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J. Biol. Chem., Vol. 277, Issue 14, 11927-11932, April 5, 2002
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From the Department of Medical Bioscience, Umeå University,
S-901 87 Umeå, Sweden
Received for publication, January 11, 2002
During short term fasting, lipoprotein lipase
(LPL) activity in rat adipose tissue is rapidly down-regulated. This
down-regulation occurs on a posttranslational level; it is not
accompanied by changes in LPL mRNA or protein levels. The LPL
activity can be restored within 4 h by refeeding. Previously, we
showed that during fasting there is a shift in the distribution of
lipase protein toward an inactive form with low heparin affinity. To
study the nature of the regulatory mechanism, we determined the
in vivo turnover of LPL activity,
protein mass, and mRNA in rat adipose tissue. When protein
synthesis was inhibited with cycloheximide, LPL activity and protein
mass decreased rapidly and in parallel with half-lives of around 2 h, and the effect of refeeding was blocked. This indicates that
maintaining high levels of LPL activity requires continuous synthesis
of new enzyme protein. When transcription was inhibited by actinomycin,
LPL mRNA decreased with half-lives of 13.3 and 16.8 h in the
fed and fasted states, respectively, demonstrating slow turnover of the
LPL transcript. Surprisingly, when actinomycin was given to fed rats,
LPL activity was not down-regulated during fasting, indicating that
actinomycin interferes with the transcription of a gene that blocks the
activation of newly synthesized LPL protein. When actinomycin was given
to fasted rats, LPL activity increased 4-fold within 6 h, even in
the absence of refeeding. The same effect was seen with Lipoprotein lipase
(LPL)1 plays an important
physiological role in regulating the release of fatty acids from
triglyceride-rich lipoproteins (1-4). The enzyme is synthesized in
several extrahepatic tissues, but the highest activities are found in
tissues that oxidize (e.g. heart and red skeletal muscle) or
store (e.g. adipose tissue) fatty acids. After
glycosylation, dimerization, and activation in the endoplasmic
reticulum, the enzyme is secreted, transported through the
extracellular matrix, and anchored to heparan sulfate proteoglycans on the intraluminal surface of nearby capillaries (3,
4).
LPL is regulated at the level of gene expression in several
physiological states: during fetal and early postnatal life, the enzyme
is present in the liver but is then suppressed (5); in the mammary
gland, the enzyme is switched on during lactation (6); in macrophages,
it is switched on when the cells are activated (7); and in brown
adipose tissue, the enzyme is switched on during cold adaptation (8).
In white adipose tissue, LPL activity changes during the day according
to the nutritional state. This appears to be mediated by
posttranscriptional mechanisms. During short term fasting, LPL activity
in rat adipose tissue decreases without corresponding changes in the
levels of mRNA and protein mass, thereby reducing the specific
activity (activity/protein mass ratio) (18, 20-22). We have found that
this occurs because the distribution of lipase protein shifts toward an
inactive form (9) and that refeeding for 4 h can restore the
suppressed activity (10). The signal and mechanism for these changes in
the activity status of the enzyme are unknown.
To delineate the regulatory mechanism, we determined the turnover rates
for LPL mRNA, mass, and activity in rat adipose tissue in the fed
and fasted states and explored whether the regulation during feeding,
fasting, and refeeding requires synthesis of new mRNA or protein.
The results point to a novel mechanism and a new perspective on the
nutritional regulation of LPL in adipose tissue.
Animals--
Male Sprague-Dawley rats (23 days old) weighing
around 60 g were bought from Möllegaard Breeding Center
(Ejby, Denmark). After transport to Umeå they were allowed to
acclimatize for 7-10 days; during this time, they reached a weight of
~120 g. The rats were kept in a well ventilated room at 21 °C and
40-50% humidity and had free access to standard laboratory chow
(Laktamin AB, Stockholm, Sweden) and tap water. The light in the room
was on between 6 a.m. and 6 p.m. In the fasting experiments,
food was withdrawn from the cages at 6 a.m., and a grid was placed
at the bottom of the cages to prevent coprophagia. In the refeeding
experiments, the rats were put back on standard chow at 6 a.m.
after a 24 h fast, and were killed at 12 noon by cervical
dislocation. The adipose depot used in all experiments was
periepididymal adipose tissue. The animal ethics committee in Umeå
approved all animal experiments.
