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First published online August 17, 2007
Journal of Experimental Biology 210, 2999-3014 (2007)
Published by The Company of Biologists 2007
doi: 10.1242/jeb.006007
Temperature adaptation in two bivalve species from different thermal habitats: energetics and remodelling of membrane lipids
1 Institut de Recherche sur les Zones Côtières, 232B rue de
l'Église, Shippagan, Nouveau-Brunswick, E8S 1J2, Canada
2 Institut des Sciences de la Mer, 310 allée des Ursulines, Rimouski,
Québec, G5L 3A1, Canada
3 Department of Fisheries and Oceans, Science Branch, Gulf Fisheries Centre,
PO Box 5030, Moncton, New Brunswick, E1C 9B6, Canada
4 Département de Biologie, Université Laval, Québec,
Québec, G1K 7P4, Canada
* Author for correspondence (e-mail: fpernet{at}umcs.ca)
Accepted 18 June 2007
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Summary |
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We found major differences between species in triglyceride (TAG) metabolism during overwintering. Mussels used digestive gland TAG stores for energy metabolism or reproductive processes during the winter, whereas oysters did not accumulate large TAG stores prior to overwintering. Mussel TAG contained high levels of 20:5n-3 compared to levels in oysters and in the diet. This may help to counteract the effect of low temperature by reducing the melting point of TAG and thus increasing the availability of storage fats at low temperature. Mussels seemed better able to mobilise 20:5n-3 and 18:4n-3 than other fatty acids.
We also found that both bivalves underwent a major remodelling of membrane phospholipids. The unsaturation index decreased in the gills and digestive glands of both species during the early stages of warming, principally due to decreases in 22:6n-3 and 20:5n-3. In digestive glands, the unsaturation index did not increase with decreasing temperature beyond a threshold attained at 9°C whereas a perfect negative relationship was observed in gills, as predicted by homeoviscous adaptation. The presence of digestive enzymes and acids in the digestive gland microenvironment may lead to specific requirements for membrane stability. That oysters had lower metabolic rates than mussels coincides with a lower unsaturation index of their lipids, as predicted by Hulbert's theory of membranes as metabolic pacemakers. Both species showed increased 20:4n-6 levels in their tissues as temperature rose, suggesting an increasing availability of this fatty acid for eicosanoid biosynthesis during stress responses.
The contrast between the species in TAG dynamics and the similarity of their phospholipid remodelling emphasises the essential functional role of membrane phospholipid structure and the contrasting use of TAG by oysters and mussels during overwintering.
Key words: lipid, fatty acid, triglyceride, phospholipid, homeoviscous adaptation, mollusc, temperature adaptation, acclimation
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Introduction |
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). The thermal sensitivity of membrane processes is due to the
strong effect of temperature on the physical properties of membrane lipids,
which in turn have a major influence on associated proteins. A decrease in
temperature usually reduces membrane fluidity, which can lead to membrane
dysfunction. Poikilotherms usually counteract this temperature effect by
remodelling membrane lipids, a process known as homeoviscous adaptation (HVA),
via changes in phospholipid headgroups, fatty acid composition and
cholesterol content that compensate for the effect of temperature on membrane
structure (Sinensky, 1974;
Hazel, 1995). Many intertidal
organisms, which commonly withstand variations in temperature of
20–30°C on a daily basis and encounter even wider thermal ranges on
a seasonal basis, are able to regulate membrane fluidity in response to
thermal change. For example, the mussel Mytilus californianus
exhibits strong seasonal variations in membrane fluidity that are consistent
with HVA (Williams and Somero,
1996). Similarly, membrane fluidity in gill phospholipids of the
sea scallop Placopecten magellanicus is positively correlated with
20:5n-3 and negatively correlated with acclimation temperature, presumably
helping to maintain membrane function at low temperatures
(Hall et al., 2002). Finally,
a major remodelling of lipids consistent with HVA occurs in hard clams
Mercenaria mercenaria exposed to a gradual cooling from 
24°C
to 0°C and acclimatisation at <0°C
(Pernet et al., 2006b).
Blue mussels Mytilus edulis and eastern oysters Crassostrea
virginica are two eurythermal suspension-feeding bivalves widely
distributed along the east coast of North America. M. edulis ranges
from Baffin Island to North Carolina
(Gosling, 1992;
Fisk et al., 2003), whereas
C. virginica is mainly found in the southern part of North America,
from the Gulf of St Lawrence to the Gulf of Mexico
(Galtsoff, 1964). In the Gulf
of St Lawrence, C. virginica is restricted to warm shallow bays and
estuaries whereas M. edulis is found almost everywhere. This reflects
the thermal preferences of the two species: they both tolerate a minimum
temperature of –2°C but maximal and optimal temperatures for M.
edulis are much lower (27°C and 10–20°C respectively) than
those of C. virginica (36°C and 20–30°C, respectively)
(Thompson and Newell, 1985;
Shumway, 1996). Therefore, low
overwintering temperatures have been suggested as a potential explanation for
sporadic overwintering mortalities of C. virginica in Atlantic Canada
(Lavoie, 1995), whereas
temperatures >20°C in this area coincided with summer mortality in
certain populations of M. edulis
(Myrand and Gaudreault, 1995;
Tremblay et al., 1998).
