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1 Pennington Biomedical
Research Center, Recent reports have demonstrated that
conjugated linoleic acid (CLA) has effects on body fat accumulation. In
our previous work, CLA reduced body fat accumulation in mice fed either
a high-fat or low-fat diet. Although CLA feeding reduced energy intake,
the results suggested that some of the metabolic effects were not a
consequence of the reduced food intake. We therefore undertook a study
to determine a dose of CLA that would have effects on body composition
without affecting energy intake. Five doses of CLA (0.0, 0.25, 0.50, 0.75, and 1.0% by weight) were studied in AKR/J male mice
(n = 12/group; age, 39 days)
maintained on a high-fat diet (%fat 45 kcal). Energy intake was not
suppressed by any CLA dose. Body fat was significantly lower in the
0.50, 0.75, and 1.0% CLA groups compared with controls. The
retroperitoneal depot was most sensitive to the effects of CLA, whereas
the epididymal depot was relatively resistant. Higher doses of CLA also
significantly increased carcass protein content. A time-course study of
the effects of 1% CLA on body composition showed reductions in fat pad
weights within 2 wk and continued throughout 12 wk of CLA feeding. In
conclusion, CLA feeding produces a rapid, marked decrease in fat
accumulation, and an increase in protein accumulation, at relatively
low doses without any major effects on food intake.
body composition; insulin; obesity; fatty acids
CONJUGATED LINOLEIC ACID (CLA) is a group of dienoic
derivatives of linoleic acid produced by bacteria in the ruminant gut (4). These CLA's are then absorbed and incorporated in lipid stores.
The anticarcinogenic effects of CLA have been studied for some time (9,
10). More recently, CLA has been shown to reduce body fat in mice (18),
as well as rats and chickens (17). In our previous study of the effects
of CLA in mice, there was a reduction in food intake associated with
CLA feeding (24). To better understand the effects of CLA on body fat
accumulation, we extended our studies by determining if a dose of CLA
would reduce body fat without affecting food intake. Additionally, we determined the time course of the effects of CLA on body fat in the mouse.
Male AKR/J mice were obtained from the Jackson Laboratory (Bar Harbor,
ME) at ~4 wk of age. All mice were housed individually in hanging
stainless steel cages with an automatic watering system in a room
maintained at 26 ± 2°C with a 12:12-h light-dark cycle. Initially, the mice were fed ad libitum Purina Mouse Chow (diet no.
5015; Ralston Purina) and then were switched to a high-fat diet (diet
no. D12290, %fat 45 kcal; Research Diets) 10 days before being
randomly assigned to treatment diets. This period of adaptation to the
high-fat diet was used in both studies described here to minimize the
effect of high-fat diet-induced hyperphagia in the treatment groups at
study initiation.
Two studies were conducted. In the dose-response study, 60 6-wk-old
mice were randomly assigned to five treatment groups
(n = 12/group) for feeding varied
doses of CLA (0% control and 0.25, 0.50, 0.75, and 1.0% CLA by
weight) in a high-fat diet (%fat 45 kcal). CLA was obtained from Nu
Chek Prep (Elysia, MN), and the reported isomer content was as follows:
39.1% cis9,trans11 CLA and
trans9,cis11 CLA; 40.7%
trans10,cis12 CLA and 1.8%
cis9,cis11 CLA; 1.3%
cis10,cis12 CLA; 1.9%
trans9,trans11 and
trans10,trans12 CLA; 1.1%
cis9,cis12 linoleic acid; and 14.1%
remainder. The 45-kcal fat diets were formulated by
Research Diets (New Brunswick, NJ), and the CLA-containing diets were
prepared by replacing corn oil with CLA (Table 1). Mice
were provided ad libitum access to a preweighed portion of the defined
diets in pellet form placed on the bottom of each cage, with fresh
preweighed diet given at each weighing. The animals and remaining diet
were weighed three times each week (Monday, Wednesday, and Friday).
Food intake was corrected for spillage, and all measurements were to
the nearest 0.1 g. Measurements were recorded 7 days before the start
of experimental diet feeding and continued throughout the 39 days of
CLA feeding.
ABSTRACT
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
INTRODUCTION
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
METHODS
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
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Table 1.