Materials--
Actinomycin-D, cycloheximide, bovine serum
albumin, aprotinin (Trasylol), and HEPES were from Sigma.
Leupeptin and pepstatin were from the Peptide Institute (Osaka, Japan).
Heparin was from Lövens (Malmö, Sweden). The substrate for
the LPL activity assay was 3H-labeled triolein in
Intralipid (10%) from Amersham Biosciences, Inc. Parker medium (Parker
199) was from SBL (Stockholm, Sweden). All other reagents were of the
highest commercial grade possible. Actinomycin and cycloheximide were
dissolved in 0.9% NaCl (saline) and injected intraperitoneally at
concentrations of 2 and 35 mg/kg body weight, respectively, unless
otherwise stated. The injected volume was 0.3 ml.
LPL Assays--
LPL was extracted from tissues by homogenization
in a Tris-HCl buffer (pH 8.2) containing detergents and protease
inhibitors (9). The homogenate was centrifuged for 15 min at 3000 rpm, after which the intermediate phase (between the floating fat droplets and the pellet) for adipose tissue and the supernatant for other tissues was used for assay of LPL activity and immunoreactivity.
LPL activity was measured as described previously (9). Briefly, 4 µl
of tissue homogenate (duplicate samples) was incubated for 60 min at
25 °C with substrate in the presence of 10 µl of heat-inactivated
serum from fasted rats (as source of apolipoprotein CII) and 6% bovine
serum albumin. The total volume was 200 µl. After termination of
lipolysis the fatty acids were extracted and counted for radioactivity.
One milliunit of lipase activity represents 1 nmol of fatty
acids released per minute.
LPL immunoreactivity was measured with a sandwich enzyme-linked
immunoadsorbent assay as described (9). Briefly, three different
dilutions of tissue homogenate were incubated in microtiter plate wells
previously coated with affinity-purified chicken anti-LPL IgG.
Detection was mediated via the 5D2 monoclonal antibody (from Dr. John
Brunzell, Seattle, WA) followed by a peroxidase-labeled anti-mouse IgG
antibody. Absorbency at 490 nm was measured with a Spectramax
microplate spectrophotometer (Molecular Devices, Sunnyvale, CA).
LPL mRNA was quantified as described (10) with a ribonuclease
protection solution hybridization assay modified from Durnam and
Palmiter (11). A 32P-labeled LPL cRNA probe synthesized
from a linearized pGEM4z plasmid was incubated for 40 h with total
nucleic acid samples from rat adipose tissue. Three different dilutions
of each sample were assayed. The samples were precipitated, collected
on Whatman filters, and counted for radioactivity. The values were
compared with a standard curve and expressed relative to the amount of DNA in the sample. DNA was measured by fluorometry as described by
Labarca and Paigen (12).
Active and inactive forms of LPL in tissue homogenates were separated
on heparin-Sepharose columns (9). The columns were eluted with a salt
gradient, and the fractions were assayed for LPL activity and
immunoreactive mass.
Hepatic lipase in rat postheparin plasma was measured as described
(13). The substrate was 3H-labeled triolein incorporated
into an olive oil/gum arabic emulsion by sonication. LPL present in the
plasma was inhibited by a high salt concentration.
Statistics--
Statistics were performed by one-way analysis of
variance. In some cases, the Bonferroni posthoc test for multiple
comparisons was used. The SPSS program for Windows was used (SPSS Inc.,
Chicago, IL).
Up-regulation of LPL Activity on Refeeding Requires Synthesis of
New Protein--
Fasting for 24 h reduced LPL activity to
25% of fed control (p < 0.001), whereas LPL
protein mass decreased only to 83% (p < 0.05) (Table
I). After refeeding for 6 h, LPL
activity had increased 4.3-fold to 107% of fed control, but LPL
protein mass remained unchanged. In rats that had been given
cycloheximide to inhibit protein synthesis, both LPL activity and
protein mass dropped sharply despite refeeding (Table I). These data
indicate that LPL protein is turned over rapidly and that the
up-regulation of LPL during refeeding requires synthesis of new
protein.
To further analyze the turnover of LPL we studied fed rats, which have
high LPL activity in their adipose tissue (Fig.
