Numerous studies performed in experimental animals, mainly in rodents, have demonstrated the fat-lowering effect of the trans-10, cis-12 isomer of conjugated linoleic acid (CLA)(Reference Wang and Jones1–Reference Park and Pariza3). In contrast, the effectiveness of CLA on humans is controversial. Whereas some authors have observed reductions in body fat accumulation, others have not noticed this effect(Reference Larsen, Toubro and Astrup4–Reference Salas-Salvado, Marquez-Sandoval and Bullo6). Moreover, this effect, when it is observed, is less prominent than when it is found in rodents.
Various reasons could explain this difference between humans and rodents(Reference Navarro, Fernández-Quintela and Churruca7). One is related to the dose of CLA. Whereas in rodent experiments animals fed diets supplemented with 0·25–2 g CLA/100 g diet received CLA amounts close to 210–250 mg CLA/kg body weight, in human studies, volunteers received 1·4–6·8 g/d. For a 70 kg adult, this represents 20–97 mg CLA/kg body weight. These doses are clearly lower than those used in rodents.
Another important reason refers to age and maturity stage. It has been proposed that young animals and subjects are probably more responsive to CLA than adults, due to their growing status or to other metabolic situations. With regard to this issue it should be pointed out that while human studies have addressed adults, the vast majority of the experiments on rodents have been conducted with growing animals.
There is very little information concerning the effectiveness of CLA in adult animals which are not anabolic. Mirand et al. (Reference Mirand, Arnal-Bagnard and Mosoni8) and Faulconnier et al. (Reference Faulconnier, Arnal and Patureau Mirand9) reported that adult rats were not responsive to the fat-to-lean partitioning effect of CLA described in growing rats. In contrast, Park et al. (Reference Park, Albright and Storkson10) observed a significant reduction in adipose tissue weight (47 %) as well as in the percentage of body fat (45 %) in mature female mice fed a CLA mixture. In line with these results, Miner et al. (Reference Miner, Cederberg and Nielsen11) also found significant reductions in adipose tissue weight (50–67 %) in adult mice fed a CLA mixture. It could be hypothesised that the effect on ageing depends on animal species.
In a previous study we observed that adult hamsters were less responsive to CLA feeding than young hamsters(Reference Navarro, Miranda and Churruca12). Although the reasons justifying this fact still remain unclear, differences in some of the molecular mechanisms described as being responsible for the CLA body fat-lowering effect in young animals, such as lipogenesis and thermogenesis, can be hypothesised.
In adipose tissue the process of TAG synthesis, known as lipogenesis, occurs mainly through two different pathways: one of them is mediated by lipoprotein lipase (LPL) which is responsible for the release of NEFA derived from chylomicrons and VLDL-TAG(Reference Eckel13). The enzyme is synthesised and secreted by adipocytes, and anchored to the luminal surface of the capillary endothelial cells. The resulting NEFA and monoacylglycerols are then available for re-esterification and storage. Thus, LPL activity plays a key role in controlling lipid deposition in adipose tissue. The transcription of LPL is controlled by PPARγ, a transcriptional factor highly expressed in adipose tissue(Reference Kersten14). Its activation thus promotes lipid storage(Reference Khan and Vanden Heuvel15).
The alternative pathway for lipogenesis involves the synthesis of fatty acids from glucose and is known as de novo lipogenesis. The relative importance of these two pathways is mainly dependent on the diet. The transcription of genes encoding lipogenic enzymes, such as fatty acid synthase (FAS) and acetyl-CoA carboxylase (ACX), is controlled by a family of membrane-bound transcriptional factors designated as sterol regulatory element-binding proteins (SREBP)(Reference Pai, Guryev and Brown16). Three types of SREBP have been identified. It has been shown that SREBP-1a and SREBP-1c, both derived from a single gene, participate in the regulation of the gene expression of enzymes involved in fatty acid synthesis(Reference Shimano17, Reference Horton18).
An important component of energy expenditure is non-shivering thermogenesis which, in rodents, takes place mostly in brown adipose tissue and is based on the functionality of uncoupling protein-1 (UCP1), a member of the inner mitochondrial membrane transporters that allows the dissipation as heat of the proton gradient generated by the oxidation of nutrients, mainly fatty acids(Reference Himms-Hagen19). This protein allows heat production by uncoupling respiration from ATP synthesis.