In the Gulf of St Lawrence, where mortality of C. virginica
occasionally occurs, 0°C is a typical overwintering temperature. No
mortality has been reported along the central Atlantic coasts, where 4°C
is a typical overwintering temperature. The southern Atlantic coast from
Chesapeake Bay to South Carolina, which has overwintering temperatures of
about 9°C, supports the highest annual growth rate of C.
virginica (Shumway,
1996). Oysters are quiescent at 0°C, begin to feed at 4°C,
and start to grow at 9°C (Loosanoff,
1958).
In this study, mussels and oysters from the Gulf of St Lawrence were
overwintered at 0°C, 4°C and 9°C in the laboratory for 3 months.
The temperature was gradually raised to and held at 20°C for 5 weeks to
simulate spring–summer conditions in the Gulf of St Lawrence. Animals
were regularly sampled for lipid analysis and physiological measurements. We
focussed our study on changes in lipid class and fatty acid composition of
digestive glands and gills in relation to clearance rates and oxygen
consumption. Digestive glands are the main site of extra- and intracellular
digestion; they typically store large amounts of neutral lipids. In contrast,
gills are involved in particle processing and gas exchange, and gill lipids
consist mainly of sterols and phospholipids. We predicted that (1) bivalves
would counteract thermal effects on membrane fluidity by remodelling membrane
lipids as stipulated by the HVA, (2) membrane lipids of M. edulis, a
species adapted to harsh Canadian winters, would be more unsaturated than
those of C. virginica, a species that is less tolerant to cold, and
(3) inter-specific differences in metabolic rates would be related to membrane
unsaturation, as predicted by Hulbert's theory of membranes as metabolic
pacemakers (Hulbert and Else,
1999; Hulbert and Else,
2005).
Unlike studies that only focus on the thermal effects on membrane lipids,
we also examined the dynamics of storage lipids in relation to overwintering
temperature. In marine bivalves, lipids are primarily stored as triglyceride
(TAG) droplets in digestive glands (Giese,
1966), and the synthesis, storage and use of TAG usually show
pronounced seasonal cycles: TAG are sequestered during periods of high food
availability in late summer and fall, and are subsequently used for
maintenance metabolism during periods of reduced feeding in the winter and for
the initiation of gametogenesis (De Zwaan
and Mathieu, 1992; Thompson et
al., 1996). Because TAG are not linked to membrane function, they
seem less likely than membrane lipids to change with temperature. However, TAG
can only be mobilised if they are in a fluid state
(Florant, 1998), a fact that
poikilotherms living at low temperatures must counteract if lipid mobilisation
is to continue.
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Materials and methods |
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, the natural
photoperiod was followed, and the temperature was maintained at 9°C. The
two species were maintained together in these tanks over the entire
experiment. Seawater was circulated through 1/2 or 1/5 HP external chillers
(J&L Aquatics, Burnaby, BC, Canada) to maintain the required temperature;
the water temperature in each tank was controlled separately. Animals were fed
a mixed suspension of Chaetoceros muelleri (CHGRA) and Isochrysis
galbana (TISO). These two algal species showed adequate characteristics
as food for several bivalve species and complementary profiles in essential
fatty acids (Pernet et al.,
2003). Animals were fed every 2 days at 20x103
cells ml–1 (50:50 of each algal species by cell number). When
seawater temperature was raised on the 12 April (see next section), the algal
concentration offered to mussels and oysters was increased from 20 to
50x103 cells ml–1. The daily ash-free dry
mass (AFDM) of the algal ration varied from 0.3–0.5% of the mean AFDM of
one animal during the overwintering period and increased to 2.3–3.2%
during the spring simulation period. Variation in food ration within each
experimental period was due to the successive removal of animals used for
lipid analyses. Microalgal stocks were obtained from the Centre for Culture of
Marine Phytoplankton (West Boothbay Harbor, ME, USA). Algae were
batch-cultured in 20-l carboys (Pernet et
al., 2003) and sampled three times during the experiment for fatty
acid determination (Table 1).
Temperature was monitored every hour in each tank throughout the experiment
with submersible Vemco 8-bit Minilog-TR data loggers (Shad Bay, NS,
Canada).
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Experimental design
Mussels and oysters were randomly divided between the three experimental
treatments in duplicate tanks on 17 January 2005: one group was maintained at
9°C and two groups experienced a gradual temperature decrease
(0.5°C/day), one to 4°C and one to 0°C
(Fig. 1A). Thus, all animals
reached the desired overwintering temperature by 31 January, after which these
temperatures were maintained for 12 weeks. Mussels and oysters that had
overwintered at 9°C, 4°C and 0°C were then warmed by
1°C/day starting on 19, 15 and 12 April, respectively, to simulate
spring–summer conditions. A 1°C/day increase is representative of
field conditions in the spring (Bricelj et
al., in press). When animals attained 20°C on 4 May, they were
held at this temperature for 5 weeks, until 8 June. Digestive glands and gills
were sampled on 17 January, before applying the overwintering temperatures; on
31 January, after attaining the overwintering temperature; on 14 February,
after short-term winter acclimation; on 12 April, which reflects long-term
winter acclimation; on 4 May, after attaining the summer temperature; and on 8
June, which reflects long-term summer acclimation
(Fig. 1).
