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Effects of long-term administration of saturated and n-3 fatty acid-rich diets on lipid utilisation and oxidative stress in rat liver and muscle tissues

Published online by Cambridge University Press:  09 May 2013

Christine Feillet-Coudray ,
Manar Aoun ,
Gilles Fouret ,
Béatrice Bonafos ,
Jeanne Ramos ,
François Casas ,
Jean Paul Cristol  and
Charles Coudray
Christine Feillet-Coudray*
Affiliation:
INRA UMR 866, Dynamique Musculaire et Métabolisme, 34060Montpellier, France
Manar Aoun
Affiliation:
UMR 204 NUTRIPASS IRD/Montpellier-1/Montpellier-2/Supagro, 34000Montpellier, France
Gilles Fouret
Affiliation:
INRA UMR 866, Dynamique Musculaire et Métabolisme, 34060Montpellier, France
Béatrice Bonafos
Affiliation:
INRA UMR 866, Dynamique Musculaire et Métabolisme, 34060Montpellier, France
Jeanne Ramos
Affiliation:
Laboratoire d'Anatomie Pathologique, CHU Gui de Chauliac, 80, Avenue Augustin Fliche, 34295Montpellier Cedex 5, France
François Casas
Affiliation:
INRA UMR 866, Dynamique Musculaire et Métabolisme, 34060Montpellier, France
Jean Paul Cristol
Affiliation:
UMR 204 NUTRIPASS IRD/Montpellier-1/Montpellier-2/Supagro, 34000Montpellier, France
Charles Coudray
Affiliation:
INRA UMR 866, Dynamique Musculaire et Métabolisme, 34060Montpellier, France
*
*Corresponding author: Dr C. Feillet-Coudray, fax +33 4 67 54 56 94, email cfeillet@supagro.inra.fr
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Abstract

The incidence of metabolic syndrome components including obesity, lipid deregulation, insulin resistance (IR) and non-alcoholic fatty liver disease is increasing rapidly in wealthy societies. The present study was designed to determine the effect of different nutritional lipid patterns (quantity and quality) on lipid utilisation and oxidative stress in the liver and muscle of rats in an integrated fashion. A total of forty-eight Wistar male rats were fed for 12 weeks with a mixed, lard or fish-oil diet, containing either 50 or 300 g lipid/kg. Rats developed liver steatosis associated with moderate liver injury when fed the 30 % lipid diets, in spite of the absence of overt obesity or IR, except when fed the lard 30 % lipid diet. The intake of the 30 % lipid diets decreased hepatic lipogenesis and mitochondriogenesis and increased lipid peroxidation and protein oxidation. Surprisingly, muscle lipid content was not modified whatever the administered diet. The intake of the 30 % lipid diets increased the muscle protein expression of fatty acid (FA) translocase/cluster of differentiation 36 (FAT/CD36), PPARγ co-activator 1α (PGC-1α) and muscle carnitine palmitoyltransferase 1 (m-CPT1), reflecting increased FA transport in the muscle associated with increased oxidative metabolism. The lard 30 % lipid diet led to IR without modifying the muscle lipid content. The fish-oil 30 % lipid diet failed to prevent the development of hepatic steatosis and made the tissues more prone to oxidation. Overall, the present study suggests that the FA composition of muscle is more important than lipid accumulation itself in the modulation of insulin sensitivity, and indicates that precaution should be taken when advising an unphysiologically high (pharmacological) supplementation with long-chain n-3 PUFA.

Keywords

SFAn-3 PUFAHigh-lipid dietsSteatosisInsulin resistanceOxidative stressMitochondria
Type
Full Papers
Information
British Journal of Nutrition , Volume 110 , Issue 10 , 28 November 2013 , pp. 1789 - 1802
Copyright
Copyright © The Authors 2013 

Insulin resistance (IR) is a key component in the development of the metabolic syndrome (MetS), a very frequent condition characterised by dyslipidaemia, abdominal obesity and hypertension, which are related to an elevated risk of type 2 diabetes mellitus and CVD(Reference Misra, Singhal and Khurana1). The incidence of MetS components, in particular obesity, IR and non-alcoholic fatty liver disease (NAFLD), is increasing rapidly in wealthy societies and has become a major public health problem, with a great impact on morbidity and mortality(Reference Cave, Deaciuc and Mendez2). Liver lipid accumulation is the first stage of NAFLD and can occur as a result of the diet, de novo lipogenesis or the lipids released from adipose tissue. Then, oxidative stress, mitochondrial dysfunction and IR can lead to large hepatocyte injury, inflammation and fibrosis, which characterise the second stage of NAFLD that is called non-alcoholic steatohepatitis(Reference Mantena, King and Andringa3). Fish oils that contain considerable amounts of n-3 fatty acid (FA) (in particular EPA and DHA) have been reported to be protective against a number of disease states and, in particular, n-3 FA supplementation may prevent or reduce the progression of hepatic steatosis(Reference Shapiro, Tehilla and Attal-Singer4). Reduced hepatic TAG synthesis and increased β-oxidation are known to contribute to the hypolipidaemic effect of fish-oil diets. However, as tissue FA composition reflects partly dietary FA content(Reference Abbott, Else and Atkins5), fish-oil diet intake may increase PUFA levels in the targeted tissues and hence render them more prone to peroxidative damage.

Skeletal muscle is an essential tissue for whole-body energy metabolism, where FA metabolism is subject to extensive in vivo regulation, in particular the control of FA entry into the cell, the transfer of FA into the mitochondria and the capacity of the β-oxidation cycle. The balance between the uptake and utilisation of FA determines the magnitude of lipid accumulation in the muscle. Skeletal muscle is an important site for insulin action, and the accumulation of TAG and NEFA patterns in the muscle seems to affect insulin-mediated glucose uptake(Reference Kraegen, James and Storlien6). Insulin sensitivity is affected by the quality and quantity of dietary fat, independently of its effects on body weight. Many reports have shown that a high intake of dietary saturated fat worsens IR(Reference Manco, Mingrone and Greco7). On the contrary, long-chain n-3 FA may prevent IR and delay the progression of the MetS(Reference Poudyal, Panchal and Diwan8), although some randomised controlled trials have failed to confirm such beneficial effects(Reference Smith9).