1). LPL activity and protein mass dropped
to 40-50% of control within 2 h after the administration of
cycloheximide and then decreased more slowly, reaching 20% of control
at 6 h. These data demonstrate that after the block of protein
synthesis by cycloheximide, the half-lives of LPL activity and protein
mass in adipose tissue are less than 2 h and that LPL activity
decreases as a result of protein turnover and not because the enzyme
protein loses its catalytic activity.
Down-regulation of LPL Activity on Fasting, but Not Up-regulation
on Refeeding, Requires Synthesis of New mRNA--
In these
experiments, we used actinomycin-D, which inhibits
DNA-dependent mRNA synthesis. When 24-h fasted rats
were injected with actinomycin and then refed, LPL activity increased
to the same level as in fed rats (Table I). LPL protein mass did not change significantly. Hence, up-regulation of LPL activity during refeeding does not require synthesis of new mRNA. Next, we
determined whether down-regulation of LPL activity during fasting
requires synthesis of new mRNA. Fed rats were injected with
actinomycin or saline, and food was removed from the cages (Fig.
2). Eighteen h later, LPL-specific
activity in adipose tissue from control rats (saline-injected) had
decreased, as expected, to 30% of fed control. Surprisingly, in
adipose tissue from actinomycin-injected rats, LPL-specific activity
was slightly increased (140% of fed, p < 0.05). These
findings show that the down-regulation of LPL-specific activity during
fasting requires synthesis of new mRNA and suggest that, during
fasting, a gene is switched on whose product prevents LPL from becoming
active even though synthesis of LPL protein continues unabated. We
predicted that if we injected actinomycin into 24-h fasted rats with
low adipose tissue LPL activity, we would turn off this proposed
inhibitory gene, allowing active LPL to be formed again. Our prediction
was upheld; 6 h after injection of actinomycin into fasted rats,
LPL activity in adipose tissue had increased almost 4-fold without
refeeding (Table I), with no statistically significant change in LPL
protein mass. These data indicate that turning off transcription with
actinomycin could reproduce the signal that causes up-regulation of LPL
activity on refeeding.
To test the possibility that the increase in LPL activity by
actinomycin might be caused by a paradoxical effect on the LPL protein
by the actinomycin molecule itself, we performed two control experiments. First, we determined whether actinomycin affected LPL
activity when added to tissue homogenates in vitro. For
this, actinomycin was added at concentrations of 5, 10, 50, and 100 µg/ml either to homogenates of adipose tissue from fasted rats before
assay of LPL activity or directly to the activity assay medium.
In vitro addition of actinomycin had no effect on LPL activity (data not shown). Second, we performed experiments with another inhibitor of DNA-dependent RNA synthesis,
The Effect of Actinomycin on LPL Activity in Adipose Tissue Is
Blunted after Prolonged Fasting--
Previously, we showed that after
24 h of fasting, LPL activity in adipose tissue is reduced, but
the level of LPL mRNA remains the same as in the fed state;
however, after 60 h of fasting, the mRNA level decreases
significantly to less than 50% of fed control (10). At this point, the
effect of refeeding is blunted. In the following experiment, we tested
whether the effect of actinomycin was similarly blunted after prolonged
fasting. When rats were fasted for 60 h, LPL activity was greatly
reduced (to 7.2% of fed control (Fig.
3)). When these rats were given
actinomycin, the increase in LPL activity after 6 h was very
modest (from 7.2 to 26% of the level in fed rats). This indicates that
the magnitude of the effect of actinomycin on adipose tissue LPL
activity depends on the level of LPL mRNA.
Dose Response of Actinomycin--
A survey of the literature
indicated that the most frequently used dose for actinomycin in
vivo is 2 mg/kg body weight. In a dose-response experiment, LPL
activity in adipose tissue increased from 1.16 ± 0.08 milliunit/µg DNA (fasted control, injected with vehicle) to 2.48 ± 0.29 milliunit/µg DNA with as little as 0.5 mg/kg 6 h after
injection (p < 0.001). With a dose of 2 mg/kg, LPL
activity reached 4.47 ± 0.01 milliunit/µg DNA. A further
increase in the dose to 6 mg/kg did not result in an additional
increase in LPL activity (p > 0.05). Hence, a
dose of 2 mg/kg was used in subsequent experiments.