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 | (1) |
Clearance rate
Clearance rate (CR) is defined as the volume of water cleared of suspended
particles per unit time and biomass
(Widdows and Johnson, 1988).
The CR was determined on 17 and 31 January, 14 February, 12 April, 4 May and 8
June for each temperature treatment. Six animals per tank of each species were
used for CR measurement (12 animals per overwintering temperature and
species). Animals were removed from their holding tank and maintained
individually in their experimental chambers in which the suspension was mixed
via gentle aeration from the bottom of the chamber. Before beginning
particle concentration measurements, animals were left undisturbed for at
least 1 h to allow their valves to open and feeding to begin. The CR was
determined using a static system in which the decrease in particle
concentration was monitored inside the chambers. At the beginning of the
incubation period, individual animals were provided TISO at an initial
concentration of 10x103 cells ml–1. Food
particles were counted every 10 min for 60 min with an electronic particle
counter (Beckman Coulter-counter Z1TM) fitted with a 100-µm aperture
tube. The greatest difference between two consecutive measurements was used to
calculate CR (Gilek et al.,
1992):
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Cmax=greatest difference in particle
concentration between two consecutive measurements, S=sedimentation
constant (0.049 and 0.059 for mussels and oysters, respectively) calculated as
the mean exponential decline in particle concentration in the chambers without
animal, V=volume of suspension, t=time between measurements
and m=dry tissue mass.
Oxygen consumption
Routine oxygen consumption
(
O2, or routine
metabolic rate) was determined at the end of the overwintering period on 12
April in each temperature treatment and during the spring–summer
simulation on 4 May and 31 May. Minimum oxygen consumption
(O2min, or
standard metabolic rate) was measured at the end of the experiment on 8 June,
after starving the animals for 8 days. Oxygen consumption for an individual
animal was determined by sealing the chamber and measuring the reduction in
%O2 with a YSI (5331) polarographic analyzer and electrode (Yellow
Springs, OH, USA). Seawater in the chamber was mixed with a magnetic stirrer.
The output signal was monitored continuously on a chart recorder until a
decrease of at least 20% O2 was reached. Respiration was then
expressed as ml O2 h–1 g–1 tissue
dry mass.
Lipid analysis
Tissue sampling
Mussel and oyster gills and digestive glands were sampled on 17 and 31
January, 14 February, 12 April, 4 May and 8 June in each temperature treatment
for determination of lipid class and fatty acid compositions. 2–3
mussels and oysters were randomly sampled in each tank for determination of
shell length, tissue AFDM, and lipid composition. Animals were dissected and
ca. 300 mg wet mass of tissue were stored in lipid-free amber glass vials with
TeflonTM-lined caps under nitrogen in 1 ml dichloromethane at
–80°C for later determination of lipid composition. Algae were
filtered on GF/C filters precombusted at 450°C and stored in amber glass
vials as previously described for tissues.
Lipid classes
Lipids were extracted following the method of Folch et al.
(Folch et al., 1957), spotted
onto S-III Chromarods (Iatron Laboratories Inc., Tokyo, Japan), and separated
into aliphatic hydrocarbons, sterol and wax esters, ketones, TAG, free fatty
acids, free fatty alcohol, free sterols, diacylglycerols, acetone mobile polar
lipids and phospholipids (Parrish,
1999). Chromarods were scanned by a flame ionization detection
system (Iatroscan Mark-VI, Iatron Laboratories Inc., Tokyo, Japan) and
chromatograms were analyzed using integration software (Peak Simple version
3.2, SRI, Torrance, CA, USA).
Neutral and polar lipid separation
Lipids were separated into neutral lipids (including triglycerides, free
fatty acids and sterols) and polar lipids (including mainly phospholipids and
minor amounts of glycolipids) using column chromatography on silica gel
hydrated with 6% water as previously described
(Pernet et al., 2006a).
Briefly, the 100 mg columns were preconditioned with 1 ml of methanol and 1 ml
of chloroform. Samples (200 µl) of lipid corresponding to 1 mg of
lipid were loaded onto the solid-phase extraction column. Samples were gently
drawn into the solid phase with a slight vacuum. Columns were washed with 1 ml
chloroform–methanol (98:2 v/v) to elute neutral lipids followed by 5 ml
of methanol to elute polar lipids. The fractions eluted were collected in 7 ml
tubes positioned in a vacuum manifold apparatus. The vacuum was adjusted to
generate a flow rate of 1 ml min–1.
Fatty acids
Fatty acid methyl esters (FAME) from neutral and polar lipids were prepared
using 12% BF3 in CH3OH following the American Oil
Chemists' Society method (AOCS,
1989). FAME were run on a Varian CP3900 gas chromatograph equipped
with a ZB-wax fused-silica capillary column (20 mx0.18 mm
i.d.x0.18 µm film thickness; Supelco, Bellfonte, PA, USA). Helium was
used as the carrier gas (flow velocity: 1 ml min–1). FAME
were injected at 250°C at a 1:10 split ratio. The temperature ramp was
140°C for 0.2 min, followed by an increase of 40°C
min–1 to 170°C, followed by an increase of 4°C
min–1 to 185°C, and finally by an increase of 2°C
min–1 to 230°C. The detector was maintained at 260°C.