Thus, in the present study we aimed to explore the effects of trans-10, cis-12-CLA on the activity and expression of lipogenic enzymes, as well as on the expression of their controlling transcriptional factors in adult hamsters. The effect on the thermogenin UCP1 in brown adipose tissue was also assessed.
Methods and procedures
Animals, diets and experimental design
The experiment was conducted with sixteen adult male Syrian Golden hamsters (aged 8 months; initial body weight 167 (sem 5) g) purchased from Harlan Ibérica (Barcelona, Spain) and its protocol was approved by the Animal Experimentation Ethics Committee of the University of the Basque Country. Animals were individually housed in polycarbonate metabolism cages (Techniplast Gazzada, Guguggiate, Italy), placed in an air-conditioned room (22 (sem 2) °C) with a 12 h light–dark cycle. All manipulations with animals were in accordance with the ‘Guide for the Care and Use of Laboratory Animals’ as promulgated by the National Institutes of Health. After a 6 d adaptation period, hamsters were randomly divided into two groups of eight animals each and fed for 6 weeks semi-purified high-fat diets consisting of 200 g casein/kg (Sigma, St Louis, MO, USA), 4 g l-methionine/kg (Sigma), 200 g wheat starch/kg (Vencasser, Bilbao, Spain), 404 g sucrose/kg (local market), 100 g palm oil/kg (Agra, Leioa, Spain), 30 g cellulose/kg (Vencasser), 1 g cholesterol/kg (Sigma), 4 g choline HCl/kg (Sigma), and supplemented with 0·5 % linoleic acid (used as a control) or 0·5 % trans-10, cis-12-CLA (Natural Lipids Ltd, Hovdebygda, Norway). Vitamin (11 g/kg) and mineral (40 g/kg) mixes were formulated according to American Institute of Nutrition (AIN)-93 guidelines(Reference Reeves, Nielsen and Fahey20) and supplied by ICN Pharmaceuticals (Costa Mesa, CA, USA). The experimental diets were freshly prepared once per week, gassed with N2 and stored at 0–4°C to avoid rancidity. All animals had free access to food and water. Food intake and body weight were measured daily.
At the end of the experimental period animals were killed under anaesthesia (chloral hydrate) by cardiac exsanguination. White adipose tissue from different anatomical locations (epididymal, perirenal and subcutaneous) and brown adipose tissue from the interscapular area (IBAT) were dissected, weighed and immediately frozen.
Enzyme activities
For total LPL activity determination, homogenates of subcutaneous adipose tissues (250 mg) were prepared in 750 μl of 10 mm-HEPES buffer (pH 7·5) containing 1 mm-dithiothreitol, 1 mm-EDTA, 250 mm-sucrose and heparin (2 g/l) and used as the enzyme source. Soluble protein in homogenates was determined using bovine serum albumin as the standard(Reference Bradford21). For heparin-releasable LPL (HR-LPL) activity determination, the enzyme source was obtained by incubating 250 mg subcutaneous adipose tissue in 750 μl of 10 mm-HEPES buffer (described above) at 37°C during 30 min. Enzyme activity was assessed following the method described by Nilsson & Schotz with modifications, as previously described(Reference Zabala, Churruca and Fernandez-Quintela22). LPL (total and HR-LPL) activity was calculated by subtracting non-LPL lipolytic activity in the presence of NaCl from the total lipolytic activity determined without NaCl. Total LPL activity was expressed as nmol oleate released/min per mg protein and HR-LPL as nmol oleate released/min per g tissue.
For FAS analysis, samples of subcutaneous adipose tissue (1·0 g) were homogenised in 2·5 ml of buffer (pH 7·6) containing 150 mm-KCl, 1 mm-MgCl2, 10 mm-N-acetyl-cysteine and 0·5 mm-dithiothreitol. After centrifugation at 100 000 g for 40 min at 4°C, the supernatant fraction was used for enzyme activity quantification that was performed by using the rate of malonyl-CoA-dependent NADPH oxidation, according to the method of Lynen(Reference Lynen23). Soluble protein in homogenates was determined using bovine serum albumin as the standard(Reference Bradford21). Enzyme activity was expressed as nmol NADPH consumed/min per mg protein.
