–42; in the latest stages, the tadpoles remain for long periods at the
air–water interface, while froglets alternate periods of partial
emersion with prolonged submersion.
Measurement of the aquatic and aerial oxygen uptake
Aquatic and aerial oxygen uptake,
wO2 and
aO2,
respectively, were measured by closed system respirometry at 25±1°C
(room temperature) on single larvae, each animal being used only once. The
metabolic chambers consisted of an acrylic tube with a 10 mm thick wall, and
of variable length and diameter. Previous measurements showed that P.
paradoxus tadpoles become restless when held with the body lying flat
inside a horizontal chamber. The tube was then vertically oriented with the
bottom end closed, and a funnel-like lid that fit over the top end over a
layer of compressible rubber. For the experiments, the chamber was screwed
shut and filled with water leaving a volume of air close to the funnel stem,
and the volumes were adjusted according to the size and stage of the tadpole.
During measurements, the water was exchanged via outlet and inlet valves, and
the samples were withdrawn through a small aperture located at a medium height
in the water column, sealed by a silicone septum (Alltech Associates, Inc.,
Deerfield, Illinois, USA). The air phase communicated with ambient air
via a valve attached to the funnel stem, and air samples were
withdrawn via a silicone septum fitted into the valve aperture.
The experiments were conducted on consecutive runs from 08:00 h to 19:00 h. Preliminary measurements were made in nearly constant, normoxic conditions, to check for any sizeable variability related to experimental procedures. The rates were then measured under acute exposure to incremental levels of aquatic hypoxia while the animals had free access to the air volume. The system was opened at 60–90 min intervals and the water carefully exchanged by the inflow of clean, sterilized water at near-neutral pH from a reservoir. The water in the reservoir was constantly mixed by a flow of air or N2 such that the resulting water PO2 was 146, 114, 88, 60, 40 mmHg, the levels representing the global mean of the initial PO2 values in each run. Further, the air at the top of the chamber was refreshed and O2 content set to normoxic levels for each subsequent experimental run. The animals were acclimated to the chamber for at least 12 h prior to measurements with a constant flow of aerated water, and the valve to the air phase open to avoid hypoxia. After closing the system, the water PO2 was allowed to decline with the animal breathing to a limit that nearly matched the initial PO2 value in the next run, and O2 content in the air phase was allowed to decline to a limit of 60% below normoxic in each run.
wO2 and
aO2 were
measured in triplicate samples of 1 ml and 50 µl, respectively, taken with
gas-tight syringes. The air in the gas phase was gently mixed with the syringe
before sampling, and the water was mixed for a few seconds with a small,
magnetic stirring bar at slow speed, and sampled. O2 concentration
in the air samples were measured using the zirconium sensor of an Oxycon
device (Cameron Instrument Co., Port Aransas, Texas, USA), and
PO2 in the water samples was measured using a
Clark-type electrode held inside a thermo-stable chamber at 25°C, the
signal being converted in a gas analyser (Cameron Instrument Co.). The
equipment was calibrated in the early morning and checked for stability during
the experiments. During measurements, the animals were shielded by an opaque
screen to minimize visual disturbance; the stage 33–42 tadpoles remained
mostly quiescent, with the snout upwards and the tail hanging downwards into
the water column, while the last stage tadpoles and froglets alternated
periods near the water surface with variable periods of submersion to the
bottom. In all cases, energy expenditure during the measurements was assumed
to be an approximation of resting levels, with 
O2 values
varying according to the tadpole size and degree of aquatic hypoxia.
Micromolar O2 concentrations were calculated from the O2
tension and the coefficients for distilled water at 25°C, and the total
O2 consumption rates
(O2) were
calculated from the
wO2 and
aO2.
The same protocol was used in control experiments with no animals in the
chambers, allowing adjustment for diffusive changes according to chamber size
and degree of aquatic hypoxia. Oxygen changes in the air and in the water
phase were measured at 60–90 min intervals under incremental levels of
aquatic hypoxia as above; the values obtained were then subtracted from, or
added to, the experimental O2 consumption rates accordingly,
averaging 0.9–6.1% of the
aO2 and
0.1–1.1% of the
wO2 values.