FAME were identified by comparison of retention times with known standards (37
component FAME Mix, PUFA-3 and menhaden oil; Supelco Bellefonte, PA, USA) and
quantified with nonadecanoic acid (19:0) as an internal standard.
Chromatograms were analyzed using the Galaxie chromatography data system
(version 1.9.3.2, Varian, Mississauga, ON, Canada).
Statistical analyses
Analyses of variance (ANOVAs) were conducted to determine differences in
initial characteristics of the neutral and polar lipids between the two
bivalve species, M. edulis and C. virginica, before exposure
to overwintering temperatures. One-way ANOVAs were conducted to determine
differences between the two species in the relative TAG concentration, the
fatty acid composition and the unsaturation index [average number of double
bonds per acyl chain as calculated in Logue et al.
(Logue et al., 2000)] of the
neutral lipids in digestive glands. Minor amounts of TAG (<0.5%) were
occasionally detected in gills and were not analyzed further. Two-way ANOVAs
were conducted to determine differences in the initial characteristics of the
membrane lipids as a function of bivalve species and tissue (gills and
digestive glands). Dependent variables were the phospholipid to sterol ratio,
the fatty acid composition and the unsaturation index of the polar lipids. The
unit of replication used in these analyses was the rearing tank in which the
animals were maintained (N=2).
Three-way split-split plot ANOVAs were conducted to determine differences
in the physiological rates (CR and
O2) and the
neutral lipids of digestive glands, i.e. the relative TAG concentration, the
unsaturation index and the major polyunsaturated fatty acids (PUFA), namely
22:6n-3, 20:5n-3 and 18:4n-3, as a function of overwintering temperature,
species and date. The unit of replication was the tank in which the
overwintering temperature was applied (N=2 for each temperature). The
main plots were overwintering temperature levels (0, 4 and 9°C), subplots
were species levels (mussel and oyster), and sub-subplots were sampling dates.
Four-way split-split plot ANOVAs were used to determine differences in the
phospholipid to sterol ratio, the unsaturation index and major PUFA of the
polar lipid fraction, namely 22:6n-3, 20:5n-3, 20:4n-6, 22:2 and 20:2 NMI, as
a function of overwintering temperature, species, tissue and date
(Fig. 1B). Features of the
four-way split-split plot experimental design were similar to those of the
three-way plot except that sub-subplots also included tissue levels (gills and
digestive glands). Here we used a mixed linear model, which models not only
the means of our data but their variances and covariances. The need for
covariance parameters arose because the experimental units on which the
variables were measured were grouped into clusters and repeated measurements
were taken on the same experimental unit. The repeated option was applied to
the interaction terms `Date' and `TissuexDate' for the three-way and
four-way split-split plot experimental designs, respectively. These terms were
combined with the covariance structure of the matrix to take into account
spatial and temporal dependence (SAS Institute 2002).
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2x), resulting
in CR values of 5.1 l h–1 g–1 dry mass
for the three overwintering groups at the end of the experiment
(Fig. 2A). As in mussels, the
CR of oysters increased during the spring–summer simulation. However,
the CR of mussels was always higher than that of oysters, where it varied
between 1.1 and 3.6 l h–1 g–1 dry mass as a
function of overwintering temperature. Oysters overwintered at 9°C showed
a greater increase in CR than those overwintered at lower temperatures.
There was no effect of overwintering temperature on the oxygen uptake of
mussels and oysters (Temperature effect: P=0.904, F=0.10,
d.f.=2; TemperaturexSpecies effect: P=0.809, F=0.23,
d.f.=2; TemperaturexDate effect: P=0.210, F=1.58,
d.f.=6; TemperaturexSpeciesxDate effect: P=0.808,
F=0.49, d.f.=6). At the end of the overwintering period, mussels and
oysters showed similar rates of oxygen uptake
(Fig. 2B, P=0.534),
but the increase in
O2 during the
spring–summer simulation was greater in mussels (4.8x) than in
oysters, where the
O2 increased by
only 3.2x (SpeciesxDate effect: P<0.002,
F=11.2, d.f.=3). After food deprivation, the oxygen uptake of mussels
and oysters maintained at 20°C for 5 weeks decreased by 2.2 and 1.8x
respectively. The
O2min of mussels
was 1.6x higher than that of oysters at 20°C
(Fig. 2B).
Storage lipids
The initial concentration of TAG in the digestive gland, expressed as mg
g–1 AFDM, was 3.7x higher in mussels than in oysters
(Table 2). TAG levels in mussel
digestive glands decreased during the entire study, whereas TAG remained
almost constant in oysters (Fig.