Time Course of the Effect of Actinomycin in Rat Adipose
Tissue--
LPL activity in adipose tissue of 24 h fasted rats
was 21% of that in fed rats (Fig. 4). By
4 h after administration of actinomycin, the activity had
increased to 51% of fed control, and by 6 h the activity was
restored (97%). There was no further significant change through
16 h (114%). In this experiment, in the fed and fasted states and
for 16 h after actinomycin administration, LPL protein mass did
not change significantly. In a separate experiment, LPL mRNA was
measured in the adipose tissue at 0, 6, 16, and 24 h after
actinomycin administration. The level of LPL mRNA was 68.4 ± 11.1 and 72.7 ± 9.2 amol/µg DNA in fed and 24 h
fasted rats, respectively (Fig. 5). After
injection of actinomycin the LPL mRNA level decreased
monoexponentially. The k values for the best-fit exponential
function (n = N0 × e Minor Effects of Actinomycin on LPL Activity in Other
Tissues--
Six h after the administration of actinomycin to fasted
rats, LPL activity increased slightly and inconsistently in lung, kidney, liver, and spleen. In soleus muscle and in heart, which like
adipose tissue express high levels of LPL, LPL activity increased 1.5- and 1.6-fold, respectively (p < 0.01) compared with
saline-injected controls. These changes were not accompanied by changes
in LPL mass. The major increase in LPL activity in adipose tissue and the minor increases in some other tissues after actinomycin resulted in
a 4.7-fold increase in LPL activity released to the circulating blood
10 min after a heparin injection. LPL activity in preheparin plasma
increased 2-fold (p < 0.001). There were no
statistically significant changes in hepatic lipase activity as
measured in liver homogenate or in postheparin plasma (data not shown).
Actinomycin Changes the Ratio between Inactive and Active Forms of
LPL--
Previously, we showed that there are two forms of LPL protein
in tissues that can be separated by heparin-Sepharose columns. In the
fasted state, the inactive form with low heparin affinity predominates.
Upon refeeding, the distribution of lipase protein shifts from the
inactive toward the active form (9), which has a high affinity for
heparin. To further test whether actinomycin had an effect similar to
that of refeeding, three rats were fasted for 24 h and then
injected with actinomycin. Six h later, epididymal adipose tissue
pieces were collected and homogenized, and the LPL protein was
separated on heparin-Sepharose. Fig. 6.
shows that in actinomycin-treated rats (Fig. 6A), most of
the enzyme protein was in the second peak, which corresponds to the
active form, whereas in the fasted rats, the first peak predominated (Fig. 6B). The ratios between the two peaks
(inactive/active) were 0.38 in the actinomycin-treated rats and 2.27 in
the fasted rats. Normal values for the peak ratios are 0.46 ± 0.04 and 2.34 ± 0.13 for fed and fasted rats, respectively (9).
These data show that LPL in adipose tissue from fasted rats injected
with actinomycin is present mainly in the active form, similar to LPL in adipose tissue from fed rats.
The Effect of Actinomycin Is Blunted in Aging Rats--
We have
previously shown that the mechanism that channels LPL toward the
inactive form on fasting is blunted in adipose tissue from aging, obese
rats (14). If actinomycin interferes with the same mechanism, its
effect should also be blunted in aging rats. To test this hypothesis,
rats weighing 505 ± 6 g were fasted for 24 h and then
injected with actinomycin (Fig. 7). In
response to actinomycin, LPL activity increased to 149% of
saline-injected control in 6 h (p < 0.01). This
was in sharp contrast to the young rats (126 ± 2 g), where
LPL activity was up-regulated to 485% of control (p < 0.001). These data show that the response of adipose tissue LPL to
actinomycin is blunted in aging rats.
This study shows that in fasting rats, a gene is switched on in
adipose tissue that makes the tissue produce an inactive form of LPL.
Inhibition of mRNA synthesis by actinomycin completely blocked the
down-regulation of LPL activity in adipose tissue during fasting.
Administration of actinomycin or One potential explanation for our results is that actinomycin
administered in vivo changes the levels of a circulating
hormone or changes nerve signaling activity to the adipose tissue and that the effect on LPL activity is secondary. Studies from the 1960s
indicate that this is not the case. In these studies, actinomycin caused a dramatic increase in LPL activity in whole fat pads from fasted rats incubated ex vivo (15, 16). This clearly
indicates that the effect of actinomycin is a direct action in the
adipose tissue, rather than secondary to changes in nerve signaling or in circulating hormones.