Diet composition
At the end of the study, after a 3-h fast, the mice were killed by cervical dislocation and decapitated. Truncal blood was collected, and plasma was frozen for later measurement of insulin and leptin by RIA (Linco Research, St. Louis, MO). Plasma glucose was measured in the control and 1.0% CLA groups by a colorimetric hexokinase glucose assay (Sigma Diagnostics, St. Louis, MO). Carcasses were dissected, and the following organs were removed and weighed: liver, spleen, left and right kidney, left and right testis, and heart. Similarly, the left and right inguinal, left and right epididymal, left and right retroperitoneal, and the mesenteric adipose depots were removed and weighed to the nearest 0.0001 g. The eviscerated carcass, which included all removed tissues except the left epididymal adipose depot, left testis, liver, spleen, and heart, was weighed and then frozen in liquid nitrogen for later body composition analysis.
The liver and spleen of control and 1% CLA groups were sectioned and fixed in 10% Formalin or glutaraldehyde for histopathological examination by light microscopy and transmission electron microscopy. Histopathological analysis was performed by two separate laboratories [the Pathology Department at the Louisianna State University Veterinary School of Medicine (Baton Rouge, LA) and the Experimental Pathology Laboratories (Herndon, VA)].
The frozen eviscerated carcasses were homogenized in 3 vol of distilled water using a Polytron (PRO300D PRO; Scientific). Homogenates were dried to constant weight in a 70°C oven and then finely ground and mixed thoroughly using a mortar and pestle. The final product was analyzed in triplicate for lipid, protein, and ash content. Lipid was analyzed using a Soxtec System HT 1043 Extraction unit using 2:1 chloroform-methanol, protein with a Perkin-Elmer Series II Nitrogen Analyzer 2410, and ash by a CEM MAS 7000 Microwave Muffle Furnace. Water content of the carcass was calculated by subtracting the dried carcass weight from the original weight of the eviscerated carcass.
An adiposity index was calculated by dividing the summed weight of the seven excised adipose depots by the weight of the eviscerated carcass (which includes all organs but without the gastrointestinal tract and the 7 adipose depots). The adiposity index has been shown to be highly correlated with lipid content assayed chemically (r > 0.97; see Ref. 26).
In the time-course study, 80 6-wk-old mice were used. Due to the large number of animals, the study was divided into two cohorts of 40 (20 control, 20 treatment) with a staggered start of 4 wk. A total of 40 mice were used as controls and were fed an unadulterated high-fat diet, whereas 40 treatment animals were fed the high-fat diet containing 1% CLA. The 1% dose used in the previous study was chosen for its effect on body composition and lack of effect on energy intake. The diets were formulated by the same company with the same ingredient mixture as that used in the dose-response study. Measurements of food intake and body weight were taken two times per week (Tuesday and Friday) using the same protocol as described in the above study.
Eight animals from the control group and eight from the treatment group were killed after 2, 4, 6, 8, and 12 wk of CLA treatment. After a 3-h fast, the mice were anesthetized using halothane, and blood was collected by heart puncture. Mice were then euthanized by cervical dislocation. Carcasses were dissected as described in the dose-response study. As in the dose-response study, seven adipose depots were excised and weighed, and an adiposity index was calculated. Livers and spleens were fixed for histopathological examination, and carcasses were analyzed for composition at the 12-wk time point only. Plasma insulin and leptin were measured at all time points, whereas glucose was measured in the control and treatment group for the 12-wk time point only.
Statistical evaluation for differences among group means was performed by an ANOVA. If a main effect was observed, post hoc comparisons using a Tukey-Kramer adjustment were made. A Wilcoxon rank sum test was used to determine differences in liver lipid accumulation. For the time-course study, repeated measures were performed with respect to time using a covariance structure. All data are presented as means ± SE.
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RESULTS |
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ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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Dose-response study. There was a
significant main effect of CLA on body weight
(P < 0.05), an effect of CLA over
time (P < 0.01), and a significant
interaction between the two (P < 0.01; Fig. 1). When compared with the controls, body
weight was significantly lower at day
18 in the 0.75% CLA group and day
21 in the 1.0% CLA group
(P < 0.05) and remained lower
throughout the remainder of the study. Energy intake was not
significantly different from control except in the 0.25% CLA group,
which was slightly increased relative to the control diet and other CLA
doses (P < 0.05; Fig. 2).
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At the end of treatment, there was a dose-dependent effect of CLA on
all adipose depots relative to the controls (Fig.
3). The adipose depot most sensitive to the
effects of CLA was the retroperitoneal, with a significant reduction in
depot weight observed at 0.50, 0.75, and 1.0% CLA
(P < 0.01 for all comparisons). The
inguinal, epididymal, and mesenteric adipose depots showed a
significant difference at the 0.75 and 1.0% doses
(P < 0.05).
