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First published online November 2, 2007
Journal of Experimental Biology 210, 4016-4023 (2007)
Published by The Company of Biologists 2007
doi: 10.1242/jeb.007708
Endurance swimming activates trout lipoprotein lipase: plasma lipids as a fuel for muscle
Biology Department, University of Ottawa, 30 Marie Curie, Ottawa, Ontario, K1N 6N5, Canada
* Author for correspondence (e-mail: jmweber{at}uottawa.ca)
Accepted 3 September 2007
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Key words: sustained swimming, aerobic exercise, fish metabolism, lipoproteins, lipolysis, red muscle, heparin, rainbow trout, Oncorhynchus mykiss
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Introduction |
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; Moyes and West,
1995; Richards et al.,
2002; Rome, 1998).
By analogy with mammals, most fish studies have investigated the metabolic
role of non-esterified fatty acids (NEFA), assuming that these lipids are
responsible for transporting energy from adipose stores to locomotory muscles
(Ballantyne et al., 1996;
Bernard et al., 1999;
Booth et al., 1999;
Weber et al., 2002). This
assumption is probably not justified, however, because (1) NEFA only account
for a small percentage of the energy in plasma lipids
(Babin and Vernier, 1989;
Plisetskaya, 1980), and (2)
endurance swimming has no effect on the turnover rate or concentration of
plasma NEFA (Bernard et al.,
1999). Although lipoproteins are used for transport to the gonads
during egg production (Babin and Vernier,
1989), they have not been considered as a possible energy shuttle
to working muscles. This is surprising because they carry most of the energy
in the circulation (Moyes and West,
1995) and could theoretically play an important role in powering
muscles during swimming. Lipoprotein lipase (LPL; EC 3.1.1.34) is the enzyme
controlling the mobilization of lipoproteins and it has been well
characterized in fish tissues (Lindberg
and Olivecrona, 2002). Its potential role in orchestrating the
supply of lipid fuel to working muscles has never been investigated. LPL is
naturally bound to proteoglycans in the endothelium, but it can be released in
the circulation by injecting heparin that has a higher affinity for the enzyme
(Cryer, 1981). In this study,
we have used heparin as a tool to characterize reserve capacity for
lipoprotein catabolism, and to help us determine how exercise might modify the
activity of this key enzyme. We could only find two studies where heparin had
been used to investigate LPL in vitro
(Lindberg and Olivecrona,
1995) or in vivo, but in a single fish in the resting
state (Skinner and Youssef,
1982).
In wild sockeye salmon, we have previously proposed that lipoproteins are
used to support swimming because their concentration changes dramatically
during migration (Magnoni et al.,
2006). However, it is unclear whether this response to migration
is only caused by exercise or by a combination of stresses including swimming,
fasting, reproduction and osmoregulation. To exclude confounding factors, this
study investigates the effects of endurance swimming on lipoprotein metabolism
of rainbow trout under controlled laboratory conditions. Previous work had
shown that the catabolism of very low density lipoproteins (VLDL) yields
smaller particles such as VLDL-remnants or LDL
(Havel, 1987;
Zechner, 1997), and that
monounsaturated fatty acids are a preferred substrate for oxidation
(Henderson and Sargent, 1985;
Kiessling and Kiessling, 1993;
Sidell et al., 1995;
Weber et al., 2002). We
hypothesize that both LPL (enzyme) and plasma lipoproteins (substrate) are
modified by prolonged exercise. It is predicted that endurance swimming will
(1) activate LPL in red muscle, and (2) alter circulating lipoprotein classes
(high-, low- and very low density lipoproteins: HDL, LDL and VLDL,
respectively), components (triacylglycerol, phospholipids and NEFA), and
composition (individual fatty acids). Our goals were to measure the effects of
endurance exercise on LPL activity and on key characteristics of circulating
lipoproteins. We have examined whether red muscle LPL and post-heparin plasma
LPL are modified by several days of continuous swimming.
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) for FA composition]. The animals were fasted for 48 h before
starting experiments to eliminate circulating chylomycrons
(Wallaert and Babin,
1994).