Several studies have shown that N-linked glycosylation and
proper processing of the glycan chains are important steps in the formation of active, secretable LPL with high heparin affinity (1,
17-21). Specifically, the trimming of glucose residues by glucosidases
in the endoplasmic reticulum seems to be a crucial step for the
attainment of activity (19-21). Glycosylated proteins that have been
processed in the cis-Golgi have glycan chains that are
resistant to cleavage by the enzyme endoglycosidase-H (Endo-H). Doolittle et al. showed that the Endo-H-resistant form of
the LPL protein predominates in adipose tissue of fed rats, whereas the
Endo-H-sensitive form predominates in adipose tissue of fasted rats
(18). We have found that the catalytically active form of LPL, purified
on heparin-Sepharose, is mainly resistant to Endo-H, whereas the
inactive form is
Endo-H-sensitive.2 These data
suggest that the mechanism for down-regulation of LPL during fasting
affects the intracellular processing or trafficking of newly
synthesized LPL, probably in the endoplasmic reticulum or early Golgi.
Further evidence for a specific mechanism for processing of the enzyme
comes from studies on mice affected by the combined lipase deficiency
mutation. LPL in adipocytes from these mice is retained in the
endoplasmic reticulum in an inactive form with glycan chains that are
sensitive to Endo-H (22, 23). An interesting possibility is that this
genetic defect is related to the mechanism that down-regulates LPL on fasting.
By injecting cycloheximide to inhibit protein synthesis, we could
follow the turnover of the existing LPL molecules. LPL activity and
mass in adipose tissue from both fed and fasted rats decreased rapidly
and in parallel, with a half-life of less than 2 h. This means
that turnover of LPL activity is directly associated with turnover of
LPL protein. There are two possible pathways for this turnover: LPL
protein may be degraded within the adipose tissue or the enzyme may be
transported with blood for degradation in the liver (24, 25).
The turnover of LPL mRNA seems to occur slowly under most
conditions. During long term fasting the half-life has been reported to
be more than 24 h in white adipose tissue (10) and 40 h in brown adipose tissue (26). During weight loss in obese Zucker rats (27)
and during improved diabetes control in humans (28), LPL mRNA
turnover was also found to be slow. In the present study, the half-life
of LPL mRNA was 13.3 h in the fed state. During cold
adaptation in rat brown adipose tissue, LPL activity increases significantly, mediated by increased transcription of the LPL gene;
upon return to warm conditions, a specific RNA-degrading enzyme is
induced that accelerates the turnover of LPL mRNA (26). Most likely
this mechanism exists also in white adipose tissue since tumor necrosis
factor Catecholamines exert a strong effect on lipid homeostasis in adipose
tissue by increasing hormone-sensitive lipase activity and by
decreasing LPL activity. In an elegant study, Ranganathan et
al. showed that the effect of epinephrine on LPL in cultured adipocytes is mediated by a protein that binds to the LPL transcript and effectively blocks its translation (30). This raises the question
whether the same RNA-binding protein causes the down-regulation of LPL
activity on fasting. If this were true, the positive effect of
actinomycin on LPL activity could be to block the transcription of this
protein. Three lines of evidence indicate that this is not the case.
First, most studies indicate that the mechanism for down-regulation of
LPL during short term fasting is posttranslational and that the levels
of LPL protein change very little (9, 18, 20, 22). If a block in LPL
synthesis mediated the decrease in LPL activity on fasting there would
have to be an associated block in LPL degradation. The present study
shows that this is clearly not the case; the turnover of LPL protein
was the same in the fed and in the fasted states. Second, Wing et
al. observed an increase in LPL activity in rat fat pads incubated
in the presence of actinomycin (16). This effect was blocked by
epinephrine, most likely by inducing the LPL mRNA-binding protein.
We have preliminary evidence that this occurs also in vivo.
The increase in LPL activity in adipose tissue after actinomycin
administration was attenuated when rats were given epinephrine, which
also caused a reduction in LPL protein mass.2 This
indicates that the RNA-binding protein is activated
posttranscriptionally by epinephrine, since actinomycin would inhibit
synthesis of its mRNA. Third, it is unlikely that a translational
inhibition of LPL followed by a decreased degradation would lead to a
change in the structure of glycan chains in the remaining LPL molecules.