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Body composition data and calculated adiposity index supported the
adipose depot weight data for the effect of CLA to reduce body fat
(Table 2). When data were expressed as
percent of eviscerated carcass, body lipid content was significantly
reduced at the 0.50, 0.75, (P < 0.05), and 1.0% (P < 0.01) CLA
dose. Carcass lipid content (g) showed a significant decrease at the
0.75 and 1.0% CLA doses and was nearly significant at the 0.5% CLA
dose (P < 0.053). All comparisons
were made relative to the controls. Correspondingly, reductions in the
adiposity index were observed for the 0.75 and 1.0% CLA doses relative
to controls (P < 0.01). There was a
trend for increased percent body protein content with higher doses of CLA, which was significant at the 1.0% dose
(P < 0.01) compared with controls.
Carcass ash content was not affected by CLA treatment.
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Mice fed CLA tended to have enlarged spleens and livers, but this
effect was not significant except at the highest dose of CLA
(P < 0.01 for both organs; Table 2).
CLA treatment had no effect on the weight of the kidneys, testes, or
heart (Table 2). Liver samples were analyzed by two veterinary
pathologists in two separate laboratories. One laboratory reported
minimal to moderate cytoplasmic vacuolization typical of lipid
accumulation, which was higher (P < 0.01) in the 1% CLA group compared with the control group (Table
3). The other laboratory reported that histopathological
examination of hepatic tissue showed mild to moderate cytoplasmic
vacuolization consistent with the presence of intracellular glycogen.
In addition, larger, clear, round vacuoles consistent with the presence
of intracellular lipid deposits were present. However, there were no
morphological features identified by light and transmission electron
microscopy that distinguished the liver samples from the 1.0% CLA
treatment and the controls. Spleens were only mildly affected by
lymphoid hyperplasia (lipid deposit), and no difference in the degree
of severity was evident between the 1.0% CLA and control groups.
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Plasma leptin levels tended to decrease with the higher CLA doses, but
there were no significant differences (Fig.
4A).
In contrast, plasma insulin showed increased levels with higher doses of CLA (Fig. 4B), becoming
significant from control in the 1.0% group
(P < 0.05). Plasma insulin
levels in the control group (4.76 ± 2.02 ng/ml) were
similar to that observed previously in AKR/J mice (3-4 ng/ml; see
Ref. 5). Plasma glucose levels were not significantly affected by CLA
treatment (145 ± 9 for controls and 153 ± 11 mg/dl for 1%
CLA).
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Time-course study. Body weight was
significantly reduced by day 22 of CLA
feeding compared with controls and remained lower throughout the 12 wk
of treatment (Fig. 5; P < 0.005). However, as the study progressed, the difference between
control and CLA treatment was diminished, particularly by 12 wk (Fig.
5). Cumulative energy intake was not affected by 12 wk of 1% CLA
treatment (Fig. 6).
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As found in the dose-response study, the adipose depot most sensitive
to CLA treatment was the retroperitoneal, with significant reductions
in weight at all time points (P < 0.005; Fig. 7A). The
inguinal and epididymal fat depots were significantly lower than
control at week 4 and through
week 12 of the study (Fig. 7,
B and
C). Mesenteric adipose depot weights
were reduced by CLA treatment, but the effects of CLA on this depot
were not apparent until week 6 (Fig.
7D).
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Liver weights were significantly higher in the 1% CLA group compared
with controls at each time point (P < 0.01; Fig. 8). CLA treatment had a tendency to
increase the weight of the spleen (Fig. 8), with a significant
difference observed at the 8-wk time point
(P < 0.01) but not at the 12-wk time
point (P < 0.09). Histopathological examination of control and 1% CLA livers and spleens at the 12-wk time
point confirmed the results in the dose-ranging study. Livers showed
mild (grade = 2) to moderate (grade = 3) centrilobular fatty change,
which was higher (P < 0.05) in
livers from the CLA group (2.75 ± 0.27) compared with controls
(1.67 ± 0.31). Splenic changes consisting of lymphoid
hyperplasia were similar in the control and CLA groups.
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Body composition analysis of the control and CLA-treated animals at the
12-wk time point showed that CLA had a significant effect on protein
and lipid content (P < 0.0001).
Whether expressed in grams or percent of eviscerated carcass, 1.0% CLA
treatment significantly decreased carcass lipid content compared with
controls (P < 0.0005; Table
4). In contrast, carcass protein was
significantly increased in the 1.0% CLA group
(P < 0.0005). There was also an indication that ash may be increased by CLA treatment when expressed as
percent of eviscerated carcass (P < 0.09; Table 4).
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Plasma insulin levels showed a tendency to increase in the CLA
treatment over time, becoming significantly different from controls at
the 8-wk time point (P < 0.05; Fig.