Measurement of body glycogen and lactate levels
Total glycogen and lactate contents were measured in larvae at distinct
developmental stages in normoxic water (mean
PO2=149 mmHg) or after acute, 3 h exposure to
hypoxic water (60 mmHg), during which the animals had free access to normoxic
air in the upper phase. Groups of animals were maintained in 60 l tanks
containing clean, sterilized water at near-neutral pH and a support made of
inert material that allowed access by late metamorphic stage individuals to
the surface without increased effort. The animals were killed by pithing and
quickly immersed in liquid N2, then stored at –85°C until
analysis.
The frozen larvae were powdered in liquid N2 and homogenised
with ice-cold, 0.6 mol l–1 perchloric acid (PCA) using a
blender. After complete deproteinization, glycogen and L-lactate
concentrations were estimated according to standard enzymatic procedures
(Bergmeyer, 1984) by following
the oxidation rate of NAD+ in a spectrophotometer Spectra Max 250
(Molecular Devices, Sunnyvale, CA, USA) at 340 nm and 25°C. The final
result was expressed as µmol glycosyl units or L-lactate per
unit body mass.
Statistical analysis
Visual inspection suggested the effects of
PO2 on
wO2 and
aO2 per unit
mass to be non-linear in some of the experimental groups. Without a
theoretical model, however, the outcome of the analysis using a different
function would be equally arbitrary, and hence, for the purpose of this study,
the correlation coefficient `r' was used as a reliable measure of the
degree of association between the variables. The data were log-transformed for
calculation of the coefficient given the indication of deviation from
bivariate normality. The percentage of variance of the whole-body
O2,
wO2,
aO2, and
metabolites attributable to body mass and to developmental stage were
estimated by analysis of covariance (ANCOVA), using the data obtained in
normoxic and hypoxic water. The relationships between whole-body
O2,
wO2 or
aO2 and body
mass were analysed at two selected water PO2
levels (146 and 60 mmHg) on log-transformed data, using the least-squares,
linear regression method. The growth and degrowth phases of the larval period
were considered as criteria of biological significance in the calculation of
two regression lines and equations, one consisting of the developmental stages
33–42, and the other of stages 43–46, and the regression
coefficient r2 was used as a measure of functional
dependence of O2 uptake rates with respect to body mass. The effect
of hypoxic water on glycogen and lactate per unit mass was tested against
normoxic water and as a function of developmental stage by two-way analysis of
variance (ANOVA). The scaling relationships of the metabolite concentrations
were analysed using the least-squares, linear regression method on
log-transformed, whole-body data as above. The analyses were performed
according to Zar (Zar, 1999),
using SigmaStat (Jandel Scientific Co., San Rafael, CA, USA) and MiniTab
(MiniTab Inc., State College, PA, USA) statistical software. The test results
and probability of error are given in the text or in the tabulated results,
differences being considered significant at P
0.05.
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O2/Mb)
of tadpoles and froglets measured in consecutive experimental runs under
normoxic conditions. It was thus assumed that the experimental procedure and
its total duration did not contribute significant variation to the data. In
normoxic water,
O2/Mb
measured 2.1–2.5 µmol g–1 h–1 in
stage 29–42 larvae, increasing to 3.9 µmol g–1
h–1 in stages 43–44 larvae, and peaking at 5.7 µmol
g–1 h–1 in stage 45 larvae
(Fig. 1).
O2/Mb
values decreased sharply on metamorphosis, and those of the froglets were
similar to the early larval stages. Acute exposure to water of reduced
PO2 caused no significant change in
O2/Mb
within the PO2 range analysed, most variability
being attributable to developmental stage (F=48.2,
P<0.0001).
Under normoxic conditions, the stage 33–37 tadpoles acquire 96% of
O2 consumed from the water, with a minor contribution from aerial
exchange (Table 1;
Fig. 2). This value is
unchanged in the subsequent stages until the emergence of the forelimbs in
stage 42, when gill respiration becomes impaired. Thereafter, the contribution
by aerial uptake increases sharply, reaching 73% in stage 45 larvae and in
froglets. Partitioning between aquatic and aerial O2 uptake was
altered on exposure to aquatic hypoxia in all groups of stages examined
(Table 1;
Fig. 2). In stage 33–37
larvae
wO2/Mb
decreased with PO2 decrease (r=0.73;
P<0.0001), this effect being accompanied by an increase in
aO2/Mb
(r=0.80; P<0.0001) that accounts for 74% of O2
consumed under the most severe hypoxia. Similarly, in larval stage
37–42, there was a positive correlation between
wO2/Mb
and the degree of aquatic hypoxia (r=0.68; P<0.0001),
aO2/Mb
showing an inverse correlation (r=0.61; P<0.0001) and
accounting for 77% of O2 consumed at the lowest
PO2 level. The
wO2/Mb
and
aO2/Mb
correlation lines cross over at approximately 60 mmHg, when the contributions
of aquatic and aerial uptakes are nearly equivalent. Significant decreases in
wO2/Mb
with decrease in water PO2 were also observed
in stage 43–44 larvae (r=0.64; P<0.0001) and in
stage 45 larvae (r=0.40; P<0.0172), the rates reaching
less than 10% of O2 consumed under the most severe hypoxia, with an
inverse correlation for
aO2/Mb
in both groups (r=0.43 and 0.44; P<0.0024 and 0.0082). In
the froglets, there was no significant change in
wO2/Mb
as a function of decreasing O2 level in the water even though a
small increase in lung ventilation was detected (r=0.37;
P=0.0234).