The present study was designed to determine the impacts of three relevant nutritional lipid patterns on lipid utilisation and FA composition and their content in rat liver and muscle, two highly metabolically interrelated organs that are central to MetS pathology. These nutritional lipid patterns include the following: (1) recommended lipid diet (mixed diet); (2) consumed lipid diet in the industrialised countries (lard diet); (3) healthy lipid diet rich in long-chain n-3 PUFA (fish-oil diet). These dietary lipid patterns have been investigated at two dietary lipid levels, 5 and 30 %, of diet weight. Most published studies that have examined the effect of fat quality and/or quantity in many different physiological and pathological models have been interested in individual FA or in individual oils that do not reflect any nutritional lipid profile(Reference Hill, Peters and Lin10, Reference Buettner, Parhofer and Woenckhaus11). Finally, we also investigated the oxidative/antioxidative stress balance in rat liver and muscle and its relationship with tissue FA content, as it is known that oxidative stress may be implicated in the progression of liver steatosis and muscle IR. The novelty of the present study is the comparison of the three diet patterns and their impacts on the phenotypes of two highly metabolically interrelated organs (liver and muscle) that are central to MetS pathology with a large number of outcomes measured, which allows an integrated overview of the physiological impact of dietary fat composition.

Materials and methods

Animals and diets

The French dietary lipid recommendation, updated in 2010, represents the core of our dietary design (http://www.anses.fr/Documents/NUT2006sa0359Ra.pdf). The French recommendation for lipids is 35–40 % of energy intake (85–95 g lipids/d), which is divided into < 12 % SFA, 18–20 % MUFA and 5–10 % PUFA (with 1–2 % n-3). Although it is very difficult to replicate the human recommendations in the rat diet, we have designed the rodent diet to be broadly reflective of human dietary recommendations and patterns. The mixed diet was set up to reproduce the recommended lipid diet and composed of a blend of different lipid sources (40 % lard+25 % sunflower oil+25 % olive oil+10 % colza oil). The lard diet was set up to reproduce the currently consumed diet in many developed countries and composed of a large percentage of animal saturated lipids (90 % lard+10 % sunflower oil). Finally, the fish-oil diet was set up to reproduce a very healthy diet and composed of a high percentage of marine polyunsaturated lipids rich in long-chain n-3 FA (35 % lard+20 % sunflower oil+20 % olive oil+5 % colza oil+20 % fish oils (12 % tuna oil+8 % sardine oil)). This mixture of tuna and sardine oils provided 3 g EPA+DHA/kg and about 0·70 g/kg of other n-3 PUFA in the 5 % lipid diets, and 18 g EPA+DHA/kg and about 4·3 g/kg of other n-3 PUFA in the 30 % lipid diets. This mixture was made to ensure an optimal DHA:EPA ratio (2:1) in this diet that privileges the DHA level that is mostly incorporated in membrane phospholipids. The recommended amount of EPA+DHA for humans is 500 mg/d (0·2 % of energy intake), and it is up to 1 g/d (0·4 % of energy intake) for those with diagnosed MetS and CVD. However, higher doses (up to 13 g/d) have been investigated in several controlled trials(Reference Parker, Johnson and Burdon12). The dose used in the present study is 3 g EPA+DHA/kg diet in the 5 % lipid diet (0·70 % of energy intake) and 18 g/kg diet in the 30 % lipid diet supplemented with fish oils (3·15 % of energy intake). An adult man consumes about 500 g of dry diet/d, which means that our dose of 3 g EPA+DHA/kg diet (60 mg/rat per d) may be considered as physiological (supranutritional) and the dose 18 g/kg diet (360 mg/rat per d) is rather unphysiologically high (pharmacological). The detailed composition of the six experimental diets is given in Table S1 (available online).

A total of forty-eight male Wistar rats (Charles River) aged 6 weeks were housed under the conditions of constant temperature (20–22°C), humidity (45–50 %) and a standard dark cycle (20.00–08.00 hours). The animals were randomised into six groups of eight and fed for 12 weeks one of the following semi-purified diets: mixed diet with 5 or 30 % lipid; lard diet with 5 or 30 % lipid; fish-oil diet with 5 or 30 % lipid. Rats were given free access to tap water and food. Body weight and diet consumption were determined weekly. Our institution guidelines for the care and use of laboratory animals were observed, and all the experimental procedures were approved by the local ethical committee in Montpellier, France (Reference CEEA-LR-11 009).

Oral glucose tolerance test

The OGTT was performed as described previously(Reference Gomez-Perez, Amengual-Cladera and Catala-Niell13). Briefly, in week 11, 16 h fasting rats were orally administered 2 g glucose/kg body weight. Blood was collected through the tail vein of conscious rats immediately before the oral administration and 10, 20, 30, 45, 60, 90, 120 and 180 min afterwards, and glucose was measured using a commercial glucometer (AccuChek Active; Roche Diagnostics). The AUC values are expressed as mg glucose/l × min.

Sampling and routine biochemical analysis

Pentobarbital was used to anaesthetise 16 h fasted rats (Ceva Santé Animale) and blood was obtained by puncture of the abdominal artery. Blood was centrifuged at 1000 g for 10 min at 4°C, and plasma or serum was collected and stored at − 80°C until analysis. Liver and gastrocnemius muscle were removed, rinsed with 0·9 % NaCl, frozen in N2 and kept at − 80°C until analysis. Plasma glucose, total cholesterol, HDL-cholesterol, TAG and NEFA levels were measured by enzymatic techniques (Konelab; Thermo Electron Corporation). Alanine transaminase and γ-glutamyl transferase were determined using standard methods on a Cobas MIRA automated analyser (Roche Diagnostics). Plasma insulin and leptin levels were quantified using ELISA kits (Linco Research).

Histological analysis

For microscopic studies, liver samples were fixed in 10 % neutral buffered formalin and embedded in paraffin. Serial tissue sections (5 μm) were processed. Liver injury, such as steatosis, portal inflammatory infiltrate and fibrosis, was evaluated by histological examination after haematoxylin and eosin staining(Reference Aoun, Fouret and Michel14).

β-Oxidation and oxidative stress parameters in the liver and muscle

Liver and muscle homogenates were prepared on ice (1 g with 9 ml phosphate buffer, 50 mm, pH 7·0) using a Polytron homogeniser. Homogenate samples were saved for thiobarbituric acid-reactive substances (TBARS) and reduced glutathione (GSH)/oxidised glutathione (GSSG) measurements. The remaining homogenates were centrifuged at 1000 g for 10 min at 4°C and the supernatants were aliquoted and kept at − 80°C until analysis. Supernatant protein level was measured by Bradford's technique(Reference Bradford15).

β-Hydroxyacyl-CoA dehydrogenase (β-HAD) was determined by a spectrophotometric technique according to the procedure of Yang et al. (Reference Yang, He and Schulz16). TBARS, sulphydryl groups (–SH), GSH and GSSG levels and catalase, glutathione peroxidase, total superoxide dismutase (SOD) and Mn-SOD activities in the tissues were measured by spectrophotometric techniques as described previously(Reference Feillet-Coudray, Sutra and Fouret17).