The nutritional regulation of LPL in adipose tissue has been viewed as
having a default state characterized by a low, basal LPL activity that
can be temporarily up-regulated after meals. Our findings in this study
suggest another perspective on the regulation: the default (fed) state
is characterized by a high LPL activity and mass synthesized from a
stable mRNA where the newly synthesized LPL is processed mainly
into the active form. The enzyme is then secreted and transported to
nearby capillaries where it acts on lipoproteins. This pathway seems to
predominate in most tissues that synthesize LPL (e.g., heart
and skeletal muscle). During periods of caloric restriction
(i.e., between meals or during fasting), LPL mRNA and
protein mass remain high; however, LPL activity in adipose tissue can
be suppressed by the induction of a short-lived gene product that
causes newly synthesized LPL to be channeled into an inactive form.
Refeeding or administration of actinomycin inhibits the expression of
this putative factor, allowing active LPL to be formed.
Why is there a need to down-regulate LPL during fasting? The action of
adipose LPL on circulating triglycerides results in the generation of
fatty acids that can either be taken up by the tissue or be released
into the blood in albumin-bound form. The ratio between these two
pathways varies greatly in human adipose tissue (31), from
predominantly storage after a large meal to predominantly release into
the circulating blood during fasting. Irrespective of the fate of the
generated fatty acids, the down-regulation of LPL during fasting will
decrease the hydrolysis of circulating triglycerides that pass through
the adipose tissue. Failure to down-regulate LPL could contribute to
the excessive generation of albumin-bound fatty acids seen in
individuals with insulin resistance, or it could contribute to an
increased deposition of fat in adipose tissue. Consistent with this
reasoning, Ong et al. found that LPL-specific activity in
adipose tissue during fasting was higher in obese subjects than in lean
controls (32). Furthermore, in obese subjects, LPL-specific activity
was unresponsive to a meal (refeeding). Our findings suggest that this
apparent unresponsiveness to a meal may in fact reflect that LPL
activity in these subjects was not down-regulated during the fasting
period. If so, this would be similar to what we have found in aging,
obese rats where LPL-specific activity failed to be down-regulated on fasting (14). This raises the intriguing possibility that switching on
and off the gene that regulates LPL activity in adipose tissue may be
deranged in obesity, insulin resistance, and related metabolic disorders.
We are indebted to Ann-Sofi Jakobsson for
excellent technical assistance.
*
This study was funded by the Swedish Medical Research
Council Grant K98-03X-00727-33C.The costs of publication of this
article were defrayed in part by the
payment of page charges. The article must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
Present address: Gladstone Institute of Cardiovascular Disease,
University of California, San Francisco, CA 94141-9100.
¶
To whom correspondence should be addressed. Tel.:
46-90-786-52-34; Fax: 46-90-786-78-40; E-mail:
Thomas.Olivecrona@medkem.umu.se.
Published, JBC Papers in Press, January 24, 2002, DOI 10.1074/jbc.M200325200
2
M. Bergö, G. Wu, T. Ruge, and T. Olivecrona, unpublished observations.
The abbreviation used is:
LPL, lipoprotein
lipase.
Down-regulation of Adipose Tissue Lipoprotein Lipase during
Fasting Requires That a Gene, Separate from the Lipase Gene, Is
Switched On*
§,,
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
-amanitin,
another inhibitor of transcription. The response to actinomycin was
much less pronounced in aging rats, which are obese and
insulin-resistant. These data suggest a default state where LPL protein
is synthesized on a relatively stable mRNA and is processed into
its active form. During fasting, a gene is switched on whose product
prevents the enzyme from becoming active even though synthesis of LPL
protein continues unabated.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
MATERIALS AND METHODS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
RESULTS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
Effect of nutritional state on LPL activity and mass in rat adipose
tissue during inhibition of transcription and/or translation
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Fig. 1.
Time course of the effect of cycloheximide on
LPL in rat adipose tissue. Fed rats were injected with
cycloheximide. At 2, 4, and 6 h, three rats were killed, and
epididymal adipose tissue was taken for assay of LPL activity ( 
) and
mass (
). Data are expressed as milliunit or ng LPL per µg of DNA
as percent of the value at time zero (means ± S.E.,
n = 3). The control (100%) values for LPL activity and
mass in adipose tissue from fed rats were 4.51 ± 0.17 milliunit/µg DNA and 13.9 ± 1.10 ng/µg DNA,
respectively.
View larger version (8K):
[in a new window]
Fig. 2.