Exercise experiments
Fish were randomly divided into two groups: control and exercise. Pairs of
animals were always measured simultaneously to be able to correct for
potential effects of fasting. Exercising fish were placed in a modified
Blazka-type swim tunnel (see Bernard et
al., 1999). Resting fish were measured in a tube with similar
dimensions to the exercise chamber of the swim tunnel. For acclimation to the
experimental setup, the animals were kept at rest in a weak water current (11
cm s–1) for 24 h. For the following 4 days, the control fish
was kept at rest, but the exercising fish had to swim at 1.5 BL
s–1 (46 cm s–1). At the end of the
experiment, both fish were rapidly removed from water and killed by a sharp
blow to the head. Blood (5 ml) was sampled from the caudal artery within 1 min
after death using EDTA as anticoagulant (1 mg ml–1). Plasma
was separated by centrifugation (5000 g for 10 min at
13°C) and used for the analysis of circulating lipoproteins. Red muscle
(
2 g) from the caudal region of the lateral line was dissected in <2
min and stored at –80°C for LPL analysis.
Heparin experiments
A single catheter was surgically implanted in the dorsal aorta using
buffered ethyl-N-aminobenzoate sulphonic acid as anaesthetic (MS-222,
Sigma, St Louis, MO, USA) and sodium citrate as anticoagulant (13 µmol
ml–1). The animals were allowed to recover for 24 h in opaque
PlexiglasTM chambers (see Haman and
Weber, 1996). Resting fish were injected with heparin (200, 600 or
1000 U kg–1 body mass; Hepalean, Organon, Toronto, ON,
Canada) and blood (0.5 ml) was collected before and after heparin injection.
Plasma was immediately separated and stored at –80°C for subsequent
analyses of LPL activity, as well as circulating triacylglycerol (TAG) and
glycerol concentrations (Sigma kits, St Louis, MO, USA).
Exercise + heparin experiments
Animals implanted with a dorsal aorta catheter were randomly divided into
two groups: resting controls and swimming. Surgical procedures and swimming
conditions were the same as above. After 4 days of rest or exercise, blood
samples (0.5 ml) were obtained through the catheter before and 1 h after the
administration of 600 U heparin kg–1 body mass to measure
plasma LPL activity.
Lipoprotein lipase
LPL activity was measured in frozen samples within 4 weeks of sampling
because preliminary experiments showed that it was not affected by freezing.
For red muscle, 0.5 g tissue was homogenized in 9 vol. buffer (10 mmol
l–1 Hepes, 1 mmol l–1 EDTA, 1 mmol
l–1 dithiothreitol and 5 U heparin ml–1 at
pH 7.4) using a ground glass homogenizer on ice. Homogenates were centrifuged
(20 000 g, 20 min at 4°C) and the clear phase between the
top layer and the pellet was used for LPL analysis. The characteristics of the
substrate used to measure LPL activity have been described in detail elsewhere
(Bengtsson-Olivecrona and Olivecrona,
1991). A 20% lipid solution (Intralipid, Sigma, St Louis, MO, USA)
was emulsified with tri[9,10(n)-3H]oleate (Amersham,
Buckinghamshire, UK). This type of emulsion has been commonly used to measure
LPL in a variety of vertebrate tissues
(Karpe et al., 1998;
Lindberg and Olivecrona,
1995), and its suitability as an artificial substrate has been
specifically demonstrated for rainbow trout plasma and tissues
(Albalat et al., 2005;
Albalat et al., 2006;
Lindberg and Olivecrona,
2002). Briefly, radiolabeled trioleate (1.7 MBq) was dried
under N2 and resuspended in 2 ml Intralipid solution and 8 ml
Cortland saline. This mixture was sonicated for 5 min at 70% pulse mode and
low setting (Branson Sonifier 450; Danbury, CT, USA). Each assay was carried
out using a 50 µl aliquot of the emulsion as substrate, mixed with 50 µl
preheated rat serum, 250 µl assay medium, and 100 µl plasma or red
muscle homogenate. The reaction was stopped after 1 h incubation at 20°C
by adding 3 ml methanol:chloroform:heptane (1.41:1.25:1 v/v/v) and 100 µl
0.1 mol l–1 NaOH. After centrifugation (1200
g, 20 min at 20°C), 1 ml of the upper phase was counted in
10 ml Safety Solve cocktail (Research Products, Mount Prospect, IL, USA) using
a liquid scintillation counter (Beckman Coulter CS6500, Palo Alto, CA, USA).
