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n-3 and n-6 Polyunsaturated fatty acids suppress sterol regulatory element binding protein activity and increase flow of non-esterified cholesterol in HepG2 cells

Published online by Cambridge University Press:  14 October 2009

Mattia Di Nunzio
Affiliation:
Department of Biochemistry ‘G. Moruzzi’, Research Centre on Nutrition and Vitamins, University of Bologna, Via Irnerio 48, 40126Bologna, Italy
Diederik van Deursen
Affiliation:
Department of Biochemistry, Cardiovascular Research School COEUR, Erasmus MC, PO Box 2040, NL-3000 CARotterdam, The Netherlands
Adrie J. M. Verhoeven
Affiliation:
Department of Biochemistry, Cardiovascular Research School COEUR, Erasmus MC, PO Box 2040, NL-3000 CARotterdam, The Netherlands
Alessandra Bordoni*
Affiliation:
Department of Biochemistry ‘G. Moruzzi’, Research Centre on Nutrition and Vitamins, University of Bologna, Via Irnerio 48, 40126Bologna, Italy
*
*Corresponding author: Dr Alessandra Bordoni, fax +39 051 2091235, email [email protected]
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Abstract

The plasma lipid-lowering effect of PUFA, one of their main beneficial effects, is considered to be related to the regulation of lipid biosynthesis through transcription factors including sterol regulatory element binding proteins (SREBP). In the present study, we compared the effect of different PUFA on SREBP activity in HepG2 cells, using a sterol regulatory element–luciferase reporter construct as a probe. Supplementation with different fatty acids reduced SREBP activity in the order 20 : 5n-3 = 18 : 2n-6 = 20 : 4n-6≫18 : 3n-3 = 22 : 6n-3 = 22 : 5n-6≫18 : 1n-9. The suppression of SREBP activity greatly depended on the degree of incorporation of the supplemented PUFA into cellular lipids, and correlated positively with the unsaturation index (r 0·831; P < 0·01) of total cell lipids. Supplemented PUFA were also metabolised to longer and more unsaturated species. These processing activities were higher for n-3 than n-6 PUFA (P < 0·01). We studied the effect of PUFA on the intracellular distribution of non-esterified cholesterol, using filipin staining and fluorescence microscopy with or without the cholesterol traffic blocker U18666A. The data show that the incorporation of PUFA increases non-esterified cholesterol flow from the plasma membrane to intracellular membranes. We conclude that suppression of SREBP activity by PUFA depends on the degree of incorporation into cellular lipids, and is associated with increased flow of non-esterified cholesterol between the plasma membrane and intracellular membranes.

Type
Full Papers
Copyright
Copyright © The Authors 2009

It is well documented that dietary intake of PUFA, and particularly a correct n-6:n-3 ratio, contributes to the prevention of many chronic diseases(Reference Simopoulos1). In order to explain how PUFA can influence so many biological processes, different mechanisms of action have been hypothesised, i.e. the modification of membrane fluidity and functionality through changes in membrane lipid composition(Reference Rajamoorthi, Petrache and McIntosh2), the alteration of eicosanoid signalling and the modulation of gene expression(Reference Worgall and Deckelbaum3Reference Sampath and Ntambi5). Their main beneficial effect, i.e. plasma lipid lowering, is nowadays considered to be related to the regulation of lipid biosynthesis through the transcription factors NF-κB(Reference Zhao, Joshi-Barve and Barve6), retinoid X receptor(Reference Lengqvist, Mata De Urquiza and Bergman7), PPAR(Reference Edwards and O'Flaherty8) and sterol regulatory element binding proteins (SREBP)(Reference König, Spielmann and Haase9).

PUFA are thought to interact indirectly with SREBP(Reference Nakamura, Cheon and Li10, Reference Bordoni, Di Nunzio and Danesi11), but the mechanism of this interaction is still unclear. It is unlikely that PUFA affect SREBP through liver X receptor (LXR), a major activator of SREBP-1c transcription, as fish oil-fed rats showed suppression of hepatic SREBP-1c target genes, but not of LXR target genes such as cytochrome P450 family 7 subfamily A polypeptide 1 (CYP7A1), ATP-binding cassette (ABC)-G5 or ABC-G8 transporters(Reference Pawar, Botolin and Mangelsdorf12). In addition, in hepatocytes the treatment with EPA (20 : 5n-3) inhibited SREBP-1c-controlled genes both in the absence and the presence of a synthetic LXR agonist(Reference Nakatani, Katsumata and Miura13). Alternatively, PUFA may act by decreasing SREBP mRNA stability(Reference Hannah, Ou and Luong14, Reference Jump15). A recent study showed that DHA (22 : 6n-3) reduces the abundance of the nuclear form of SREBP-1 (nSREBP-1) in rat hepatocytes through 26S-proteasome- and Erk-dependent pathways(Reference Botolin, Wang and Christian16).