9A). Interestingly, levels of plasma leptin in the CLA-treated animals were significantly reduced at the 6-wk time point (P < 0.001) but were not different from control values at the 8- and 12-wk
time points. Plasma glucose levels were not significantly different
between CLA-treated and control animals at the 12-wk time point (207 ± 13 in controls vs. 223 ± 9 in CLA group).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
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The major findings of the current studies are that CLA feeding causes a reduction in body fat accumulation, as well as an increase in body protein accumulation in male mice (AKR/J) at relatively low doses (0.5-1.0% CLA) and in as short a time as 2 wk at the 1% CLA dose. This confirms another study of the effects of 0.5% CLA in ICR female mice (18) and the findings of our previous study in male mice (24). In contrast to our previous report, there was no consistent suppression of food intake with the 1% CLA diet. We believe that the discrepancy regarding food intake between studies was due to differences in the experimental design. In the previous study, the novel high-fat diet was started at the same time as the CLA treatment. The interaction of the novel diet and CLA diet simultaneously could have led to a conditioned aversion (6) to the new diet if there were mild behavioral or central nervous system effects of the CLA. In the studies described in this report, an association between the novel taste of the diet and any central nervous system effects of CLA treatment were avoided by staging the presentations. The potential ability of CLA to condition a taste aversion should be explored further but was outside the scope of the present studies.
However, CLA may have an effect on food intake. The intake of the 0.25% CLA group was actually higher than the control group, there was a suggestion (P < 0.09) that the intake of the 0.75% CLA group was lower than controls (Fig. 2), and the cumulative intake of the 1% CLA group during the time-course study appeared to be lower at 8 wk (P < 0.08). In a 28-day study examining the effects of 0.5% CLA in female mice, food intake was significantly lower at two time points but was not significantly different at the end of the study (18). Although not reported in that study, it appears from the daily food intake reported in Fig. 2 that cumulative food intake would be lower over the 28-day study. However, in the current study, the cumulative intake of the 1% CLA group was nearly identical to that of the control group in both the dose-response study and by the end of the time-course study. We conclude that, although CLA may have a slight and transient effect on energy intake, the effect on body fat accumulation at the 0.5, 0.75, and 1.0% CLA doses was not due to a suppression of food intake. The significant increase of food intake by the 0.25% CLA dose is interesting and deserves further study.
There are several possible mechanisms for the reduced body fat accumulation in response to CLA feeding. We previously demonstrated that CLA feeding causes an increase in energy expenditure and an increase in fat oxidation (24). That CLA increases fat oxidation is also supported by increased carnitine palmitoyltransferease activity in fat pad, muscle, and liver of mice fed CLA (18). Another possibility is a reduction in triglyceride uptake and storage in adipose depots, since CLA has been shown to inhibit lipoprotein lipase activity in 3T3-L1 adipocytes (18).
As we previously reported, the response of fat pads from different sites to CLA feeding was varied, ranging from a 40% reduction in the retroperitoneal and mesenteric fat pads to a 22% decrease in the epididymal fat pad. The fat pads also responded rapidly to CLA treatment, with significant decreases observed in the retroperitoneal fat pad 2 wk after the start of CLA treatment, the inguinal and epididymal sites at 4 wk, and the mesenteric fat pad at 6 wk. Although the majority of the CLA effect was observed by 4-6 wk, the decrease in fat pads relative to controls was not a transient effect, as the differences were observed throughout the 12-wk time-course study. The time-course study further suggests that CLA treatment reduces the accumulation of carcass lipid but does not prevent it when mice are fed a high-fat diet.
The increases in liver and spleen weights observed in our previous study were replicated in the current studies. Histopathological examination indicated that much of the increase in liver weight was due to fat accumulation, consistent with another report examining the effect of CLA feeding on liver lipids (2). The increase in liver weight was not transient, as significant differences were observed throughout the 12-wk time-course study. There were no observable pathophysiological changes in the liver or spleen. A recent toxicological evaluation of CLA fed at 1.5% to Fischer 344 rats showed no treatment-related effects in 15 major organs (20).