3, Table 3). During
the entire study, mussels used 48.9 mg g–1 AFDM of TAG, which
represented 80% of the initial TAG level. The unsaturation index of
digestive gland TAG was initially 21% higher in mussels than in oysters and in
the diet (Table 2,
Fig. 3). The species effect on
the unsaturation index was mainly attributable to PUFA and more particularly
to 20:5n-3, which was 1.6–1.8x higher in mussels than in oysters
and the food, respectively. During the experiment, the unsaturation index of
the digestive gland TAG varied as a function of species and date
(Fig. 3,
Table 3). In mussels, the
unsaturation index remained elevated during overwintering and decreased only
during the spring–summer simulation at 20°C. In oysters, the
unsaturation index increased 12% during overwintering and decreased until
attaining initial values when temperature was raised to 20°C. A stepwise
multiple regression model using groups of fatty acids as explanatory variables
and the unsaturation index as the response variable showed that the
unsaturation index was positively correlated with PUFA
(y=5.2xPUFA–21.8; r2=0.909,
N=60, P<0.001; Fig.
3). A second regression model using individual PUFA as explanatory
variables showed that variations in the unsaturation index were mostly
attributable to 22:6n-3 for the two species
(y=11.0x22:6n-3+111.7; r2=0.734,
N=60, P<0.001; Fig.
3) and 20:5n-3 (y=5.9x22:6n-3+151.7;
r2=0.735, N=60, P<0.001;
Fig. 3). The fatty acid 22:6n-3
increased significantly by 16% in the digestive gland TAG in the two species
during overwintering before decreasing until the end of the study. The fatty
acids 20:5n-3 and 18:4n-3 in mussel digestive glands decreased during the
entire study, whereas in oysters, 20:5n-3 decreased only when the temperature
was increased to 20°C and 18:4n-3 remained constant
(Fig. 3,
Table 3).
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The relative mobilisation of 17 fatty acids from mussel and oyster digestive glands was approximated as the ratio of their molar percentage (mol %) in initial TAG to that in TAG at the end of the study period (Fig. 4). A ratio greater than, equal to, or lower than unity indicates that the fatty acid is mobilised more, equally, or less readily than the total TAG-fatty acids, respectively. Overall, the most readily mobilised fatty acids in mussels were 18:4n-3 and 20:5n-3, which ranged from 2.19–3.05 and 1.99–2.39, respectively. Interestingly, during overwintering, 18:4n-3 seemed to be mobilised less readily in mussels overwintered at 0°C and 4°C than in mussels maintained at 9°C whereas the inverse was true during the spring–summer simulation: 18:4n-3 seemed to be mobilised more readily in mussels overwintered at 0°C than in mussels maintained at higher temperatures. In oysters, the most readily mobilised fatty acid was 20:1n-9, which ranged between 1.34 and 2.00. Due to the low contribution of 20:1n-9 to the total TAG-fatty acids (<1%, Table 2), selective mobilisation of 20:1n-9 only had a marginal effect on the fatty acid composition of TAG.
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Membrane lipids
The phospholipid to sterol (ST) ratio varied as a function of time, tissue
and species (Fig. 5,
Table 4,
Table 5). Mussel and oyster
tissues showed a 1.2-fold increase in their phospholipid to sterol ratio
between 12 April and 4 May, when temperature increased from 0°C, 4°C
or 9°C to 20°C. The phospholipid to sterol ratio of digestive glands
was 1.4x higher than that of gills (11.9 and 8.4, respectively;
Fig. 5), mainly due to the
higher ST content in gills (Table
4). Interestingly, mussels were characterised by a phospholipid to
sterol ratio 1.5x higher than in oysters, irrespective of time or tissue
(Fig. 5).
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The unsaturation index was initially 5.2% higher in mussels than in oysters and 3.3% higher in digestive glands compared to gills (Table 4). The unsaturation index varied as a function of tissuexdate. In gills, the unsaturation index increased slightly (by 3.6%) during early overwintering, remained elevated during overwintering, and decreased markedly during the spring–summer simulation at 20°C. In digestive glands, the unsaturation index remained constant during overwintering and decreased markedly during the spring–summer simulation. The unsaturation index also varied as a function of speciesxtissue (Fig. 5, Table 5). As observed for TAG, the unsaturation index of polar lipids was positively correlated with PUFA (y=4.4xPUFA–6.4; r2=0.867, N=120, P<0.001; Fig. 5) and more particularly with 22:6n-3 (y=7.8x22:6n-3+144.4; r2=0.633, N=120, P<0.001; Fig. 5) and 20:5n-3 (y=4.6x22:6n-3+192.8; r2=0.601, N=120, P<0.001; Fig. 5). The fatty acid 22:6n-3 remained constant during overwintering and decreased by 35.5% during the spring–summer simulation, irrespective of species or tissue. The fatty acid 20:5n-3 varied as a function of tissuexdate, speciesxdate and speciesxtissue (Fig. 5, Table 5). Although some minor differences occurred in the dynamics of 20:5n-3 during overwintering between species and tissues, 20:5n-3 decreased during the spring–summer simulation in digestive glands and gills for both mussels and oysters (Fig. 5).