Immunoblotting

Tissue samples were homogenised using an Ultra Turax homogeniser in an ice-cold extraction buffer. Proteins were separated with 10 or 8 % SDS–PAGE and then transferred onto nitrocellulose membranes. The membranes were blocked in 5 % non-fat milk for 1 h at room temperature. The membranes were incubated overnight with a primary antibody against acetyl-CoA carboxylase (ACC, 1:1000), phospho-ACC (p-ACC, 1:1000), Akt (1:1000), phospho-Akt (p-Akt, 1/1000), FA translocase/cluster of differentiation 36 (FAT/CD36, 1:500), muscle carnitine palmitoyltransferase 1 (m-CPT1, 1:200), FA synthase (FAS, 1:1000), fatty acid transport protein 4 (FATP4, 1:1000), PPARγ co-activator 1α (PGC-1α, 1:1000) and stearoyl-CoA desaturase 1 (SCD1, 1:200) in a blocking buffer. After washes in Tris-buffered saline/Tween, the membranes were incubated for 1 h with horseradish peroxidase-labelled antibodies (1:2000). After further washes, the blots were treated with enhanced chemiluminescence detection reagents. β-Actin was used as the loading reference, and blot intensities were measured using ImageJ software (NIH). The antibodies of ACC, p-ACC, Akt, p-Akt and FAS were obtained from Cell Signaling Technology, Inc.; FAT/CD36 and FATP4 from Abcam; m-CPT1 and SCD1 from Santa Cruz Biotechnology; and PGC-1α from Calbiochem, Millipore SAS.

Liver and muscle mRNA expression

Real-time quantitative PCR was used to measure the mRNA expression of the target genes in the tissues and was performed as described previously(Reference Aoun, Michel and Fouret18). The primer sequences used for real-time RT-PCR are given in Table S2 (available online). After normalisation by 18S for the liver and RPS9 for the muscle, all results are expressed as a percentage of the control.

Extraction and analysis of liver and muscle lipids

Tissue samples were homogenised in NaCl (9 g/l) and Triton X-100 (0·1 %), and NEFA, TAG and total cholesterol levels in the tissue homogenates were quantified by enzymatic methods (Wako-NEFA-C kit – Oxoid; Cholesterol RTU kit and TG PAP kit – Biomerieux). The lipids were then extracted from the tissue homogenates using the method of Folch et al. (Reference Folch, Lees and Sloane Stanley19), and P was quantified in the chloroform–methanol extracts in order to determine total phospholipid quantity as described previously(Reference Bartlett20). The chloroform–methanol lipid extract, spiked with 17 : 0 (2·5 μg/l) as an FA internal standard, was used for total FA analysis by GC after trans-esterification as described previously(Reference Poudyal, Panchal and Diwan8).

Tissue desaturase, unsaturation and peroxidisation indices

Because it is not possible to directly measure the activity of the enzymes that catalyse the desaturation and elongation reactions in FA metabolic pathways, results obtained in animals have supported the use of surrogate measures of desaturase activity such as the use of desaturase indices(Reference Warensjo, Ohrvall and Vessby21). These indices are based on the ratio of the product to the precursor of individual FA. Desaturase indices were calculated as follows: Δ9, 16 : 1n-7/16 : 0; Δ6, 18 : 3n-6/18 : 2n-6; Δ5, 20 : 4n-6/20 : 3n-6. However, the Δ6 index in our muscle homogenates was estimated as 20 : 3n-6/18 : 2n-6, since the proportion of 18 : 3n-6 was too low for reliable quantification. It should be noted that this ratio also measures the elongase activity, but this step is not considered to be rate limiting, suggesting that this ratio is also a good estimate of Δ6 activity(Reference Warensjo, Riserus and Gustafsson22). The unsaturation index is the sum of the fraction of each FA multiplied by the number of double bonds in that acid(Reference Pietrangelo, Grandi and Tripodi23). The peroxidisability index (PI) was calculated as described previously(Reference Hu, Frankel and Leibovitz24):

$$\begin{eqnarray} PI = (\%\,dienoic\times 1) + (\%\,trienoic\times 2) + (\%\,tetraenoic\times 3) + (\%\,pentaenoic\times 4) + (\%\,hexaenoic\times 5). \end{eqnarray}$$

Statistical analysis

Results are expressed as means and standard deviations. Statistical analysis was based on a two-way ANOVA followed by Fisher's multiple comparison test. When there was no significant interaction between the quantity and quality of the lipid groups, the comparison between the 5 and 30 % lipid groups was done on the basis of the mean response for the three lipid quality groups combined. However, when there was a significant interaction, Fisher's post hoc test was performed among the lipid quality groups, testing the effect of the diet pattern (lipid type) within the 5 and 30 % lipid groups, separately. Correlations were performed with the Spearman method. The limit of statistical significance was set at P <0·05. Statistical analysis was performed using the StatView program (SAS Institute).

Results

Characteristics of the rats

Body weight was statistically similar among the six experimental groups, but showing a strong trend to increase with the 30 % lipid diets (Table 1). In fact, both the final body weight and weight gain were increased in the lard 30 % lipid diet group compared with the mixed and the fish-oil 30 % lipid diet groups (ANOVA, P< 0·05). The adipose tissue weight tended to increase in the 30 % lipid diet-fed rats compared with the 5 % lipid diet-fed rats, and was increased in the lard 30 % lipid diet-fed group (+35 %) compared with the other groups. The dietary and energy intakes were higher in rats receiving the lard 30 % lipid diet compared with those receiving the mixed or the fish-oil 30 % lipid diet.

Table 1 Body weight and weight gain, dietary and energy intakes and plasma glucose, lipid, insulin and leptin levels (Mean values and standard deviations, n 8)

HDL-C, HDL-cholesterol; LDL-C, LDL-cholesterol; ALAT, alanine transaminase; γ-GT, γ-glutamyl transferase; ND, non-detectable; OGTT, oral glucose tolerance test.

a,bMean values with unlike superscript letters were significantly different (P< 0·05).

* A two-way ANOVA was used, followed by Fisher's multiple comparison test. When there was an interaction, a one-way ANOVA followed by Fisher's multiple comparison test was conducted on the 5 % diet groups and the 30 % diet groups distinctly.

To convert enzyme activity in units to nkatal, multiply by 16·67.