Effect of fasting on LPL-specific activity in
the presence of the mRNA synthesis inhibitor actinomycin. At
6 a.m. the first morning, five fed rats were killed, five were
injected with actinomycin, and five were injected with saline. The
injected rats were then fasted for 18 h and killed at 12 midnight.
Epididymal adipose tissue was taken for measurement of LPL activity and
mass. Data are expressed as activity/mass ratio (LPL-specific activity,
milliunit/ng).
-amanitin. Three groups of rats were fasted for 24 h. Then, one
group was given free access to food (refed), one was injected with
-amanitin (3 mg/kg body weight in saline), and one was injected with
saline only (fasted controls). Six h later, the rats were killed, and adipose tissue LPL activity and protein mass were determined. LPL-specific activity (milliunit/mg) in adipose tissue increased from
0.14 in the fasted group to 0.40 in the refed group as expected on
refeeding. In the -amanitin-treated group, LPL specific activity also increased (0.35 milliunit/mg, p < 0.001 versus fasted controls, data not shown). These results
indicate that the effect of actinomycin on LPL activity in adipose
tissue was not a spurious finding; it could be reproduced with an
unrelated inhibitor of transcription, -amanitin.
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Fig. 3.
Effect of actinomycin on LPL in adipose
tissue from rats fasted for 60 h. Rats were fasted for 24 and
60 h, injected with actinomycin, and sacrificed 6 and 12 h
later. Epididymal adipose tissue was taken for subsequent measurement
of LPL activity. Data are expressed as milliunit/µg DNA (means ± S.E., n = 4).
k ×
t) were 0.052 ± 0.013 h1 and
0.041 ± 0.012 h1 for the fed and fasted states,
respectively. This corresponds to half-lives of 13.3 h and
16.8 h (p > 0.05).
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Fig. 4.
Time course of the effect of actinomycin on
LPL activity and mass in adipose tissue from fasted rats. Groups
of rats were fasted for 24 h and injected with actinomycin. At 4, 6, 10, and 16 h, rats were killed by decapitation, and epididymal
adipose tissue was taken for measurement of LPL activity ( ) and mass
(). Data were calculated as milliunit or ng LPL/µg DNA and are
expressed as percent of fed (means ± S.E., n = 5).
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Fig. 5.
Turnover of LPL mRNA in adipose tissue
from rats following injection of actinomycin. Fed ( ) and
24 h fasted (
) rats were injected with actinomycin. At 0, 6, 16, and 24 h, three or four rats were killed by decapitation, and
epididymal adipose tissue was taken for measurement of LPL mRNA as
described under "Materials and Methods." Data are expressed as amol
LPL mRNA/µg DNA.
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Fig. 6.
Effect of actinomycin on the relation between
inactive and active LPL in adipose tissue. Three rats were fasted
for 24 h and injected with actinomycin. Six h later, adipose
tissue was taken and prepared as described under "Materials and
Methods." The homogenates were pooled and applied to a
heparin-Sepharose column (A). For comparison, pooled
homogenates from three 24-h fasted rats were also separated on
heparin-Sepharose (B). LPL protein was eluted with a salt
gradient, and the fractions were assayed for LPL activity ( ) and
mass ().
View larger version (14K):
[in a new window]
Fig. 7.
Effect of actinomycin on LPL in adipose
tissue from aging rats. Old rats weighing 505 ± 6 g
were fasted for 24 h and injected with actinomycin
(Act-D) or saline. Six h later, epididymal adipose tissue
was taken for measurement of LPL activity. The same procedure was
performed in young rats weighing 126 ± 2 g. Data were
calculated as milliunit/µg DNA and are expressed as percent of
corresponding saline-injected rats (means ± S.E.,
n = 5).
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
-amanitin, another inhibitor of
transcription, to fasted rats completely restored LPL activity within
6 h.
can accelerate the breakdown of LPL mRNA (29). However,
this mechanism does not seem to act during fasting since the turnover
of LPL mRNA did not change (half-life = 16.8 h). For this
reason, mRNA was available for continuous synthesis of LPL protein
even after the animals had been given actinomycin. With such a stable
mRNA, it is not possible for the cell to rapidly regulate LPL
activity on a transcriptional level. Instead, the regulation must be
mediated on the translational or posttranslational level.
ACKNOWLEDGEMENT
FOOTNOTES
Both authors contributed equally to this work.
ABBREVIATIONS
REFERENCES
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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