Another possibility is that the SREBP suppression is linked to the incorporation of PUFA into cell membranes. Cholesterol is abundant in mammalian plasma membranes (PM), accounting for as much as 50 % (mol/mol) of total lipid. It globally modulates the molecular organisation of the membrane, and its distinct affinity for different lipids drives the formation of membrane subdomains(Reference Silvius17). When PUFA are incorporated to a greater extent into membrane phospholipids, their poor affinity for cholesterol drives the formation of PUFA-enriched and cholesterol-depleted subdomains(Reference Stillwell, Shaikh and Zerouga18). Since maturation of SREBP is regulated by the non-esterified cholesterol (NEC) content of the endoplasmic reticulum membranes(Reference Weber, Boll and Stampfl19), it is conceivable that PUFA inhibit SREBP processing by causing redistribution of NEC from the PM to the endoplasmic reticulum.

To test this hypothesis, we supplemented HepG2 cells with different concentrations of various PUFA, and we compared the degree of their incorporation into cell lipids with the activity of SREBP, measured by using a sterol regulatory element–luciferase (SRE-luc) construct as a probe. Furthermore, the distribution of NEC over the PM and intracellular membranes was assessed by fluorescence microscopy. We chose HepG2 cells as the model system since the liver plays a central role in the regulation of cholesterol homeostasis.

Methods and materials

Materials

Dulbecco's modified Eagle's medium and Dulbecco's PBS were purchased from Lonza (Breda, The Netherlands), and Reporter Gene assay lysis buffer from Roche (Almere, The Netherlands). Fetal calf serum and Lipofectamine Plus were from Invitrogen (Groningen, The Netherlands), and U18666A and fatty acids from Sigma (St Louis, MO, USA). All other chemicals and solvents were of the highest analytical grade. The SRE-luc reporter construct was generated by insertion of part of the hamster hydroxy-3-methylglutaryl-CoA synthase promoter region into pGL3-Basic(Reference Botma, van Deursen and Vieira20). pGAP-RL (a kind gift from Dr A. A. F. de Vries, Leiden, The Netherlands) contained part of the human glyceraldehyde 3-phosphate dehydrogenase (GAP) promoter, and was generated by insertion of the 0·5 kb HindIII-XhoI fragment of pGAP489CAT(Reference Aki, Yanagisawa and Akanuma21) into pRL-null.

Methods

HepG2 cells tissue culture

HepG2 human hepatoma cells were maintained in Dulbecco's modified Eagle's medium supplemented with 10 % (v/v) fetal calf serum, penicillin (100 IU/ml) and streptomycin (100 μg/ml) at 37°C, 95 % air, 5 % CO2. Once per week, cells were split 1:10 into a new 75 cm2 flask; medium was refreshed once per week.

Fatty acid supplementation

Fatty acids were dissolved at different concentrations (6, 60 and 120 μm, w/v) in 100 % isopropanol, and bound to bovine serum albumin (BSA). Fatty acid–BSA complexes were prepared fresh each time at a final BSA concentration of 0·5 % (in serum-free Dulbecco's modified Eagle's medium), and cells were incubated for 21 h with fatty acids. Final isopropanol concentration in the media was kept below 1 % (v/v). Control cells received corresponding amounts of BSA and isopropanol.

Determination of HepG2 fatty acid composition

Cells were seeded in six-well plates. After 24 h, at 75–80 % confluence, cells were supplemented with fatty acid–BSA complexes at 60 μm-fatty acid concentration. After 21 h, cells were washed four times with ice-cold Dulbecco's PBS, scraped off and collected by centrifugation for 3 min at 1000 g and 4°C. Total cellular lipids were extracted according to Folch et al. (Reference Folch, Lees and Sloane Stanley22), and methyl esterified according to Stoffel et al. (Reference Stoffel, Chu and Ahrens23). The fatty acid composition (as methyl esters) was determined by GC (GC 8000; Fisons, Milan, Italy) using a capillary column (SP 2340; 0·2 μm film thickness) at a programmed temperature gradient (160–210°C; 8°C/min) as previously reported(Reference Bordoni, Angeloni and Leoncini24).

Luciferase assay

Cells were seeded in twenty-four-well plates. After 24 h, at 75–80 % confluence, cells were transfected with SRE-luc (0·4 μg per well) and pGAP-RL (60 ng per well) using Lipofectamine Plus as described previously(Reference Botma, van Deursen and Vieira20). After 3 h, the medium was refreshed and supplemented with fatty acids at 6, 60 and 120 μm (w/v) concentrations. After 21 h, cells were washed three times with ice-cold Dulbecco's PBS and lysed. Luciferase activity was determined in the cell extracts with the Dual-Glo luciferase assay kit (Promega, Leiden, The Netherlands) using a Packard Top Count NXT luminometer (Packard Instruments Co., Inc., Meriden, CT, USA). Data were normalised for Renilla activity measured in the same sample to account for differences in cell viability and transfection efficiency. At 120 μm-PUFA, Renilla expression levels were similar for the different fatty acids used, and amounted to 5721 (sd 471) counts (n 4) v. 6115 (sd 1986) counts (n 4) without fatty acid supplementation (P = 0·713; paired t test).