Plasma insulin level was higher in rats fed the 30 % lipid diets than in those fed the 5 % lipid diets (Table 1). Moreover, the AUC of the OGTT, reflecting IR, was increased with the 30 % lipid diets in comparison with the 5 % lipid diets, particularly with the lard 30 % lipid diet in comparison with the mixed and the fish-oil 30 % lipid diets. Plasma glucose and leptin levels were increased with the lard 30 % lipid diet in comparison with the mixed and the fish-oil 30 % lipid diets. Blood NEFA levels were not different among the groups (Table 1), whereas plasma TAG and total cholesterol levels were decreased in rats fed the 30 % lipid diets and in particular in those fed the fish-oil 30 % lipid diet in comparison with those fed the mixed and the lard 30 % lipid diets. The HDL:LDL ratio was increased with the fish-oil diet in comparison with the mixed and the lard diets. Plasma alanine transaminase was not modified whatever the group, whereas γ-glutamyl transferase was increased moderately with the 30 % lipid diets, reflecting slight liver injury.

Liver lipid, fatty acid composition and desaturase indices

The liver histological evaluation of hepatic steatosis showed that the rats fed the 5 % mixed and the 5 % lard-rich diets had microvacuolar steatosis with few hepatocytes displaying intracytoplasmic droplets (Fig. 1). Liver sections from the rats fed the 5 % fish oil-rich diet also showed a few steatotic macrovacuoles with simple bulky fat vacuoles that distended the hepatocyte and pushed the nucleus. On the other hand, histological studies on the liver sections from the rats fed the 30 % lipid diets showed high-grade macrovacuolar steatosis in the three studied groups. As expected, liver weight was increased in the 30 % lipid diet-fed rats compared with the 5 % lipid diet-fed rats, but lipid quality had no effect on liver weight. In addition, liver NEFA, TAG and total cholesterol levels were increased with the 30 % lipid diets, reflecting overt liver steatosis. Moreover, total cholesterol level was increased with the fish-oil 30 % lipid diet in comparison with the mixed and the lard 30 % lipid diets. The liver phospholipid level was not modified whatever the diet (Table 2).

Fig. 1 Liver histology after haematoxylin/eosin staining of liver sections from representative rats of each group: (A) 5 % basal diet; (B) 5 % lard-rich diet; (C) 5 % fish oil-rich diet; (D) 30 % basal diet; (E) 30 % lard-rich diet; (F) 30 % fish oil-rich diet. Original magnification 100 × .

Table 2 Liver lipids and oxidative stress parameters (Mean values and standard deviations, n 8)

β-HAD, β-hydroxyacyl-CoA dehydrogenase; TBARS, thiobarbituric acid-reactive substances; GSH, reduced glutathione; GSSG, oxidised glutathione; SOD, superoxide dismutase; GPx, glutathione peroxidase.

a,b,cMean values with unlike superscript letters were significantly different (P< 0·05).

* A two-way ANOVA was used, followed by Fisher's multiple comparisons test. When there was an interaction, a one-way ANOVA followed by Fisher's multiple comparison test was conducted on the 5 % diet groups and the 30 % diet groups distinctly.

To convert enzyme activity in units to nkatal, multiply by 16·67.

The intake of the 30 % lipid diets increased total liver SFA, MUFA and PUFA levels compared with that of the 5 % lipid diets (Table 3). The lard diet had no effect on the liver FA composition, although the OGTT was positively correlated with the liver SFA levels (P< 0·05; r 2 0·120). In the fish-oil diet-fed rats, total n-3 PUFA quantities, and in particular DHA (22 : 6n-3), were higher in comparison with those fed the mixed or the lard diet (Table 3). The n-3:PUFA ratio was increased with the fish-oil diet (Table 3), and the OGTT was negatively correlated with the liver n-3:PUFA ratio (P< 0·05; r 2 0·114).

Table 3 Total fatty acid (FA) composition of the liver homogenates (mg FA/g tissue)* (Mean values and standard deviations, n 8)

ND, non-detectable; UI, unsaturation index; PI, peroxidation index.

a,b,cMean values with unlike superscript letters were significantly different (P< 0·05).

* The results of the major FA (>0·1 %) are expressed as mg FA/g liver.

A two-way ANOVA was used, followed by Fisher's multiple comparison test. When there was an interaction, a one-way ANOVA followed by Fisher's multiple comparison test was conducted on the 5 % diet groups and the 30 % diet groups distinctly.

Δ9-Desaturase index = 16 : 1n-7/16 : 0.

§ Δ6-Desaturase index = 18 : 3 n-6/18 : 2n-6.

Δ5-Desaturase index = 20 : 4n-6/20 : 3n-6.

Both Δ9-desaturase and Δ6-desaturase indices were decreased in rats fed the 30 % lipid diets compared with those fed the 5 % lipid diets, whereas the Δ5-desaturase activity index was not affected by the dietary fat level (Table 3). With regard to the diet quality, the Δ6-desaturase and Δ5-desaturase activity indices were decreased in rats fed the fish-oil diet in comparison with those fed the mixed or the lard diet. There was no effect of dietary lipid quantity on the liver lipid unsaturation index and PI parameters. Both these indices remained comparable in rats receiving the 5 or the 30 % lipid diets. However, and as expected, the quality of dietary lipids had an impact on both these indices, which were increased in rats fed the fish-oil diet in comparison with those fed the mixed or the lard diet, more in those fed the 30 % lipid diets than in those fed the 5 % lipid diets (Table 3).

Liver lipogenesis pathway signalling

The liver protein expression of FAT/CD36 and the mRNA expression of FA-binding protein 1 (FABP1) and liver carnitine palmitoyltransferase 1 (L-CPT1) were decreased with the 30 % lipid diets (Fig. 2). The liver protein expression of FATP4 was not modified with the 30 % lipid diets but was increased with the lard 30 % lipid diet in comparison with the mixed or the fish-oil 30 % lipid diet (Fig. 2). The protein expression of PGC-1α was decreased with the 30 % lipid diets, while the liver mRNA expression of PPAR-α was not modified (Fig. 2). The liver protein expression of SCD1 (Fig. 3) was decreased with the 30 % lipid diets and was increased with the lard diet in comparison with the fish-oil diet. The liver protein expression of FAS and p-ACC was decreased with the 30 % lipid diets, but the total protein expression of ACC remained unchanged (Fig. 3). In addition, the mRNA expression of MCD was not modified whatever the diet, whereas the mRNA expression of MCAD was decreased with the 30 % lipid diets in comparison with the 5 % lipid diets (Fig. 3). β-HAD activity was modified with the 30 % lipid diets in comparison with the 5 % lipid diets (Table 2). Indeed, β-HAD activity was decreased with the mixed and the fish-oil 30 % lipid diets in comparison with the lard 30 % lipid diet.