Overall, there was no significant effect of overwintering temperature on the fatty acid composition of membrane lipids. However, regression models using temperature as an explanatory variable and the unsaturation index of animals acclimated at 0°C, 4°C, 9°C (April 12) and 20°C (June 8) as the response variable showed that the unsaturation index in gills was negatively correlated with temperature (Fig. 6A). Interestingly, the unsaturation index of mussels was higher than that of oysters, irrespective of acclimation temperature. In mussel gills, 20:5n-3 showed a wider range of variation (8.0–16.5%) than 22:6n-3 (12.7–16.7%) in response to acclimation temperature, whereas in oyster gills, 20:5n-3 and 22:6n-3 varied to the same extent (Fig. 6B). In contrast to gills, the unsaturation index in digestive glands was not significantly correlated with acclimation temperature: a threshold value was attained at 9°C and did not increase further with a decrease in temperature.
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The fatty acid 20:4n-6, an eicosanoid precursor of many biologically active lipids, showed species- and tissue-specific patterns (Table 4). Indeed, 20:4n-6 was initially lower in mussels (4.4%) than in oysters (5.9%) and lower in digestive glands (4.3%) compared to gills (6.0%, Table 4). The fatty acid 20:4n-6 varied as a function of overwintering temperaturexspeciesxdate (Fig. 7, Table 5). During the overwintering period, 20:4n-6 increased in mussels whereas it remained stable in oysters. Therefore, at the end of the overwintering period, mussels and oysters showed similar levels of 20:4n-6. During the spring simulation period, 20:4n-6 increased markedly in mussels, increased moderately in oysters overwintered at 0°C and 9°C, and did not increase significantly in oysters overwintered at 4°C.
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). In contrast, C. virginica,
which generally occurs in warmer habitats, showed low and constant TAG
concentrations during overwintering. This mirrors biogeographical patterns of
reliance on lipids for energy metabolism among marine species. For example,
herbivorous copepods from polar and temperate areas use lipid stores for
energy and reproductive needs during the fall and winter, presumably in
response to the cyclic annual productivity typical of northern food webs,
whereas zooplankton from tropical biomes generally do not accumulate large
lipid stores (Lee et al.,
2006). Likewise, the capacity for lipid storage increases in
cold-adapted and cold-acclimated fish
(Pörtner, 2002;
Guderley, 2004). Although
mussels and oysters overlap in their distribution, the discrepancy in their
TAG metabolism may reflect the fact that mussels grow better in colder
habitats than oysters do.
Alternatively, differences in TAG metabolism between the two species may
reflect differences in their reproductive cycle at low temperatures. The
synthesis, storage and use of TAG often show pronounced seasonal cycles in
bivalves: TAG are sequestered during periods of high food availability in late
summer and fall, and are subsequently used for maintenance metabolism during
periods of reduced feeding in the winter and for initiation of gametogenesis
(De Zwaan and Mathieu, 1992;
Thompson et al., 1996;
Barber and Blake, 2006 and
references therein). It is therefore likely that the TAG stored in digestive
glands of mussels were transferred to the developing gonads during
overwintering. By contrast, oysters that showed low and constant levels of TAG
during overwintering may be quiescent, waiting for the spring revival to
initiate gametogenesis. According to their specific environment, bivalves may
support gametogenesis using recently ingested food, stored reserves or a
combination of the two (Barber and Blake,
2006).
Discrepancies in TAG dynamics between mussels and oysters during
overwintering partly reflect differences in feeding rate. At 9°C, the
temperature at which animals were maintained for 8 weeks before the experiment
began, the CR of mussels was higher (2.8 l h–1
g–1 dry mass) than that of oysters, where the CR was well
below <0.5 l h–1 g–1 dry mass
(Fig. 2A). Therefore, mussels
likely accumulated more lipids from phytoplankton prior to overwintering than
did oysters, explaining the higher TAG levels in mussel digestive glands at
the onset of the experiment. While the CR of mussels increased with
overwintering temperature, as found by Cusson et al.
(Cusson et al., 2005) and
references therein, that of oysters maintained at 0°C, 4°C and 9°C
was similar. Although few studies have specifically examined the effect of
temperature on feeding in C. virginica, one paper reports that this
species does not feed below 5°C
(Loosanoff, 1958), in
agreement with our results.
Not only were mussels characterised by a greater capacity for TAG
accumulation compared to oysters, but they also seemed better able to
selectively incorporate 20:5n-3. This essential fatty acid was markedly higher
in mussel than in oyster TAG and largely exceeded dietary levels. Although the
fatty acid composition of the TAG in bivalve digestive glands generally
reflects that of their diet (Soudant et
al., 1999), scallop larvae fed a diet rich in 20:5n-3
preferentially accumulate 22:6n-3 at the expense of 20:5n-3 in their TAG,
suggesting regulation of the incorporation/utilisation of essential PUFA in
TAG (Delaunay et al., 1993).
M. edulis may deposit more 20:5n-3 into TAG than C.
virginica, thus increasing the availability of storage fats at low
temperatures (Florant,
1998).
During overwintering, mussels decreased the proportion of certain
unsaturated fatty acids in TAG, with 20:5n-3 and 18:4n-3 declining markedly
during the study, whereas oysters showed fewer changes (Figs
3 and
4). The Antarctic fish
Trematomus newnesi preferentially oxidises unsaturated fatty acids
(Lund and Sidell, 1992), with
the hormone-sensitive lipase (HSL) of its adipose tissue preferring substrates
in the order PUFA>monoenes>saturates
(Hazel and Sidell, 2004).