All LPL determinations were performed in triplicate.
Lipoprotein analysis
Lipoprotein classes were separated by ultracentrifugation (Beckman TL
Optima; Palo Alto, CA, USA) using a self-generated gradient (Optiprep,
Axis-Shield, Oslo, Norway) (see Graham et
al., 1996). Fresh plasma (3.2 ml), Optiprep gradient (0.8 ml) and
buffered saline (0.7 ml) were layered in Optiseal ultracentrifuge tubes
(Beckman Coulter, Palo Alto, CA, USA) before centrifugation (350 000
g, 3 h at 13°C). The different lipoprotein fractions were
collected: high-density lipoproteins (1.6 ml), LDL (1.6 ml) and VLDL (1.5 ml).
The exact nature of the three lipoprotein fractions was confirmed with agarose
gels (Paragon electrophoresis system, Beckman Coulter, Fullerton, CA, USA).
Fractions were stored at –80°C for subsequent analysis. Protein
content was measured using the Bradford reagent (Sigma). Three lipid classes
[NEFAs, TAG and phospholipids (PLs)] were separated in each lipoprotein
fraction following published methods
(Magnoni et al., 2006), and
their FA concentration and composition were measured by gas chromatography
after methylation (NEFAs) or acid transesterification (TAG and PLs)
(Abdul-Malak et al., 1989;
Chapelle and Zwingelstein,
1984). Heptadecanoic acid (17:0) was used as an internal standard
because preliminary experiments showed that this acid is absent from NEFA, TAG
and PL of trout plasma. The fatty acid methyl esters obtained were analyzed on
an Agilent Technologies 6890N gas chromatograph equipped with a fused silica
capillary column (Supelco DB-23, 60 mx0.25 mm i.d., 0.25 µm film
thickness), using hydrogen as carrier gas at constant pressure and linear flow
of 43 cm s–1. The system was equipped with an automatic
injection system (Agilent Technologies 7683B Series). The following conditions
were used during analysis: (a) oven temperature was programmed for 1 min at
130°C, up to 170°C at 6.5°C min–1, up to
215°C at 2.75°C min–1, held at 215°C for 12 min,
up to 230°C at 40°C min–1, and held at 230°C for
3 min, (b) injector temperature was 270°C using a 50:1 split ratio, and
(c) detector temperature was 280°C. Each methyl ester was identified
specifically by determining its exact retention time with an authentic
standard (Supelco, Bellefonte, PA, USA). Only the fatty acids representing
more than 1% of total fatty acids in each lipid fraction are included in
calculations.
Statistical analyses
A Student's? t-test was used to evaluate the effects of swimming
on LPL activity in red muscle. In all other cases, statistical differences
were assessed using analysis of variance (ANOVA), or Kruskal–Wallis
ANOVA on ranks when the assumption of normality or homoscedasticity was not
met. When significant changes were detected by ANOVA, the Holm–Sidak
method was used for pairwise comparisons. Percentages were transformed to the
arcsine of their square root before statistical analysis and all values given
are means ± standard error of the mean (s.e.m.).
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Lipoproteins were also analyzed by separating their various components. The
concentrations of PL, TAG and NEFA in the three classes of lipoproteins are
shown in Fig. 3. Endurance
swimming had no measurable effect on these parameters (P>0.05).