Fig. 2 Liver protein expression of fatty acid translocase/cluster of differentiation 36 (FAT/CD36), fatty acid transport protein 4 (FATP4) and PPARγ co-activator 1α (PGC-1α), and liver gene expression of fatty acid-binding protein 1 (FABP1), liver carnitine palmitoyltransferase 1 (L-CPT1) and PPAR-α. (A) Western blot was performed on protein extracts from the liver of rats, using anti-FAT/CD36, anti-FATP4 and anti-PGC-1α antibodies. Anti-β-actin antibody was used to confirm equal loading. Western blot was quantified using ImageJ software (NIH). (B) Quantitative real-time PCR analysis of the mRNA expression of FABP, L-CPT1 and PPAR-α in the liver. Values are means (n 6–8), with standard deviations represented by vertical bars. (A) There was a significant effect of lipid quantity on FAT/CD36 and PGC-1α protein expression (P< 0·001). There was a significant effect of lipid quantity on FATP4 protein expression (P< 0·01) with a significant interaction between the quantity and quality of lipid (P< 0·05). (B) There was a significant effect of lipid quantity on FABP1 and L-CPT1 gene expression (P< 0·05). , Basal diet; , lard-rich diet; , fish oil-rich diet.

Fig. 3 Liver protein expression of stearoyl-CoA desaturase 1 (SCD1), fatty acid synthase (FAS) and phospho-acetyl-CoA carboxylase (p-ACC) and p-ACC:ACC ratio, and liver gene expression of malonyl CoA decarboxylase (MCD) and medium-chain acyl-CoA dehydrogenase (MCAD). (A) Western blot was performed on protein extracts from the liver of rats, using anti-SCD1, anti-FAS, anti-ACC and anti-p-ACC antibodies. Anti-β-actin antibody was used to confirm equal loading. Western blot was quantified using ImageJ software (NIH). (B) Quantitative real-time PCR analysis of the mRNA expression of MCD and MCAD in the liver. Values are means (n 6–8), with standard deviations represented by vertical bars. (A) There was a significant effect of lipid quantity and quality on SCD1 protein expression (P< 0·001, P< 0·05, respectively). There was a significant effect of lipid quantity on p-ACC and FAS protein expression (P< 0·001). (B) There was a significant effect of lipid quantity on MCAD gene expression (P< 0·05). , Basal diet; , lard-rich diet; , fish oil-rich diet.

Liver oxidative stress parameters

Liver TBARS levels were markedly increased in rats fed the 30 % lipid diets (Table 2); moreover, liver lipid oxidation was increased with the fish-oil diet in comparison with the mixed and the lard diets. Within the 5 % lipid diets, the liver TBARS level was increased by 22 % with the fish-oil diet compared with the mixed diet, whereas within the 30 % lipid diets, the liver TBARS level was increased by 104 % with the fish-oil diet compared with the mixed diet. TBARS levels were positively correlated with the liver n-3:PUFA ratio (P< 0·001; r 2 0·319) and the PI (P< 0·001; r 2 0·377). Protein oxidation was increased with the 30 % lipid diets as –SH levels were decreased, while the quality of dietary FA in the diet had no effect (Table 2). GSH and GSSG levels were decreased with the 30 % lipid diets, while GSH:GSSG remained unchanged. Liver catalase, SOD, Mn-SOD and glutathione peroxidase activities were not modified with the 30 % lipid diets in comparison with the 5 % lipid diets (Table 2). However, glutathione peroxidase activity was decreased with the fish-oil 30 % lipid diet in comparison with the lard 30 % lipid diet, and catalase activity was increased with the fish-oil 5 % lipid diet in comparison with the lard 5 % lipid diet.

Muscle lipid fatty acid composition and desaturase activity

Muscle NEFA, TAG and phospholipid levels were not modified whatever the diet (Table 4). Total cholesterol level was not modified with the 30 % lipid diets but was increased with the lard 5 % lipid diet in comparison with the mixed and the fish-oil 5 % lipid diets. Total SFA and MUFA were not modified with the 30 % lipid diets, while total PUFA were higher in the muscle of rats fed the 30 % lipid diets than in those fed the 5 % lipid diets (Table 5). In rats fed the lard diet, total SFA, and in particular 18 : 0, was increased and the OGTT was positively correlated with the muscle 18 : 0 levels (P< 0·05; r 2 0·130). In rats fed the fish-oil diet, total n-3 PUFA quantities (DHA) were higher in comparison with those fed the mixed and the lard diets. The n-6:n-3 ratio was decreased and the n-3:PUFA ratio was increased with the fish-oil diet (Table 5), and the OGTT was negatively correlated with the muscle n-3:PUFA ratio (P< 0·05; r 2 0·084).

Table 4 Muscle lipids and oxidative stress (Mean values and standard deviations, n 8)

β-HAD, β-hydroxyacyl-CoA dehydrogenase; TBARS, thiobarbituric acid-reactive substances; GSH, reduced glutathione; SOD, superoxide dismutase; GPx, glutathione peroxidase.

a,bMean values with unlike superscript letters were significantly different (P< 0·05).

* A two-way ANOVA was used, followed by Fisher's multiple comparison test. When there was an interaction, a one-way ANOVA followed by Fisher's multiple comparison test was conducted on the 5 % diet groups and on the 30 % diet groups distinctly.

To convert enzyme activity in units to nkatal, multiply by 16·67.

Table 5 Total fatty acid (FA) composition of the muscle homogenates (mg FA/g tissue)* (Mean values and standard deviations, n 8)

UI, unsaturation index; PI, peroxidation index.

* The results of the major FA (>0·1 %) are expressed as mg FA/g skeletal muscle.

A two-way ANOVA was used, followed by Fisher's multiple comparison test. When there was an interaction, a one-way ANOVA followed by Fisher's multiple comparison test was conducted on the 5 % diet groups and the 30 % diet groups distinctly.

Δ9-Desaturase index = 16 : 1n-7/16 : 0.

§ Δ6-Desaturase index = 20 : 3n-6/18 : 2n-6. Because 18 : 3n-6 quantification was not possible in many muscle samples, we applied the 20 : 3n-6/18 : 2n-6 ratio to assess the Δ6-desaturase index according to Warensjo et al. (22).

Δ5-Desaturase index = 20 : 4n-6/20 : 3n-6.

As shown in Table 5, the muscle 16 : 1n-7/16 : 0 ratio, the Δ9-desaturase activity index, was dramatically decreased in rats fed the 30 % lipid diets compared with those fed the 5 % lipid diets. The Δ6-desaturase activity index, measured as the 20 : 3n-6/18 : 2n-6 ratio because the muscle 18 : 3n-6 was not measurable, was decreased in rats fed the 30 % lipid diets compared with those fed the 5 % lipid diets. The Δ5-desaturase activity index, 20 : 4n-6/20 : 3n-6 ratio, was increased in rats fed the 30 % lipid diets compared with those fed the 5 % lipid diets, and was decreased in rats fed the fish-oil diet in comparison with those fed the mixed and the lard diets. Finally, the muscle unsaturation index and PI were not modified with the 30 % lipid diets in comparison with the 5 % lipid diets, while these indices were increased in rats fed the fish-oil diet in comparison with those fed the mixed and the lard diets.