Extraction and analysis of RNA and quantification by reverse transcription-polymerase chain reaction
Total RNA was isolated from 100 mg of either subcutaneous or perirenal adipose tissues using Trizol (Invitrogen, Carlsbad, CA, USA) according to the manufacturer's instructions. RNA samples were then treated with a DNA-free kit (Ambion; Applied Biosystems, Foster City, CA, USA) to remove any contamination with genomic DNA. The yield and quality of the RNA were assessed by measuring absorbance at 260, 270, 280 and 310 nm and by electrophoresis on 1·3 % agarose gels. A quantity of 1·5 μg of total RNA of each sample was reverse-transcribed to first-strand complementary DNA (cDNA) using an iScript™ cDNA Synthesis Kit (Bio-Rad, Hercules, CA, USA).
Relative ACX, FAS, SREBP-1a, SREBP-1c, LPL and PPARγ mRNA levels were quantified using real-time PCR with an iCycler™–MyiQ™ Real-time PCR Detection System (Bio-Rad). β-Actin mRNA levels were similarly measured and served as the reference gene.
SREBP-1c, LPL, PPARγ and β-actin were quantified by SYBR® Green chemical real-time PCR. A quantity of 0·1 μl of each cDNA was added to the PCR reagent mixture (SYBR® Green Master Mix; Applied Biosystems), with the upstream and downstream primers (300 nm each). The PCR parameters were as follows: initial 2 min at 50°C, denaturation at 95°C for 10 min followed by forty cycles of denaturation at 95°C for 15 s and combined annealing and extension at 60°C for 1 min for SREBP-1c, LPL and β-actin, and 63·5°C for 1 min for PPARγ.
ACX, FAS, SREBP-1a and β-actin were quantified by Taqman real-time PCR. A quantity of 1 μl of each cDNA was added to the PCR reagent mixture (Premix Ex Taq™; Takara Bio Inc., Shiga, Japan), with the upstream (200 nm-FAS, SREBP-1a and β-actin and 300 nm-ACX) and downstream (200 nm-ACX and β-actin and 300 nm-FAS and SREBP-1a) primers and probes (0·5 μm-β-actin, 2·5 μm-ACX and FAS and 5 μm-SREBP-1a). The PCR parameters were as follows: initial denaturation at 95°C for 5 s followed by forty cycles of denaturation at 95°C for 5 s and combined annealing and extension at 60·7°C for 30 s for ACX, 60°C for 60 s for FAS and SREBP-1a and 64°C for 30 s for β-actin.
Information concerning specific sense and antisense primers and probes is shown in Table 1. All sample mRNA levels were normalised to the values of β-actin and the results expressed as fold changes of threshold cycle (Ct) value relative to controls using the 2− ΔΔCt method(Reference Livak and Schmittgen24).
SREBP, sterol regulatory element-binding protein; LPL, lipoprotein lipase; ACX, acetyl-CoA carboxylase; FAM, 6-carboxyfluorescein; BHQ, black hole quencher; FAS, fatty acid synthase.
Uncoupling protein-1 Western blot analysis in interscapular brown adipose tissue
Samples of IBAT (100 mg) were homogenised with cellular PBS (150 mm-NaCl; 3 mm-KCl; 3 mm-NaH2PO4; 7·5 mm-Na2HPO4; 1 μm-phenylmethanesulfonylfluoride; 10 μm-iodoacetamide; pH 7·4) and their protein concentration was determined by using the Bradford method(Reference Bradford21). Protein (30 μg) was separated by SDS–PAGE in a 10 % gel at 150 V for 1 h, and was electrotransferred to a polyvinylidene difluoride membrane (Bio-Rad) at 90 V during 70 min. Blots were blocked with 5 % powdered non-fat milk in PBS with 0·1 % Tween-20 (PBS–Tween) for 1 h and incubated with specific rabbit antibodies against UCP1 (1:3000) (SC-6529; Santa Cruz Biotechnology, Inc., Santa Cruz, CA, USA).