Phospholipid was the main lipid component of HDL (63% of total fatty acids in
HDL) and LDL (59% of total fatty acids in LDL), whereas TAG was the main lipid
component in VLDL (46% of total fatty acids in VLDL). NEFAs only represented
6–11% of total FA in the various lipoprotein fractions. The detailed
fatty acid composition of PLs, TAG and NEFAs in the three lipoprotein classes
was also analyzed. Because no measurable effect of endurance swimming was
detected on fatty acid composition (P>0.05), only pooled data for
control and exercised fish are presented in
Table 1, which groups
individual fatty acids into the major classes: saturated (SFAs),
monounsaturated (MUFAs) and polyunsaturated (PUFAs). In all lipoproteins,
PUFAs are the main fatty acids in PLs (63–71%) and TAG (47–51 %),
whereas SFAs are dominant in NEFAs (64–80%). MUFAs are thought to
provide the best fuel for oxidation
(Sidell et al., 1995) and they
account for an important fraction of TAG fatty acids (34–40%).
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Effects of heparin
The time course of changes in plasma LPL activity after injection of
heparin is presented in Fig. 4.
Baseline LPL activity was 0.04±0.01 µmol FA released
min–1 ml–1 plasma and it was strongly
stimulated 30–60 min after heparin administration, when maximal values
were recorded (1.07±0.20 and 1.32±0.67 µmol FA released
min–1 ml–1 plasma for heparin doses of 200
and 600 U kg–1, respectively) (P<0.001). Activity
stayed elevated above baseline for 2 h after heparin injection, but values
measured from 4 to 48 h after injection were not different from baseline
(P>0.05). Maximal stimulation of plasma LPL was already obtained
at 200 U heparin kg–1 because no significant difference
between the two doses were detected (P>0.05). This was confirmed
by administration of 1000 U kg–1 in four additional fish
(data not shown). Fig. 5 shows
the effects of heparin administration on the concentrations of plasma TAG and
plasma glycerol. Injecting 200 or 600 U heparin kg–1 had no
detectable effect on the concentrations of TAG or glycerol
(Fig. 5)
(P>0.05).
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Combined effects of swimming and heparin on plasma LPL
The effects of prolonged swimming and heparin on plasma LPL activity are
presented in Fig. 6. Heparin
had a major stimulating effect on plasma LPL activity (P<0.001),
but this strong response was not significantly different between resting fish
and those that had been swimming for 4 days at 1.5 BL
s–1 (P>0.05).
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Effects of swimming on red muscle LPL
Fish LPL has been characterized in most tissues (red and white muscle,
mesenteric fat, gonads and liver) where it is strongly modulated by seasonal
cycles associated with fasting and reproduction
(Black and Skinner, 1986;
Black and Skinner, 1987;
Fremont et al., 1987;
Ibáñez et al.,
2003; Lindberg and Olivecrona,
1995; Saera-Vila et al.,
2005). Our study is the first to examine the effects of sustained
swimming on this enzyme, and it shows that LPL is stimulated by exercise in
lateral red muscle, which is the engine for endurance swimming. The threefold
increase in LPL activity observed in trout muscle after prolonged exercise is
consistent with the response reported for several mammals, including rats
[two- to threefold (Bagby et al.,
1986; Ladu et al.,
1991a; Oscai et al.,
1982)], dogs [twofold
(Budohoski, 1985)] and humans
[threefold (Lithell et al.,
1984)]. In vitro experiments show that the addition of
LPL to co-culture systems containing lipoprotein-secreting hepatocytes and
muscle cells of fish increases muscle FA uptake by 60%
(Alam et al., 2004).
Tissue uptake of fatty acids from circulating lipoproteins is thought to be
limited by the rate of TAG hydrolysis and, therefore, it is mainly regulated
by LPL activity (Nilsson-Ehle,
1980). Numerous hormones, including insulin, catecholamines,
glucocorticoids and thyroxine, are well-known modulators of LPL. The relative
distribution of their various receptors is responsible for tissue-specific
responses (Mead et al., 2002).
The activation of mammalian LPL by exercise is linked to increased mRNA levels
in skeletal muscle (Kiens et al.,
2004), with catecholamines and insulin acting as the most probable
hormonal modulators (Chernick et al.,
1986; Enerback and Gimble,
1993; Ladu et al.,
1991b; Lithell et al.,
1981; Seip et al.,
1997). In addition to systemic regulation by hormones, local
signals associated with contractile activity have been implicated in LPL
modulation. In rats, a significant role for contractile activity is supported
by experiments in which electrical stimulation was performed unilaterally.