Muscle lipogenesis pathway signalling and phospho-Akt/Akt protein expression

The muscle protein expressions of FAT/CD36 and m-CPT1 (Fig. 4) were increased, respectively, significantly and almost significantly (P= 0·0506), with the 30 % lipid diets. The muscle protein expression of FATP4 and the mRNA expression of FABP3 were not modified whatever the diet (data not shown). The muscle protein expression of SCD1 (Fig. 4), FAS and p-ACC (data not shown) was not modified whatever the diet. However, the protein expression of SCD1 tended to decrease with the fish-oil diet (Fig.4; P= 0·0588). Moreover, the mRNA expression of MCD was not modified whatever the diet (data not shown). The muscle mRNA expression of MCAD (data not shown) and muscle β-HAD activity (Table 4) were not modified whatever the diet. The muscle protein expression of PGC-1α was almost significantly increased with the 30 % lipid diets (Fig.4; P= 0·053), while the mRNA expression of PPAR-α was not modified (data not shown). The muscle protein p-Akt:Akt ratio was not modified whatever the diet (data not shown), although the p-Akt:Akt ratio was negatively correlated with the OGTT (P< 0·05, r 2 0·193).

Fig. 4 Muscle protein expression of fatty acid translocase/cluster of differentiation 36 (FAT/CD36), muscle carnitine palmitoyltransferase 1 (m-CPT1), stearoyl-CoA desaturase 1 (SCD1) and PPARγ co-activator 1α (PGC-1α). Western blot was performed on protein extracts from the muscle of rats, using anti-FAT/CD36, anti-m-CPT1, anti-SCD1 and anti-PGC-1α antibodies. Anti-β-actin antibody was used to confirm equal loading. Western blot was quantified using ImageJ software (NIH). Values are means (n 6–8), with standard deviations represented by vertical bars. There was a significant effect of lipid quantity on FAT/CD36 protein expression (P< 0·05) or almost significant effect on m-CPT1 (P= 0·051) and PGC-1α protein expression (P= 0·053). There was a nearly significant effect of lipid quality on SCD1 protein expression (P= 0·059) (fish oil v. mixed and lard diets. , Basal diet; , lard-rich diet; , fish oil-rich diet.

Muscle oxidative stress parameters

As shown in Table 4, 30 % lipid intake had no impact on muscle lipid oxidation (TBARS levels) or protein oxidation (–SH group levels). However, the muscle TBARS level was increased with the fish-oil diet and positively correlated with the muscle n-3:PUFA ratio (P< 0·05; r 2 0·124) and the PI (P< 0·05; r 2 0·087). The muscle GSH level was decreased with the 30 % lipid diets, whereas the GSSG level was not detectable in the muscle by our spectrophotometric method. Muscle antioxidant enzyme activities (SOD, Mn-SOD and glutathione peroxidase) remained unchanged, but catalase activity was increased with the 30 % lipid diets in comparison with the 5 % lipid diets (Table 4), and was increased with the fish-oil 30 % lipid diet in comparison with the mixed and the lard 30 % lipid diets.

Discussion

The present study was designed to determine the impacts of different relevant patterns of dietary lipids (quantity and quality) on lipid utilisation and FA content in rat liver and muscle tissues and their consequences on NAFLD and IR. The present results show that the intake of 30 % lipid diets increased liver FA and TAG contents and led to liver steatosis (liver lipid droplets). The lard diet had no effect on liver FA composition, probably because of the high dietary level of MUFA or the in vivo synthesis of MUFA from SFA. In accordance with this observation, the protein expression of SCD1, a Δ9-desaturase that catalyses the synthesis of monounsaturated long-chain FA from saturated fatty acyl-CoA, was increased with the lard diet. In contrast, the fish-oil diet considerably modulated the liver FA composition, where n-3 PUFA level was increased in the liver of rats fed the fish-oil diet. Moreover, the fish-oil diet decreased the liver Δ6-desaturase and Δ5-desaturase activity indices, which is in line with the recent reports(Reference Lamaziere, Wolf and Barbe25).

Liver FA can be derived from the diet and are synthesised de novo in case of excess carbohydrates, and then they are oxidised or esterified to glycerol for the synthesis of TAG(Reference Dobrzyn and Ntambi26). In the present study, the protein expression of the major actors of lipid metabolism (FAT/CD36, FABP1, ACC and FAS) was decreased and the protein expression of SCD1 was almost suppressed in rats fed the 30 % lipid diets. Moreover, the p-ACC:ACC ratio and the gene expression of MCD were unchanged. Surprisingly, the protein expression of FATP4 was increased in rats fed the lard 30 % lipid diet. As the content of palmitic acid is higher in the lard diet than in the mixed and the fish-oil diets, it is possible that the protein expression of FATP4 was increased because FATP4 was more effective than the other FA transporters in palmitate transport, as suggested previously(Reference Nickerson, Alkhateeb and Benton27). It has been well documented that hepatic lipogenesis is markedly reduced with high-lipid diets, with the transcription of hepatic genes encoding FAS, SCD1 and ACC being rapidly suppressed, and that this effect is more pronounced with n-3 FA(Reference Jump and Clarke28). Moreover, it has been reported that n-3 supplementation may prevent or reduce hepatic steatosis(Reference Shapiro, Tehilla and Attal-Singer4). However, in the present study, we did not observe any reduced lipogenesis or lower liver lipid content with the fish-oil diet compared with the other two studied diets.