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Influence of body mass on whole-body, O2 consumption rates and partitioning, in normoxic and hypoxic water
In normoxic water (PO2=146 mmHg), body mass
accounts for 87% of the overall variability in
O2 of P.
paradoxus larvae and froglets (ANCOVA; F=35.8;
P=0.0001); significantly, developmental changes in the gas exchange
organs account for 14% (F=4.4; P=0.001). This reflects the
strong dependence of
wO2 on body mass
Mb (F=38.0; P=0.0001), with a lesser
effect of developmental changes (F=3.4; P=0.004). The
aO2 is
predominantly influenced by developmental stage (F=90.8;
P=0.0001), and varies significantly as a function of larval size
(F=14.6; P=0.0001) (Table
2; Fig. 3).
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Separate analysis of the growth and degrowth phases revealed that the slope
for the relationship between
O2 and body mass
is b=1.02 and 0.97, respectively
(Table 2;
Fig. 3), implying that
O2 uptake first increases proportionally to body mass increase
(r2=0.77; P<0.0001), then decreases in
proportion to mass reduction during larval development
(r2=0.61; P<0.0001).
wO2 similarly
increases in strict proportion to the increase in body mass during growth
stages, with b=1.02 (r2=0.76;
P<0.0001), and although representing only a small fraction of the
total O2 uptake,
aO2 increases
out of proportion to body mass increase, with b=1.13
(r2=0.67; P<0.0001). During degrowth stages,
while the decrease in the
wO2 with body
mass decrease is disproportionate, with b=1.18
(r2=0.75; P=0.0001),
aO2 increases
with b=0.77 (r2=0.45; P=0.0002),
implying an increasingly higher capacity for O2 uptake by the lungs
during the late metamorphic stages.
In hypoxic water (PO2=60 mmHg), body mass
similarly explains most of the variability (87%) in the
O2 of tadpoles
and froglets (ANCOVA; F=37.3; P<0.0001). However, the
influence of body mass on the
wO2 is less
pronounced (F=4.38; P=0.045), while the mass dependence of
aO2 is greatly
increased (F=17.7; P=0.0001), with 65% of the variability in
aO2 attributable
to body mass compared to 14% in normoxic water. According to the regression
analysis, the slope for
O2 in hypoxic
water declined to b=0.83 over the growth stages
(r2=0.69; P<0.0001), implying a variable
effect of hypoxia on O2 uptake as a function of larval size, larger
larvae being more affected than smaller ones
(Table 2;
Fig. 3). Accordingly, the
depression in aquatic O2 uptake is notably large in the larger
tadpoles, causing the slope for
wO2 with body
mass to approach zero (b=0.11), and associated with an increase in
aO2 out of
proportion to body mass, with b=1.44 (r2=0.57;
P=0.0023). During the degrowth stages, there is a change in the slope
for the relationship between
wO2 and
aO2 with body
mass to b=0.75 (r2=0.127; P=0.087) and
0.99 (r2=0.61; P<0.0001), respectively,
suggesting that the effects of aquatic hypoxia are more severe in the large
tadpoles than in froglets.
Glycogen and lactate contents
In normoxia (PO2=149 mmHg), glycogen and
lactate concentrations per unit mass change remarkably with developmental
stage (Fig. 4). Glycogen
represents 2.33± 0.51 glycosyl units g–1 body mass
(mean ± s.e.m.) in stage 33–37 larvae, increasing sixfold in
stages 38–42 (15.32±4.41), and almost tenfold in stages
43–45 (22.32±7.53), a sharp decrease following in the newly
metamorphosed froglets (4.48±0.75). Lactate measures 2.28± 0.26
µmol lactate g–1 body mass (mean ± s.e.m.) in stage
33–37 larvae and is similar during stages 38–42, then increases
sharply twofold (4.48±1.7) and threefold (7.63±0.64) in the late
metamorphic stages, remaining similarly elevated in the young froglets
(Fig. 4).