Mammalian HSL shows similar substrate preferences
(Raclot, 2003). Although this
lipase has not been studied in bivalves, the decrease in 20:5n-3 and 18:4n-3
from the TAG in mussel digestive glands suggests a similar selectivity. The
minimal changes of oyster TAG during overwintering may reflect the limited TAG
deposition at the start of the study more than differences in the HSL
properties. Despite the fact that 20:5n-3 and 18:4n-3 decreased markedly in
mussel TAG during overwintering, the more constant levels of 22:6n-3, 20:4n-6
and NMI fatty acids and the decrease of 16:0 maintained the % PUFA and the
unsaturation index constant during overwintering.
The marked decrease in 20:5n-3 in TAG of mussel digestive gland during
overwintering could reflect utilisation of this PUFA for maintenance during
periods of reduced feeding or for initiation of gametogenesis. In support of
the latter, a recent study showed that the female gonad of the scallop
Nodipecten subnodosus specifically accumulates 20:5n-3 during
gametogenesis (Palacios et al.,
2005). If 20:5n-3 is also accumulated in the developing gonads of
mussels, it must come from dietary sources or from stored lipids since
bivalves have a limited capacity for de novo synthesis of long-chain
PUFA (DeMoreno et al., 1976;
Langdon and Waldock, 1981;
Delaunay et al., 1993;
Caers et al., 2003).
The rate of change of 18:4n-3 levels in digestive gland TAG fell as a function of overwintering temperature and then rose during the spring–summer simulation (Fig. 4). At first glance, a reduced mobilisation of 18:4n-3 at low temperatures would seem to help maintain fluidity, and thus the availability of the TAG, at low temperatures. However, the unsaturation index of the TAG, which is a good indicator of the melting point, was similar among mussels overwintered at 0°C, 4°C and 9°C. Therefore, it is unlikely that reduced mobilisation of 18:4n-3 counteracted an ordering effect of low temperatures on the TAG. The functional role of reduced mobilisation of 18:4n-3 at low temperatures remains unclear.
Membrane lipids: HVA and metabolism
The increase in the phospholipid to sterol ratio during the early stage of
warming in mussels and oysters (Fig.
5) suggests that sterols were not used for HVA
(Robertson and Hazel, 1995;
Crockett, 1998;
Zehmer and Hazel, 2003). If
the distribution of sterols in cellular membranes is similar to that in
vertebrates (Lange et al.,
1989; Lange and Steck,
1996) changes in the relative importance of plasma and organelle
membranes could be the cause of this pattern. HVA may have been accomplished
by the decreased unsaturation of phospholipid acyl chains with increasing
temperature. Furthermore, the sterols of marine bivalves include a complex
mixture of phytosterols (Knauer et al.,
1998) that have less of an ordering effect on membranes than
cholesterol (Suckling et al.,
1979).
The higher phospholipid to sterol ratio of digestive glands compared to
gills agrees with patterns in rainbow trout, in which the ratio of cholesterol
to phospholipid is markedly higher in gills than in other tissues (including
liver) (Robertson and Hazel,
1995). The high cholesterol levels in gills may enhance their
permeability. The higher phospholipid to sterol ratio in digestive glands
could reflect a greater relative importance of organelles. Accordingly, in
C. virginica, the mitochondrial volume fraction was twice as high in
digestive gland as in gills (Cherkasov et
al., 2006).
The unsaturation index decreased during the beginning of warming in mussel
and oyster gills and digestive glands, principally due to 22:6n-3 and 20:5n-3
(Fig. 5). Although membrane
fluidity was not measured in our study, these temporal variations in 22:6n-3
and 20:5n-3 may counteract the disordering effect of rising temperatures.
Accordingly, 22:6n-3 is thought to be important in controlling membrane
fluidity during cold acclimation of fish
(Dey et al., 1993;
Buda et al., 1994;
Tiku et al., 1996;
Logue et al., 2000).
Furthermore, a 45% increase in 20:5n-3 in gill membranes of the sea scallop
P. magellanicus after 21 days of acclimation at 5°C correlates
with an increase in membrane fluidity
(Hall et al., 2002).
For both mussels and oysters, the unsaturation index of digestive gland
phospholipids was not correlated with acclimation temperature, whereas a
perfect negative relationship was observed in gills as predicted by HVA. Thus
the unsaturation index attained a threshold value at 9°C in digestive
glands while it continued to increase with falling temperatures in gills. The
microenvironments of gills and digestive glands may require different physical
responses by the membranes. In support of this hypothesis, the basolateral and
brush border membranes from intestinal epithelia of cold- and warm-acclimated
rainbow trout respond to thermal acclimation in opposite fashions
(Crockett and Hazel, 1995).
Basolateral membranes exhibit perfect homeoviscous efficiency due to an
increase in the unsaturation index, whereas brush border membranes from
cold-acclimated fish are more ordered than those from warm-acclimated fish.
These authors suggest that bile and digestive lipase, two constituents of the
brush border membrane microenvironment, may impose unusual physical
requirements. The fact that the unsaturation index of digestive gland
phospholipids did not increase beyond a threshold value at 9°C in both
oysters and mussels suggests a need for stability of the membrane to
counteract regular exposure to digestive enzymes and acids.