Mitochondrial biogenesis is largely controlled by the transcriptional co-activator PGC-1α. This later induces the genes involved in mitochondrial β-oxidation, such as MCAD and L-CPT1 (Reference Lin, Handschin and Spiegelman29, Reference Lehman, Barger and Kovacs30). In the present study, the protein expression of PGC-1α was decreased with the 30 % lipid diets, without any effect of the dietary lipid quality. In accordance with this, the gene expression of L-CPT1, which allows FA to cross the mitochondrial membrane(Reference Kerner and Hoppel31), and the gene expression of MCAD, the first enzyme in the β-oxidation cycle, were down-regulated with the 30 % lipid diets. Moreover, β-HAD activity, the third enzyme in the β-oxidation cycle, was decreased in the liver of rats fed the 30 % lipid diets, except in the liver of those fed the 30 % lard diet. Both β-HAD activity and the protein expression of FATP4 were increased with the lard 30 % lipid diet, while they were decreased or tended to decrease with the other two 30 % lipid diets. It has been proposed that FATP4 is important as a lipid transport protein directing lipids for lipid oxidation in muscle(Reference Jeppesen, Jordy and Sjoberg32), and the present results suggest that FATP4 may also be important to direct FA towards β-oxidation in the liver. A deregulation of mitochondrial function may be implicated in liver fat accumulation observed with the 30 % lipid diets, where mitochondrial β-oxidation (measured by the gene expression of MCAD and β-HAD activity) was decreased. The intake of the 30 % lipid diets led to a higher supply with energy substrates and this may be responsible for the decrease in β-HAD activity with the 30 % lipid diets, except with the lard diet where β-oxidation remained high, probably to allow a high-rate oxidation of the saturated ‘toxic’ FA from this diet.

Oxidative stress, an important component of NAFLD, plays a role in the progression of liver steatosis to non-alcoholic steatohepatitis. Interestingly, lipid peroxidation and protein oxidation were increased in rats fed the 30 % lipid diets. These results may reflect an increase in mitochondrial reactive oxygen species production in the liver of rats with hepatic steatosis, despite lower mitochondriogenesis and β-oxidation activities. Moreover, the other important result of the present study is that lipid peroxidation was highly increased with the fish-oil diet. Within the 5 % lipid diets, the liver TBARS level was increased by 22 % with the fish-oil diet compared with the mixed diet, whereas within the 30 % lipid diets, the liver TBARS level was increased by 104 % with the fish-oil diet compared with the mixed diet. It is known that unsaturated FA are preferable substrates for lipid peroxidation, and, in fact, liver TBARS levels were positively correlated with the liver n-3:PUFA ratio and the PI. In a previous work, it has also been reported that a high intake of DHA increased, in a dose-dependent way, liver lipid peroxidation in rabbits, where the highest tested dose was 1 % DHA of energy intake(Reference Gladine, Roy and Rigaudière33). Moreover, oxidative stress and mitochondrial dysfunction may lead to large hepatocyte injury, inflammation and fibrosis(Reference Cave, Deaciuc and Mendez2, Reference Mantena, King and Andringa3). Therefore, the fatty liver from the rats fed the fish-oil diet may be prone to the transformation of liver steatosis into non-alcoholic steatohepatitis.

As expected, muscle FA content partly mirrored the quality of the FA in the studied diets, with more SFA in the muscle of rats fed the lard diet and more n-3 FA in the muscle of rats fed the fish-oil diet. In line with this observation, previous studies have also reported that the FA composition of muscle lipids is influenced by the type of FA in the administered diet(Reference Lee, Pinnamaneni and Eo34, Reference Abbott, Else and Hulbert35). However, the long-term intake of the 30 % lipid diets did not modify the muscle TAG content in the present study, but had an impact on the desaturase indices. Although it is known that PUFA decrease and SFA increase the expression of SCD1 in the liver(Reference Ntambi36), there are few data describing SCD1 regulation by dietary FA in skeletal muscle(Reference Lee, Pinnamaneni and Eo34). In a previous work(Reference Aoun, Michel and Fouret37), we observed an elevated SCD1 index to be associated with increased fat accumulation in skeletal muscle. In this work, the SCD1 index, calculated as the Δ9-desaturase index, was sharply decreased with the 30 % lipid diets. While the activity of SCD1 was not modified by the quality of the diet, the protein expression of SCD1 was almost decreased with the fish-oil diet. The Δ6-desaturase index was also decreased in rats fed the 30 % lipid diets compared with those fed the 5 % lipid diets. As in the liver, the muscle Δ5-desaturase index was decreased with the n-3 diet, showing a systemic effect of the n-3 diet on different tissues.

In skeletal muscle, PGC-1α is known to stimulate mitochondrial biogenesis via the co-activation of nuclear respiratory factor 1, to regulate genes involved in oxidative phosphorylation and to co-activate the PPAR, thereby regulating the pathways of lipid metabolism(Reference Lin, Handschin and Spiegelman29). We observed that the protein expressions of both PGC-1α and m-CPT1 were almost significantly increased with the 30 % lipid diets, with both PGC-1α and m-CPT1 being regulated by PPAR-δ in the muscle(Reference Dressel, Allen and Pippal38). Similarly, increased mitochondriogenesis had been previously reported with a high-fat diet(Reference Gomez-Perez, Capllonch-Amer and Gianotti39). In contrast, in a previous work(Reference Aoun, Michel and Fouret37), we observed that the gene expression of PGC-1α was down-regulated by a high-fat/high-sucrose diet, and some authors have demonstrated that palmitic acid or high SFA down-regulate the mRNA expression of PGC-1α(Reference Coll, Jové and Rodríguez-Calvo40). In parallel to the increase in the protein expression of PGC-1α with the 30 % lipid diets, we observed an increase in the protein expression of FAT/CD36. However, the protein or gene expressions of other transporters such as FATP4 and FABP3 were not modified. It has been demonstrated that the promoter of FAT/CD36 has a PPAR response element sequence(Reference Teboul, Febbraio and Gaillard41); therefore, an increased protein expression of PGC-1α could result in an enhanced protein expression of FAT/CD36, as has been reported already, while the gene or protein expressions of other FA transporters were not modified(Reference Choi, Befroy and Codella42). The present results are in favour of an increased uptake of FA with the 30 % lipid diets and in favour of an activation of muscle oxidative metabolism that prevented the accumulation of lipids in the muscle.

We observed that the AUC of the OGTT was positively correlated with the muscle SFA levels and negatively correlated with the muscle n-3:PUFA ratio. This observation was not surprising as several studies in animals have demonstrated a differential impairment in the degree of insulin sensitivity, after feeding with a saturated fat diet or n-6 or n-3 polyunsaturated fat diets(Reference Galgani, Uauy and Aguirre43). In the present study, only the rats fed the lard 30 % lipid diet were insulin resistant. So, it was probably the modification of the FA composition in the muscle cell membrane that led to IR rather than the modification of the lipid content in the muscle.

Lipid peroxidation and protein oxidation were not modified in the muscle of rats fed the 30 % lipid diets, while total GSH was decreased and catalase activity was increased. These results, associated with the probable activation of muscle oxidative metabolism, might reflect increased mitochondrial reactive oxygen species production that was counteracted by the antioxidant systems. Moreover, muscle TBARS levels were positively correlated with the muscle n-3:PUFA ratio and the peroxidisation index. This means that the muscle from the rats fed the fish-oil diet, as in the case of the liver, may be more prone to oxidative injury. However, with the fish-oil 30 % lipid diet, catalase activity was increased, once again probably to protect the cells against H2O2 and the oxidation of membrane phospholipids.