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The 3 h exposure to aquatic hypoxia (PO2=60 mm Hg) with access to normoxic air showed an interaction effect with developmental stage on glycogen concentration per unit mass (ANOVA; F=2.99; P=0.028); however, a large, interindividual variability is associated with this response (Fig. 4). Multiple comparisons among mean values revealed a significant decrease of 66% during larval stages 38–42 compared to values in normoxic water, a similar tendency being seen in stages 43–44. Hypoxia exposure may differentially affect the whole-body glycogen content of growing larvae according to body size, the slope for the regression being less steep than in normoxic conditions, suggesting that large tadpoles are more severely affected than smaller ones. However, the coefficient r2=0.147 does not predict functional dependence between the variables, and the small sample size and mass range in this group prevent a solid conclusion. The regression for the degrowth phase is likewise less steep after hypoxia exposure (r2=0.52; P=0.002), and in this case, the calculated equation predicts a 50% reduction in body glycogen in 20 g larvae, and no change in 5 g animals, typically froglets.
Hypoxia exposure caused no significant change in lactate content per unit mass compared to normoxic values (Fig. 4). However, the large change in the mass exponent for the whole-body content, to b=2.04 (r2=0.46; P=0.021), suggests that larger tadpoles accumulate surplus lactate in hypoxic water (Table 3). According to the calculated equations, body lactate content would increase by 84% in 20 g larvae relative to normoxic levels. In the degrowth stages, hypoxia exposure caused a decline in slope to b=0.79 (r2=0.64; P=0.0001), and the equations indicate that under these conditions 20 g larvae contain 36% less lactate compared to normoxic levels, while the contents would be similar in 5 g froglets.
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Metabolic rate and the costs of growth and metamorphosis
The mass-specific O2 consumption rates of larval P.
paradoxus are fairly constant and low in the early larvae until the
emergence of the forelimbs, values lying within the ranges reported for other
frogs, despite large inter-specific differences in the degree of size
variation during the larval period and in the adult mode of life
(Gatten Jr et al., 1992). This
phase constitutes more than three quarters of the larval period in P.
paradoxus, lasting for 120 days under laboratory conditions
(Cais, 1982) and possibly less
in the natural environment, during which the larvae undergo minor
developmental changes and body size increases; in the present study, the
minimum and maximum weights at capture were 0.1 g (stage 26) and 72 g (stage
40), respectively. By contrast, Rana catesbeiana tadpoles can grow at
very slow rates to a large size by increasing the developmental time during
one or two overwintering cycles, as seen under temperature conditions that
lead to interruption of metamorphosis
(Emerson, 1988). Overall, then,
the great size quickly attained by P. paradoxus tadpoles may result
from higher rates of whole body protein accretion.
The tail represents 78% of body length in the largest tadpoles of P.
paradoxus (stages 38–42), and its wet muscle mass increases
exponentially (1.19) with body mass in the absence of significant changes in
dry:wet tissue mass ratio (C.M.K. and S.C.R.d.S., unpublished data). Using
available data on developmental time (Cais,
1982) and a tail muscle protein content of 10 mg% obtained from
our samples, a rough calculation gives 1.4 mg day–1 for the
rate of tail muscle protein synthesis in tadpoles growing at 1% per day. The
fraction of O2
expended on this process would be between 19 and 42%, employing a minimum cost
of peptide bond formation of between 7 and 16 mmol O2
g–1 of protein (Houlihan,
1991). While representing a smaller fraction of the body mass,
other sites of protein synthesis to be considered in the growing larvae are
the liver and the gastrointestinal tract, as protein turnover by these tissues
reaches very high rates compared to white muscle
(Houlihan, 1991). Further,
tadpoles are typically herbivores, exhibiting elevated rates of intestinal
nutrient transport to extract the amino acids required for growth from large
quantities of plant matter (Toloza and
Diamond, 1990). The costs of growth would then include the energy
expended on eating, digesting and absorbing food in excess of that needed for
maintenance, which amounts to 60–80% of metabolic rate in young toads,
Bufo bufo (Jørgensen,
1988) and may represent a large fraction of the routine rates of
metabolism in P. paradoxus tadpoles.