The feeding of CLA in this study was associated with a paradoxical
increase in circulating insulin levels, suggesting that the animals
were becoming insulin resistant over time. This was observed by 6 wk of
feeding 1% CLA, and this hyperinsulinemia became even more pronounced
by 12 wk of treatment (Figs. 4 and 9). The results are paradoxical,
since a reduction in adipose mass, which was achieved by CLA treatment,
is usually associated with improved insulin sensitivity and decreased
plasma insulin levels (13). In addition, CLA has been shown to improve
glucose tolerance and insulin sensitivity in the Zucker obese fatty
rat, which has an early-onset massive obesity (8). Data from a reporter assay suggested that CLA may be acting as a weak PPAR
agonist, much
like troglitazone, which is an insulin-sensitizing agent (8). It should
also be noted that the mouse strain used in the current studies (AKR/J)
has been shown to have higher insulin levels and respond to a high-fat
diet with higher insulin levels than SWR/J mice (5, 25). Therefore, we
will need to verify the effect of CLA on insulin levels in other strains.
The apparent paradox in the study reported here might be explained by
the milder degree of obesity in the dietary obese mouse model compared
with the Zucker fatty rat and the reported effects of CLA to stimulate
lipolysis in adipocytes (18). If CLA induces a mild chronic lipolytic
state such that fatty acids are more readily available to skeletal
muscle, this could lead to a mild insulin resistance. Elevations of
fatty acids are known to lead to impaired insulin-stimulated glucose
disposal, perhaps through the glucose fatty acid cycle (19).
Theoretically, the greater availability of fatty acids for oxidation
inhibits glucose oxidation, which may be due to a reduced glucose
uptake in muscle (7) and in the whole body (22). Fatty acids may also
prime the 
-cell for glucose-stimulated insulin secretion (3, 16,
21). When palmitate is added to the perfusion media in isolated
pancreata, glucose-stimulated insulin secretion is restored in the
presence of an inhibitor of malonyl-CoA synthesis (3). This effect of fatty acids on insulin release is dependent on chain length and degree
of unsaturation (15); however, the effects of CLA on islet function
have not been tested.
Therefore, the moderate hyperinsulinemia induced by CLA could be
attributable to effects on both glucose utilization, resulting in mild
peripheral insulin resistance, and CLA, having direct stimulatory
effects on islet insulin release. The reason for the apparent
improvement in insulin sensitivity in Zucker fatty rats could be due to
the relative balance of effects in this model of severe obesity. Zucker
fatty rats already have high levels of insulin and free fatty acids
(14) due to decreased fatty acid oxidation (1, 12, 23). In addition,
these animals exhibit an increased fatty acid esterification, leading
to increased lipid deposition in pancreatic islets that may negatively
alter -cell function (11). Therefore, CLA may decrease fatty acid levels by increasing fatty acid oxidation as well as influencing PPAR activation, resulting in improved insulin sensitivity. Clearly, the effect of CLA in various models of obesity must be tested to
provide further insights into the mechanisms by which CLA influences lipid and carbohydrate metabolism.
The mechanism by which CLA increases total protein content is unknown. This response could be due to differential insulin resistance among tissues (7). If adipocytes become insulin resistant with CLA treatment this could partially explain the paradoxical increased fatty acid oxidation with increased insulin levels. If at the same time, skeletal muscle remains sensitive to insulin, the increased insulin levels could lead to increased protein synthesis and deposition. Another possibility is that CLA somehow causes an increase in growth hormone. This later possibility could also play a role in the increased fatty acid oxidation and increased insulin levels.
In summary, feeding mice CLA at 1% or lower concentrations as a dietary admixture reduces body fat accumulation and increases body protein accumulation. These effects of CLA on body composition occur fairly rapidly; some can be observed as early as 2 wk after treatment and persist. The increased liver weights observed in our previous and current study appear to be due to lipid accumulation. This could be due to the increased delivery of fatty acids to the liver in response to CLA feeding. That CLA feeding in the current studies causes an increase in serum insulin even as body fat stores are reduced is an interesting observation that requires further study.
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ACKNOWLEDGEMENTS |
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This study was supported by the National Cattlemen's Beef Association and Kraft Foods, Inc.
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FOOTNOTES |
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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. §1734 solely to indicate this fact.
Address for correspondence and reprint requests: J. P. DeLany, Pennington Biomedical Research Center, Louisiana State University, 6400 Perkins Rd., Baton Rouge, LA 70808 (E-mail: delanyjp{at}mhs.pbrc.edu).
Received 31 August 1998; accepted in final form 12 January 1999.
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TOP
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METHODS
RESULTS
DISCUSSION
REFERENCES
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) or a high-fat diet containing 1% CLA (
). Adipose depots
were dissected upon death at 2, 4, 6, 8, and 12 wk after beginning the
CLA diet. Each point represents the mean ± SE of 8 animals except
week 4 (1% CLA,
n = 7), week
6 (control, n = 7),
and week 12 (control,
n = 6).
* P < 0.05 and
** P < 0.001, differences from
control.