Blots were washed in PBS–Tween and incubated with anti-rabbit horseradish peroxidase-conjugated secondary antibody (1:20 000) for 1 h. After that, blots were washed in PBS–Tween and developed by chemiluminescent detection using a standard kit (ECL Kit; Amersham plc, Little Chalfont, Bucks, UK). Band intensity was measured by densitometric scanning (Bio-Rad GS-700 Imaging Densitometer) and analysed with Multi-Analyst/PC 1.1 software (Bio-Rad). Monoclonal anti-mouse β-actin (Amersham NA931VS, dilution 1:2000) antibody was used as a loading control to normalise the signal obtained for brown adipose tissue UCP1.
Statistical analysis
Results are presented as mean values with their standard errors. Statistical analysis was performed using SPSS (version 13.0; SPSS Inc., Chicago, IL, USA). Data were analysed by Student's t test. Statistical significance was set up at the P < 0·05 level.
Results
Body weight, food intake and white adipose tissue weights
As we previously reported(Reference Miranda, Fernández-Quintela and Churruca25), no significant differences either in food intake or in final body weight were found between both experimental groups. Hamsters fed the trans-10, cis-12-CLA diet showed reduced epididymal ( − 12·3 %) and perirenal ( − 18·4 %) adipose tissue weights, but this effect did not reach statistical significance. In contrast, subcutaneous fat pad weights were significantly lower in hamsters after CLA feeding ( − 21·0 %; P < 0·05) (Fig. 1).
Enzyme and transcription factor expressions in adipose tissues
No significant changes were induced by CLA feeding either in the expression of lipogenic enzymes (ACX and FAS) or in the expression of the transcriptional factors regulating their activity, SREBP-1a and SREBP-1c (Table 2). With regard to LPL, the same situation was found; no changes were observed in the expression of the enzyme, or in PPARγ (Table 2). This lack of changes refers to both subcutaneous and perirenal adipose tissues.
LA group, group fed a linoleic acid diet, used as a control; CLA group, group fed a conjugated linoleic acid-supplemented diet; LPL, lipoprotein lipase; ACX, acetyl-CoA carboxylase; FAS, fatty acid synthase; SREBP, sterol regulatory element-binding protein.
* Results are shown as mRNA levels expressed as arbitrary units.
Enzyme activities in subcutaneous adipose tissue
CLA feeding did not induce significant changes in HR-LPL activity (2·87 (sem 0·65) nmol oleate released/min per g tissue in the linoleic acid group v. 3·08 (sem 0·65) nmol oleate released/min per g tissue in the CLA group). Moreover, no significant changes were observed between both experimental groups in total LPL or FAS activities (Fig. 2).
Interscapular brown adipose tissue weight and uncoupling protein-1 protein content
Although no differences between both experimental groups were found in IBAT weight (0·35 (sem 0·03) g in the linoleic acid group v. 0·33 (sem 0·01) g in the CLA group), trans-10, cis-12-CLA induced a significant increase in the amount of UCP1 (P < 0·05) (Fig. 3).
Discussion
It has been widely demonstrated that trans-10, cis-12-CLA induces a strong reduction in body fat accumulation in rodents. The extent to which this CLA isomer reduces adipose tissue size depends on several factors, such as the animal species. Thus, the sensitivity of rodents to CLA is as follows: mouse>hamster>rat(Reference Kelley and Erickson26–Reference Pariza28). Another factor suggested to alter CLA effectiveness is the age of the animals or subjects(Reference Wahle, Heys and Rotondo29). Nevertheless, little is known about this issue because the vast majority of the studies performed on rodents have used young, growing animals and information concerning the effects of CLA in adult animals is scarce.