Oxygen consumption increases sharply in P. paradoxus tadpoles on
emergence of the forelimbs concomitant with the abolishment of gill
respiration and food intake, and may remain elevated until completion of
metamorphosis over a period of approximately 10 days
(Cais, 1982). Compositional
changes during the advanced stages of metamorphosis, such as those in water
content and in the relative size of internal organs, may partially explain
this increase in metabolic rate. The dry:wet muscle tissue ratio increases
slightly, both in the degenerating tail and in the growing leg of P.
paradoxus tadpoles. In addition, there is a 19-fold increase in liver
tissue mass from the early to the latest larval stages (C.M.K. and S.C.R.d.S.,
unpublished data), associated to an increase in the liver somatic tissue index
from 0.5 to 2% of body mass, implying that the biosynthetic capacity of this
organ relative to body mass would increase in late metamorphosis. The heart
size decreases with decreasing body size according to b=0.72, the net
effect being a 1.7-fold increase in relative organ mass in later stage larvae
(C.M.K. and S.C.R.d.S., unpublished data), and together these changes may
increase O2 consumption by an increase in the relative mass of
metabolically active tissue. Accordingly, studies focusing on phenotypic
plasticity and physiological adaptation have shown that the relative size of
the heart, liver and kidney may explain much of the inter-individual and
inter-specific variability seen in O2 demand at the whole-body
level (Selman et al., 2001;
Williams and Tieleman,
2000).
Despite the extensive tissue reorganization, however, O2
consumption decreases on completion of metamorphosis in P. paradoxus,
and the mechanisms promoting the sharp increase in energy expenditure in the
tadpoles, prior to metamorphosis, remain unknown. The late metamorphic events
in anurans are marked by tail reabsorption, when more than half of the body
weight is lost; the energy requirements of caudal proteolysis may be
substantial in P. paradoxus tadpoles, given the large relative mass
of muscle tissue that is degraded in a matter of a few days. Increases in the
rates of anabolic processes underlying the extensive tissue reorganization,
such as in the gastrointestinal tract, may also contribute significantly to
the increase in metabolic rates at the whole body level
(Hourdry et al., 1996).
Besides, the amino acids resulting from tail resorption provide the animal
with a continuous source of carbohydrate via the gluconeogenic
pathway; recently we have found increased enzyme activity related to
gluconeogenesis in the liver of tadpoles during late metamorphosis (F. M.
Oshiro, S. C. R. de Souza, J. E. P. W. Bicudo and M. S. C. Bianconcini,
unpublished observations). In mammals, nearly one-quarter of body
O2 use takes place in the liver and gastrointestinal tract under
standard conditions (Rolfe and Brown,
1997); assuming a similar proportion in the organs of P.
paradoxus tadpoles, a fourfold increase in the rates of liver and
gastrointestinal tissue respiration would be necessary to fully account for
the twofold increase in O2 consumption rates at the whole-body
level during late metamorphosis.
Developmental changes in O2 consumption of frogs do not share a
common pattern, and the available data are far from exhaustive
(Burggren and Just, 1992). A
study with Xenopus laevis illustrates the contrasts with P.
paradoxus tadpoles, showing a peak in
O2 per unit mass
on hatching, and another in newly metamorphosed frogs, while in the more
advanced larval stages, rates decline slightly due to a presumed decrease in
energy expenditure linked with cessation of gill respiration
(Hastings and Burggren, 1995).
The significance of the distinct metabolic patterns seen during the
metamorphic transition of anurans is difficult to interpret based on the
information available, and species-specific characteristics may also be
involved, together with plasticity of morphological and physiological
characters in response to the environment.
Partitioning of O2 uptake and the effects of the larval size
In normoxic water, the early larvae of P. paradoxus rely almost
exclusively on aquatic O2 exchange to maintain routine metabolism,
as do other anuran larvae studied (Feder,
1984). On emergence of the forelimbs, the contribution of aerial
breathing increases sharply together with an equivalent decrease in aquatic
O2 uptake. Under aquatic hypoxia, gill ventilation is apparently
inhibited and lung breathing stimulated at PO2
values around 90 mmHg and lower,
O2 per unit mass
in the developmental groups remaining nearly constant over the
PO2 range analysed. Previous data from Rana
catesbeiana reveal a remarkable capability of the larvae to counteract
the effects of aquatic hypoxia by increasing gill ventilation during forced
submersion in water of decreasing PO2, with
effective O2 regulation occurring down to a critical
PO2 of around 30 mmHg
(Crowder et al., 1998). This
pattern may differ among ranid frogs, as suggested by the study with R.
berlandieri, showing a marked decrease in total O2 uptake
during submersion in low PO2 water and
insufficient capacity to offset the effects of aquatic hypoxia by air
breathing (Feder, 1983).