The inverse relationship between the unsaturation index of gill
phospholipids and acclimation temperature was principally due to changes in
22:6n-3 and 20:5n-3, but the magnitude of the response of these fatty acids
varied between oysters and mussels (Fig.
6B). The decrease of 20:5n-3 with a rise in temperature was much
stronger in mussels than oysters. Reliance on 20:5n-3 for remodelling membrane
phospholipids in mussels goes hand in hand with the importance of this fatty
acid in TAG metabolism. As the melting point of 20:5n-3 is 10°C lower than
that of 22:6n-3, efficiency of HVA in mussels is likely higher than that of
oysters. HVA efficiency varies among species, ranging from 20 to 100% for
thermal acclimation and averaging 70% for thermal adaptation
(Hazel, 1995).
Both oxygen uptake and membrane unsaturation were higher in mussels than
oysters, irrespective of temperature, time or tissue
(Fig. 2B). Similarly, standard
O2 and
phospholipid unsaturation show a positive correlation in comparisons of wild
and selectively bred hard clams (Pernet et
al., 2006b). The unsaturation of membrane phospholipids is
positively correlated with basal metabolic rate
(Hulbert and Else, 1999;
Hulbert and Else, 2005) in
allometric comparisons of mammals and birds. The positive relationship between
standard O2 and
phospholipid unsaturation in mussels and oysters suggests that Hulbert's
theory of membranes as metabolic pacemakers may be applicable to
invertebrates.
Membrane lipids: why do 20:4n-6 and NMI fatty acids not follow HVA?
One of the most important functions of C20 PUFA is as precursors
of eicosanoids, a group of hormones that includes prostaglandins, leukotrienes
and hydroxyeicosatetraenoic acids (Smith
and Murphy, 2003). The increase in 20:4n-6 in mussels during the
spring–summer simulation period (Fig.
7) may compensate for the concomitant decrease in 20:5n-3.
Eicosanoid production is associated with stressful or energetically expensive
situations, such as gametogenesis and spawning in bivalves or stimulation of
immune function in other invertebrates
(Osada et al., 1989;
Stanley and Howard, 1998).
Since eicosanoids produced from 20:4n-6 are generally more active than those
produced from 20:5n-3, the replacement of 20:5n-3 by 20:4n-6 in mussels may
have significant impacts. Levels of 20:4n-6 in mussels may have risen during
the spring–summer simulation through the stimulation of immune function
due to increased bacterial loads in the seawater as temperature rose.
Similarly, an increase in 20:4n-6 in scallop and haddock larvae coincided with
elevated mortality and exposure to pathogenic and opportunistic microbes
(Pernet et al., 2005;
Plante et al., 2007). Bivalve
haemocyte membrane lipids contain elevated amounts of 20:4n-6, presumably to
regulate immune responses (Delaporte et
al., 2003). We suggest that the increase in 20:4n-6 levels during
the spring–summer simulation may reflect an increased demand for
20:4n-6-rich immune cells to control bacterial proliferation in mussels
(Delaporte et al., 2006).
In contrast to our previous work on juvenile hard clams, where we observed
an increase in 22:2 NMI during a decrease in temperature
(Pernet et al., 2006b), NMI
fatty acids in mussel and oyster tissues showed no consistent response to
temperature change (Fig. 8). In
contrast to essential PUFA, NMI fatty acids are synthesised de novo
by bivalves (Zhukova, 1991).
Therefore, the synthesis of NMI fatty acids was suggested as an alternative to
the selective incorporation of essential PUFA at low temperatures,
particularly when phytoplankton concentrations are low or when feeding has
ceased (Pernet et al., 2006b).
When extended, this argument would suggest that the synthesis of NMI fatty
acids could be important in animals that do not have any source of PUFA,
either from exogenous feeding or endogenous reserves. Although endogenous TAGs
are generally considered as energy reserves, they also constitute a PUFA
reservoir that could be used for remodelling membrane lipids as the need
arises. This hypothesis suggests that oysters had more changes in NMI than
mussels because they had fewer TAG reserves at the onset of overwintering.
In conclusion, we found major differences between species in lipid dynamics that correlate with the species' thermal habitats, with mussels apparently maintaining the fluidity of digestive gland TAG during over-wintering, presumably to facilitate their use at cold temperatures. The exploitation of cold habitats by oysters may be limited by reduced feeding at low temperatures and their limited changes in TAG fluidity during over-wintering at cold temperatures. On the other hand, over-wintering led to marked membrane remodelling in both oysters and mussels. In both species, the unsaturation of gill phospholipids perfectly followed HVA, whereas in digestive glands, unsaturation and temperature were only related down to 9°C. By comparing mussels and oysters before and during acclimation to three over-wintering temperatures, and after the spring revival, we obtained a comprehensive view of their lipid dynamics and physiological responses. More broadly, this study suggests that lipids can be used as biochemical indicators of condition to gain mechanistic insight into the effects of climate change on economically important poikilotherms that occur in stressful habitats or at the edge of their distribution range.
List of abbreviations
O2
O2min
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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