In order to address this issue, we designed the present experiment for adult hamsters by using the same experimental protocol as that used in a previous study by our laboratory, carried out using young (aged 9 weeks) hamsters. In that study, trans-10, cis-12-CLA significantly reduced adipose tissue from perirenal (24–29 %; P < 0·01), epididymal (21–31 %; P < 0·05) and subcutaneous (30–43 %; P < 0·001) locations(Reference Zabala, Churruca and Fernandez-Quintela22, Reference Navarro, Zabala and Macarulla30). In contrast, in the present study, the response of adult hamsters to trans-10, cis-12-CLA feeding was weaker because only the subcutaneous depot was significantly reduced (21 %; P < 0·05). Perirenal and epididymal depots were reduced (18 and 12 %, respectively), but this effect did not reach statistical significance. These results are quite similar to those found in adult rats as compared with young rats(Reference Mirand, Arnal-Bagnard and Mosoni8, Reference Faulconnier, Arnal and Patureau Mirand9).
As indicated in the introduction section, numerous studies performed in experimental animals, mainly in rodents, have demonstrated strong reductions of body fat induced by trans-10, cis-12-CLA. However, the effects in human subjects, when these are observed, are less prominent. It must be pointed out that whereas human studies have addressed adults, the vast majority of the experiments performed with rodents have been conducted on growing animals. Taking into account the reduced effectiveness of CLA observed in adult hamsters in the present study, and in adult rats(Reference Mirand, Arnal-Bagnard and Mosoni8, Reference Faulconnier, Arnal and Patureau Mirand9), it is feasible that one of the reasons explaining the reduced response in human subjects is the adulthood of volunteers.
Several mechanisms of action have been proposed to explain the body fat-lowering effect of CLA. A considerable consensus has been reached concerning the reduction in adipose tissue LPL-mediated fat uptake. Reduced LPL activity in 3T3-L1 adipocytes after supplementation with CLA in the culture medium has been reported in several papers(Reference Park, Albright and Liu31–Reference Park, Storkson and Liu34). In in vivo studies Lin et al. (Reference Lin, Kreeft and Schuurbiers35) observed that trans-10, cis-12-CLA inhibited HR-LPL and Xu et al. (Reference Xu, Storkson and Kim36) reported a significant reduction in both HR-LPL and intracellular LPL activities in adipose tissue from mice fed a diet supplemented with a 0·5 % CLA mixture for a very short experimental period (4 d). Accordingly, in our previous study performed in young hamsters, trans-10, cis-12-CLA significantly reduced total and HR-LPL activity, as well as its expression(Reference Zabala, Churruca and Fernandez-Quintela22). This reduction in LPL resulted in diminished adipose tissue size and explained, in part, the body fat-lowering action of this CLA isomer.
In the present study we analysed the effects of trans-10, cis-12-CLA on LPL and its regulating transcriptional factor PPARγ expression in adipose tissue, to determine the potential involvement of this enzyme in the reduction of CLA effectiveness observed in adult hamsters, when compared with young hamsters. Due to the fact that subcutaneous adipose tissue, but not the perirenal depot, was significantly reduced by CLA, these expressions were measured in both fat pads in order to find potential tissue-specific differences. Although the CLA group showed reduced values in LPL expression, this difference did not reach statistical significance (P = 0·12 for perirenal adipose tissue and P = 0·50 for subcutaneous adipose). No significant changes were found in PPARγ expression in both depots.
Because, as stated before, subcutaneous adipose tissue was significantly reduced, we also measured total and HR-LPL activity in order to find any potential post-transcriptional enzyme activation. No changes in LPL activity were observed. These results suggest that the lack of CLA effect on LPL expression and activity may be one reason that explains the reduced CLA body fat-lowering effect observed in adult hamsters.
With regard to the effects of CLA on adipose tissue lipogenesis, conflicting results have been reported when either enzyme activities or expression were assessed. West et al. (Reference West, Blohm and Truett37) observed increased fatty acid synthesis, despite a significant reduction in adipose tissue weight, in growing mice fed a 1 % CLA mixture. Increased lipogenic enzyme activities, without changes in adipose tissue size, were reported in adult rats fed 1 % trans-10, cis-12-CLA for 6 weeks by Faulconnier et al. (Reference Faulconnier, Arnal and Patureau Mirand9). Further, Kang et al. (Reference Kang, Miyazaki and Ntambi38) found an increase in FAS mRNA induced by 0·2 % trans-10, cis-12-CLA feeding for 4 weeks in mice. In contrast, Azain et al. (Reference Azain, Hausman and Sisk39) did not find changes in FAS activity induced by CLA feeding in rats and other authors found reduced expression of FAS and ACX in mice(Reference Tsuboyama-Kasaoka, Takahashi and Tanemura40, Reference Clement, Poirier and Niot41).