In conclusion, we examined in the present study the impact of fat quantity and quality on liver and muscle metabolism in an integrated fashion. The present results demonstrated that high lipid intake differently influenced the rat liver and muscle lipid utilisation and their FA composition. In the liver, lipogenesis was markedly reduced with the 30 % lipid diets to prevent liver lipid accumulation, whereas mitochondriogenesis was decreased, maybe to limit mitochondrial reactive oxygen species overproduction, and finally led to liver lipid accumulation and peroxidation. On the contrary, the muscle uptake of FA from the 30 % lipid diets was increased, but the high activation of muscle oxidative metabolism tended to prevent the accumulation of lipids in the muscle. The lard diet led to the development of IR, without an increase in the muscle lipid content, pointing out that the lipid quality (such as ceramides) and the FA composition of the muscle modulated insulin sensitivity rather than the tissue lipid accumulation itself. The fish-oil diet failed to prevent hepatic steatosis and the high level of PUFA in this diet made the tissues more prone to oxidation, and thus there is a risk for the transformation of liver steatosis into non-alcoholic steatohepatitis. These results clearly show that the dietary intake of SFA should be reduced, and precaution should be taken when advising a high unphysiological intake of PUFA-rich products such as fish oils.

Supplementary material

To view supplementary material for this article, please visit http://dx.doi.org/10.1017/S0007114513001311

Acknowledgements

The authors acknowledge Drs Alain Grynberg and Délphine Rousseau (INRA, Paris) for their assistance, whose advices were important for diet conception and preparation. The authors also thank the staff of the animal facilities for animal use. The present study received no specific grant from any funding agency in the public, commercial or not-for-profit sectors.

C. F.-C. and C. C. designed the research; C. F.-C., M. A., G. F., B. B. and J. R. conducted the research, C. F.-C., M. A., F. C., J. P. C. and C. C. analysed the data; C. F.-C. wrote the paper and had responsibility for the final content. All the authors read and approved the final manuscript.

The authors declare that there is no conflict of interest.

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Figure 0

Table 1 Body weight and weight gain, dietary and energy intakes and plasma glucose, lipid, insulin and leptin levels (Mean values and standard deviations, n 8)

Figure 1

Fig. 1 Liver histology after haematoxylin/eosin staining of liver sections from representative rats of each group: (A) 5 % basal diet; (B) 5 % lard-rich diet; (C) 5 % fish oil-rich diet; (D) 30 % basal diet; (E) 30 % lard-rich diet; (F) 30 % fish oil-rich diet. Original magnification 100 × .

Figure 2

Table 2 Liver lipids and oxidative stress parameters (Mean values and standard deviations, n 8)

Figure 3

Table 3 Total fatty acid (FA) composition of the liver homogenates (mg FA/g tissue)* (Mean values and standard deviations, n 8)

Figure 4

Fig. 2 Liver protein expression of fatty acid translocase/cluster of differentiation 36 (FAT/CD36), fatty acid transport protein 4 (FATP4) and PPARγ co-activator 1α (PGC-1α), and liver gene expression of fatty acid-binding protein 1 (FABP1), liver carnitine palmitoyltransferase 1 (L-CPT1) and PPAR-α. (A) Western blot was performed on protein extracts from the liver of rats, using anti-FAT/CD36, anti-FATP4 and anti-PGC-1α antibodies. Anti-β-actin antibody was used to confirm equal loading. Western blot was quantified using ImageJ software (NIH). (B) Quantitative real-time PCR analysis of the mRNA expression of FABP, L-CPT1 and PPAR-α in the liver. Values are means (n 6–8), with standard deviations represented by vertical bars. (A) There was a significant effect of lipid quantity on FAT/CD36 and PGC-1α protein expression (P< 0·001). There was a significant effect of lipid quantity on FATP4 protein expression (P< 0·01) with a significant interaction between the quantity and quality of lipid (P< 0·05). (B) There was a significant effect of lipid quantity on FABP1 and L-CPT1 gene expression (P< 0·05). , Basal diet; , lard-rich diet; , fish oil-rich diet.

Figure 5

Fig. 3 Liver protein expression of stearoyl-CoA desaturase 1 (SCD1), fatty acid synthase (FAS) and phospho-acetyl-CoA carboxylase (p-ACC) and p-ACC:ACC ratio, and liver gene expression of malonyl CoA decarboxylase (MCD) and medium-chain acyl-CoA dehydrogenase (MCAD). (A) Western blot was performed on protein extracts from the liver of rats, using anti-SCD1, anti-FAS, anti-ACC and anti-p-ACC antibodies. Anti-β-actin antibody was used to confirm equal loading. Western blot was quantified using ImageJ software (NIH). (B) Quantitative real-time PCR analysis of the mRNA expression of MCD and MCAD in the liver. Values are means (n 6–8), with standard deviations represented by vertical bars. (A) There was a significant effect of lipid quantity and quality on SCD1 protein expression (P< 0·001, P< 0·05, respectively). There was a significant effect of lipid quantity on p-ACC and FAS protein expression (P< 0·001). (B) There was a significant effect of lipid quantity on MCAD gene expression (P< 0·05). , Basal diet; , lard-rich diet; , fish oil-rich diet.

Figure 6

Table 4 Muscle lipids and oxidative stress (Mean values and standard deviations, n 8)

Figure 7

Table 5 Total fatty acid (FA) composition of the muscle homogenates (mg FA/g tissue)* (Mean values and standard deviations, n 8)

Figure 8

Fig. 4 Muscle protein expression of fatty acid translocase/cluster of differentiation 36 (FAT/CD36), muscle carnitine palmitoyltransferase 1 (m-CPT1), stearoyl-CoA desaturase 1 (SCD1) and PPARγ co-activator 1α (PGC-1α). Western blot was performed on protein extracts from the muscle of rats, using anti-FAT/CD36, anti-m-CPT1, anti-SCD1 and anti-PGC-1α antibodies. Anti-β-actin antibody was used to confirm equal loading. Western blot was quantified using ImageJ software (NIH). Values are means (n 6–8), with standard deviations represented by vertical bars. There was a significant effect of lipid quantity on FAT/CD36 protein expression (P< 0·05) or almost significant effect on m-CPT1 (P= 0·051) and PGC-1α protein expression (P= 0·053). There was a nearly significant effect of lipid quality on SCD1 protein expression (P= 0·059) (fish oil v. mixed and lard diets. , Basal diet; , lard-rich diet; , fish oil-rich diet.

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