Despite the influences of phylogeny per se, and the more obvious
differences in methodological approach, there is evidence of dissimilarities
in the ability of anuran larvae to compensate for environmental O2
fluctuations by gill ventilation. In P. paradoxus tadpoles,
adjustments in gill and lung ventilation are apparent in water
PO2 levels at which gas exchange across the
integument is presumably effective, and may indicate early reliance on aerial
O2 uptake associated with the large larval size on transformation.
Hypoxia exposure affects growth rates in many ways, as shown by reductions in
feeding rate, respiration rate, faecal production and protein synthesis
(Zhou et al., 2001). In the
habitat where P. paradoxus tadpoles are found, O2 supply
is neither homogeneous nor stable, circumstances in which air breathing may be
favoured.
Body mass in P. paradoxus tadpoles covaries with the effects of
developmental stage on whole-body O2 uptake, and accounts for some
90% of the variability under normoxic conditions, similar to observations on
other anuran larvae (Feder,
1982). However, the scaling patterns seen in P. paradoxus
are distinct, and reveal a general tendency for O2 uptake to
increase in direct or more than direct proportion to mass, as in the early
ontogenetic stages of mammal and fish species
(Hulbert and Else, 2000;
Wieser, 1995). The gas
exchange organs of mammals and fishes presumably increase their efficacy with
growth and development, while in metamorphosing amphibians, growth coincides
at some point with gill degeneration. Despite this, and the inherent
limitation of the skin for gas exchange, aquatic O2 uptake
increases in direct proportion to the increase in mass in P.
paradoxus tadpoles, and the relationship nearly overlaps the
corresponding curve for total O2 uptake under resting conditions.
Since this pattern does not prevent the developing animal from increasing
metabolism with activity changes and metabolic state, some reserve capacity
may be available at the O2 transfer step. One consequence of this
pattern, however, may be that air breathing must subsidise any further
increase in energy expenditure in the largest individuals, as the scaling for
aerial O2 uptake in normoxia appears to indicate (b=1.13).
Under hypoxia, the depression in cutaneous O2 uptake is notably
large in the larger tadpoles, causing the slope of the aquatic O2
uptake in the growth stages to change from 1.02 to almost zero
(b=0.11), and they may depend disproportionately on air breathing to
maintain O2 consumption rates, as the slope of the aerial uptake
indicates (b=1.44).
During the degrowth stages of late metamorphosis, the scaling relationships
for aquatic O2 uptake imply that the mass-specific rates of aquatic
O2 uptake are twice as great in the latest larval stages than in
froglets (b=1.18). P. paradoxus larvae not only have
unusually shaped tails, with the keel extending further onto the head compared
to tadpoles of R. catesbeiana of similar size, but tail reabsorption
takes longer than in other frogs (Emerson,
1988). In the present study, tail length corresponds to 63% of
total body length in stages 43–45, the oldest larvae resembling adult
frogs with a larval tail hanging in the water column. Since its size and
surface area actually increase relative to body mass during these stages of
body mass reduction, the tail appears to function as an important site of
O2 transfer until completion of metamorphosis. In water of low
O2 content, however, cutaneous O2 uptake becomes
limiting and late-stage larvae may increase lung ventilation more than newly
metamorphosed frogs to sustain their much higher metabolic rate, as suggested
by the change in the mass exponent for aerial O2 uptake
(b=0.77) in normoxia to close to unity under hypoxia.