In our previous study performed in young animals, trans-10, cis-12-CLA feeding significantly reduced the mRNA expressions of ACX and FAS(Reference Zabala, Churruca and Fernandez-Quintela22). In the present study, a tendency towards higher values in the expression of lipogenic enzymes in the perirenal depot was observed (P = 0·09) in the CLA group. Nevertheless, changes were not statistically significant in any of the two analysed depots. In line with these data, the expression of SREBP-1a and SREBP-1c, which are the transcriptional factors controlling these two enzymes, remained unchanged. As stated above in this discussion, the subcutaneous was the most sensitive depot. Considering that FAS expression was increased almost two-fold in the CLA group when compared with the linoleic acid group, the activity of this enzyme was assessed in the subcutaneous fat pad, showing no statistical differences.
Taken as a whole, these results suggest that CLA intake affects adipose tissue lipid metabolism in adult hamsters in a different way to young ones. This fact can explain the differences observed in both age groups in terms of CLA effectiveness.
In addition to the direct effects of trans-10, cis-12-CLA on adipose tissue metabolic pathways, other mechanisms have been proposed to explain its body fat-lowering effect. A negative energy balance due to increased energy expenditure may play a role(Reference Pariza, Park and Cook42–Reference Ryder, Portocarrero and Song44). IBAT in rodents plays a major role in controlling body weight through diet-induced thermogenesis. This is primarily mediated by the uncoupling of mitochondrial respiration resulting from the marked oxidative capacity of brown adipocytes. To find an explanation justifying the reduction in body fat observed in adult hamsters, in the present study we decided to analyse the effect of trans-10, cis-12-CLA on UCP1 in IBAT. We observed that the animals fed this CLA isomer showed significantly increased amounts of this thermogenin. This effect can result in increased thermogenesis, leading to body fat decrease.
The results published concerning these effects are not very consistent(Reference West, Blohm and Truett37, Reference Tsuboyama-Kasaoka, Takahashi and Tanemura40, Reference Ryder, Portocarrero and Song44–Reference Choi, Jung and Park49). Ealey et al. (Reference Ealey, El-Sohemy and Archer45) found significantly lower UCP1 protein levels in brown adipose tissue from mice fed a 1 % CLA mixture compared with controls but increased levels in CLA-fed rats, showing that regulation of UCP by CLA occurs in different manners depending on the animal species. The present results are in good accordance with those found in rats. Nevertheless, in order to make comparisons between these two studies and the present study, it is important to emphasise that whereas we used trans-10, cis-12-CLA, the body fat-lowering active isomer, Ealey et al. (Reference Ealey, El-Sohemy and Archer45) used a CLA mixture.
In conclusion, these results demonstrate that adult hamsters show little responsiveness to trans-10, cis-12-CLA, which is lower than that observed in young hamsters. One of the reasons explaining this difference is the lack of effect on LPL. More studies are needed to better characterise the effects of CLA on adult animals and to find the reasons explaining this reduction in CLA effect induced by ageing.
Acknowledgements
The present study was supported by grants from the Ministerio de Educación y Ciencia (AGL2005-02 494), Gobierno Vasco (GIC07/120-IT-265-07; CTP 05/R5), University of País Vasco (GIU06/82) and CYTED (Programa Iberoamericano de Ciencia y Tecnología para el desarrollo). J. M. is a recipient of a doctoral fellowship from the Ministerio de Educación y Ciencia. Palm oil was a generous gift from Agra-Unilever Foods España S.A. (Leioa, Spain).
The contributions of each author were as follows: V. M. R. and E. S. carried out UCP1 Western blot analysis in IBAT; J. M. and I. C. performed RNA quantification by real-time RT-PCR; A. F.-Q. measured LPL enzyme activity; A. F.-Q. and M. T. M. carried out the bibliography revision; M. P. P. supervised the results and manuscript writing.
No conflicts of interest are reported by any of the authors.