Stimulated muscles showed a threefold increase in LPL activity, whereas
contralateral (rested) muscles did not respond
(Hamilton et al., 1998). Taken
together, current data on the exercise-induced up-regulation of mammalian LPL
do not allow assessment of the relative importance of these various
mechanisms. For fish, even less information is available, but a significant
role for insulin modulation of muscle LPL appears doubtful. Recent experiments
show that in vivo administration of insulin causes the activation of
adipose tissue LPL in rainbow trout, but has no measurable effect on red
muscle (Albalat et al., 2006).
The exercise-induced activation of LPL observed in our study is therefore
probably associated with changes in circulating catecholamines or contractile
activity. For example, prolonged exercise causes a decrease in circulating
epinephrine levels (Shanghavi and Weber,
1999) that may be involved in LPL activation. Even though further
studies are needed to characterize exact regulation mechanisms in fish,
results clearly show that red muscle LPL is recruited during prolonged
swimming, making lipoproteins available as a fuel for locomotion.
Effects of heparin on plasma LPL
This study characterizes the activation of plasma LPL by heparin in intact
fish. It provides a time course of changes in circulating LPL activity for
different doses (200–1000 U heparin kg–1) and shows
that a maximal response is reached 1 h after injecting 600 U
kg–1. We are aware of only one other study investigating this
issue; it reports the partial response of an individual fish after injection
of 100 U kg–1 (Skinner
and Youssef, 1982). The maximal LPL activity measured here was
much higher than in this previous study and it occurred later (60 vs
35 min after injection). Such discrepancy is not simply due to the higher
doses used here, but mainly to the actual substrate for the LPL assay.
Intralipid-based emulsions (this study) are considered a better imitation of
real lipoproteins than those made with gum arabic (as in
Skinner and Youssef, 1982)
that yield sub-optimal hydrolysis of radiolabeled trioleate
(Bengtsson-Olivecrona and Olivecrona,
1991). This view is further supported by in vitro
measurements of plasma LPL on Intralipid emulsions that give values of up to
0.8 µmol FA min–1 ml–1
(Lindberg and Olivecrona,
2002), approaching maximal activities reported here (1.32 µmol
FA min–1 ml–1;
Fig. 4). Under baseline
conditions, LPL is mostly bound to the endothelium, and plasma LPL activity is
therefore very low (here, only 3% of peak, post-heparin values; see
Fig. 4). The injection of
heparin causes a drastic increase in activity by (1) releasing the enzyme in
plasma, and (2) inhibiting its normal uptake by the liver for degradation
(Chajek-Shaul et al., 1988).
The impressive 27-fold increase in activity observed here in plasma after
release of the enzyme by heparin demonstrates that rainbow trout tissues have
a remarkable reserve capacity for lipoprotein hydrolysis.
Combined effects of swimming and heparin on plasma LPL
One of the goals of this study was to determine whether the changes in
tissue LPL caused by exercise would be measurable in post-heparin plasma.
Contrary to expectation, the observed increase in red muscle LPL
(Fig. 1) was not mirrored by
post-heparin plasma LPL (Fig.
6). However, close examination of the data reveals a
non-significant trend towards an increase in the exercise group that would be
consistent with our red muscle results. It is also conceivable that the
activation of red muscle LPL is accompanied by inhibition of the enzyme in
other tissues, yielding no overall change in post-heparin plasma LPL.
Alternatively, the effect of exercise on red muscle LPL may not be large
enough to influence LPL activity in post-heparin plasma because trout red
muscle only represents 7% of total body mass. For example, rats using a larger
muscle mass than the trout of our experiments show a significant increase in
post-heparin plasma LPL after exercise
(Hamilton et al., 1998).