Other functions have been attributed to surfacing behaviour in developing
tadpoles, such as prevention of lung collapse during organ development in the
early larval stages (Burggren and West,
1982; Bruce et al.,
1994; Crowder et al.,
1998). The emergence of central chemoreceptive reflexes regulating
O2 and CO2 by lung ventilation precedes the
disappearance of central gill respiratory regulation in R.
catesbeiana, and as development advances, the central lung pattern
generator gradually becomes more functional, dominating in the late
metamorphic stages (Torgenson et al., 1997). In P. paradoxus, there
is a disproportionate increase in the aerial O2 uptake to size
increase during larval growth stages, and a sharp increase in air breathing
rates on forelimb emergence, reaching 20-fold in 30 g larvae, according to the
calculated equation. Some plasticity in the ontogeny of respiratory control
may have developed in P. paradoxus tadpoles, associated with their
large size at metamorphosis. Other physiological and biochemical adjustments
may also contribute to providing adequate O2 transfer and delivery
to the body tissues. Burggren et al.
(Burggren et al., 1992)
described changes in blood pressure variables in P. paradoxus of
dramatic speed and magnitude, causing a threefold increase in mean, systemic,
arterial blood pressure in late-stage larvae compared to younger larvae. This
may be explained in part by the developmental changes in the relative heart
mass, described above, and thus scaling effects on adjustments by the
cardiovascular system may promote increased blood perfusion and contribute to
an increase in the O2 uptake and delivery steps to the body tissues
in the later stages of P. paradoxus metamorphosis.
Metabolic implications of changes in glycogen and lactate levels
Body glycogen content rises in P. paradoxus larvae from stages 38
to 42, and remains high over the period of late metamorphosis, dropping in
newly metamorphosed froglets. Lactate content increases sharply after
emergence of the forelimbs and remains high after metamorphosis. Together,
these changes express increased anaerobic potential and power generation for
burst activity in the late larval stages. Given that food intake is
interrupted during late metamorphosis in P. paradoxus, the high,
sustained glycogen content suggests that an endogenous substrate is required
for carbohydrate synthesis during the fasting period, possibly amino acids
resulting from protein catabolism in the tail, in agreement with our recent
findings of increased enzyme activity related to gluconeogenesis in the larvae
of late stages (F. M. Oshiro, S. C. R. de Souza., J. E. P. W. Bicudo and M. S.
C. Bianconcini, unpublished observations).
The lack of significant changes in lactate concentration per unit mass
after 3 h of aquatic hypoxia is not unexpected, given the ability of P.
paradoxus tadpoles to maintain aerobic, resting metabolic rates by
increasing lung ventilation. Lactate does not build up in other anuran larvae,
except after prolonged exposure to severe hypoxia
(PO2<10 mmHg)
(Crowder et al., 1998), or on
exertion, at rates dependent on the intensity and duration of exercise
(Gatten, Jr, 1985;
Quinn and Burggren, 1983). In
this context, however, the significant decrease in body glycogen in P.
paradoxus larvae in stages 37–42 exposed to hypoxic water appears
paradoxical. One explanation is that carbohydrate stores may be mobilised and
used to fuel oxidative processes, due to the higher energy yield per
O2 molecule from glucose
(Hochachka and Somero, 2002);
this mechanism is apparently essential to the development of hypoxia tolerance
in animals (Hochachka et al.,
1996; West and Boutilier,
1998). An alternative interpretation comes from the suggestion
that whole-body glycogen and lactate in larval P. paradoxus are
markedly affected by body size. In the growing larvae, the calculated
equations predict a large increase in lactate and glycogen levels of 2.8 and
4.1-fold, respectively, for a twofold increase in body size, similar to the
pattern observed in teleost fish (Somero
and Childress, 1980). After hypoxia exposure, there is a tendency
for body glycogen to decrease more in the larger larvae, and a clear
suggestion of a change in the mass exponent for lactate, implying that larger
tadpoles produced surplus lactate after exposure to hypoxic water, calculated
to be 1.8-fold of lactate in 20 g larvae compared to normoxic conditions. In
the stages of larval growth, the tadpoles ascend periodically in the water
column to ventilate their lungs, and apparently increase the frequency of
ascending during hypoxic exposure. This behaviour tends to disappear during
late metamorphosis, and the greater reliance on air breathing of the largest
tadpoles might explain the differential production of lactate as a function of
size in P. paradoxus.
In conclusion, multiple adjustments at the O2 transfer step during the early development of P. paradoxus correlate with body mass changes resulting from the growth processes, similar to observations of metabolic scaling on fishes and mammals. Developmental programs operating through changes in organs and body parts may ultimately effect adjustments in the metabolic capacities of tissues and related systems, so that O2 transfer and energy expenditure may be reconciled with the large larval size and metamorphosis.
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References |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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6 animals, staged according to Cais
after Gosner (Cais, 1982