Lipoprotein concentration and composition
We were unable to demonstrate significant effects of endurance exercise on
the concentration or the composition of circulating lipoproteins. It might be
argued that the non-significant trends towards a decrease in the FA/protein
ratio and increase in TAG concentration observed for VLDL
(Fig. 2C and
Fig. 3B) may have become
significant with a larger sample size than used here. However, demonstrating
such effects of swimming does not appear practical or necessary for two
reasons: (1) sensitivity analysis reveals that sample sizes of more than 40
would be needed to reach significance with a minimal statistical power of 0.8
(SigmaStat 3.1, Systat Software Inc. 2004), and (2) by itself, a change in
concentration would not be sufficient to prove a role for lipoproteins as a
muscle fuel because mismatches between changes in flux and concentration are
common occurrences in animals, including rainbow trout (see
Haman et al., 1997). The large
increase in muscle LPL activity caused by swimming
(Fig. 1) implies that the rate
of lipoprotein turnover is stimulated and, therefore, that lipoprotein
concentration is a poor indicator of lipoprotein flux. This observation
reinforces the necessity for developing more sensitive methods to analyze the
effects of endurance swimming on lipoprotein metabolism, and, in particular,
to quantify lipoprotein flux. The exercise-induced activation of LPL is not
accompanied by changes in NEFA concentration and, therefore, locomotory
muscles must be able to take up NEFA rapidly after lipoprotein hydrolysis as
previously suggested (Cryer,
1981; Merkel et al.,
2002). Because prolonged swimming had no measurable effect on the
fatty acid composition of circulating lipoproteins, this study does not
support the hypothesis that any specific fatty acid is preferentially used by
locomotory muscles (selectivity).
The 27-fold increase in plasma LPL activity caused by heparin
(Fig. 4) does not have any
measurable effect on plasma TAG concentration
(Fig. 5), the main substrate
for the enzyme. In contrast, plasma TAG concentration of mammals is decreased
by endurance exercise (Ensign et al.,
2002; Hardman,
1998), and in vivo heparin administration has a marked
lipolytic effect on circulating TAG
(Skoglund-Andersson et al.,
2003). The high lipoprotein concentrations of fish compared to
mammals (Babin and Vernier,
1989) may be responsible for the concentration inertia observed
here in trout. Because concentration stays constant, tissue uptake of
lipoprotein-derived fatty acids must be regulated by changes in LPL activity
rather than by a mass action effect of its substrate
(Nilsson-Ehle, 1980).
Most lipoprotein studies report concentrations in mass % (mg/100 ml).
However, this unit fails to reveal quantitative differences in energy content
because lipoprotein classes contain different amounts of protein, as well as
cholesterol. To avoid this problem, Fig.
3 expresses concentrations of the different lipid components in
µmol FA ml–1 plasma (because fatty acids contain most of
the energy in lipoproteins). This figure shows that the great majority of the
energy circulating in the plasma lipids of rainbow trout resides in PLs (55%)
and TAG (37%), whereas NEFAs only make a minor contribution (8% of the
energy). Within each lipoprotein class, fatty acid content is similar, but
protein content is highly variable (HDL>LDL>VLDL). Therefore, the
FA/protein ratio ranges between 0.2 for HDL and 2.0 for VLDL
(Fig. 2). Using protein content
from Fig. 2B (in mg protein
ml–1 plasma: HDL=33, LDL=5 and VLDL=0.7) and published values
for percentage protein in each lipoprotein class by mass [% protein: HDL=45,
LDL=30 and VLDL=13 (Babin and Vernier,
1989)], we can estimate that 70% of all trout lipoproteins are
HDL, 21% are LDL and the remaining 9% are VLDL.
Conclusion
Red muscle LPL is activated by endurance swimming and rainbow trout show a
very high reserve capacity for the hydrolysis of circulating lipoproteins.
These novel characteristics of trout LPL and the fact that lipoproteins
contain 92% of the energy in plasma lipids imply that lipoproteins are used as
an energy shuttle between fat reserves and working muscles. Such a mechanism
contrasts with the classic mammalian strategy where lipid fuel is supplied by
NEFA–albumin complexes. Because lipoprotein concentration does not
reflect changes in flux, direct measurements of lipoprotein kinetics will be
needed as soon as adequate methods are developed.
List of abbreviations
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Acknowledgments |
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References |
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TOPSummaryIntroductionMaterials and methodsResultsDiscussionReferences |
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