Filipin staining

HepG2 cells were seeded on coverslips. After 24 h, cells at about 20 % confluence were supplemented with 60 μm-fatty acid–BSA complex. In some experiments U18666A (2 μg/ml), a blocker of intracellular cholesterol trafficking(Reference Härmälä, Pörn and Mattjus25), was also added. Cells were washed after 21 h incubation, and fixated using 3 % paraformaldehyde in Dulbecco's PBS for 60 min. Thereafter, the cells were washed three times, treated with 50 mm-glycine in Dulbecco's PBS for 30 min to quench paraformaldehyde, and stained with filipin (40 μg/ml) for a further 30 min. Coverslips were mounted on microscope slides and the epifluorescence was examined using an inverted Olympus IX50 microscope. Images were acquired and analysed using AnalySiS imaging software (Soft Imaging Systems, Münster, Germany) as previously described(Reference Lim, Bijvelds and Nigg26).

Statistical analysis

Data are presented as mean values and standard deviations of at least three independent experiments. Differences were tested for statistical significance by unpaired Student's t tests (P < 0·05).

Results

The incorporation of supplemented PUFA into cell lipids was determined by GC (Table 1). All PUFA were readily incorporated at the expense of MUFA, while the molar content of SFA was not significantly affected. When incubated with linoleic acid (LA; 18 : 2n-6), α-linolenic acid (ALA; 18 : 3n-3), arachidonic acid (ARA; 20 : 4n-6) or EPA, the corresponding elongated and more unsaturated fatty acids accumulated as well, suggesting that these PUFA are further metabolised upon cellular uptake. Metabolic conversion of the n-3 fatty acids was more efficient than the n-6 fatty acids. In fact in LA-supplemented cells the products:precursor ratio was 0·29 (sd 0·04), compared with 0·70 (sd 0·13) in ALA-supplemented cells (P < 0·01). Supplementation with oleic acid (OA; 18 : 1n-9) did not result in significant changes in the relative content of OA, nor of any of the other fatty acids.

Table 1 Fatty acid composition (mol %) of HepG2 cells in the control condition and after PUFA supplementation

(Mean values and standard deviations for three independent experiments)

OA, oleic acid; LA, linoleic acid; ARA, arachidonic acid; DPA, docosapentaenoic acid; ALA, α-linolenic acid.

Mean value was significantly different from that of the control cells: * P < 0·05, ** P < 0·01, *** P < 0·001.

Cells were incubated for 21 h with 60 μm-fatty acids.

The effect of n-6 and n-3 PUFA on SRE-luc activity in HepG2 cells is shown in Fig. 1(a) and (b), respectively. PUFA were supplemented at a very low concentration (6 μm) and at two physiological plasma concentrations (60 and 120 μm). Data were compared with the effects of corresponding concentrations of OA. OA did not cause any reduction of SRE-luc activity at 6 μm, and only a mild reduction at 60 μm. At 6 μm, LA and ARA reduced SRE-luc activity by 50 % (Fig. 1(a)). Maximal inhibition of 75 % was observed at 60 and 120 μm. Docosapentaenoic acid (22 : 5n-6) had no effect at the low concentration, while its inhibitory effect was similar to LA and ARA at 120 μm. Among n-3 PUFA (Fig. 1(b)), EPA appeared as effective as LA and ARA at all concentrations used. In contrast, the inhibitory effect of ALA and DHA was apparent only at 60 and 120 μm.

Fig. 1 Effect of n-6 and n-3 PUFA supplementation on sterol regulatory element–luciferase (SRE-luc) activity. HepG2 cells were incubated for 21 h with different concentrations of n-6 (a) and n-3 (b) fatty acids, and the effect on SRE-luc activity was determined. Fatty acids used were linoleic acid (□), arachidonic acid (⋄), docosapentaenoic acid (●), α-linolenic acid (○), EPA (▾) and DHA (▲). The effects of PUFA were compared with similar concentrations of oleic acid (■). Data are expressed as percentage of control from three separate experiments each performed in quadruplicate. Values are means, with standard deviations represented by vertical bars. Mean value was significantly different from that of the control cells: * P < 0·05, ** P < 0·01, *** P < 0·001.

We then compared the degree of cellular lipid modification with the inhibition of SRE-luc activity obtained in 60 μm-PUFA-supplemented cells. Interestingly, the more a supplemented fatty acid or its metabolites were incorporated into total cellular lipids, the stronger was its effect on SRE-luc activity. An inverse correlation was present between SRE-luc activity and the total PUFA content of cellular membranes (r − 0·79; P = 0·02) (Fig. 2(a)), and between SRE-luc activity and the unsaturation index of total cellular lipids (r − 0·83; P < 0·01) (Fig. 2(b)). It is therefore evident that the enrichment of PUFA in HepG2 cells is correlated with the degree of suppression of SREBP activity.

Fig. 2 Correlations (—) between sterol regulatory element–luciferase (SRE-luc) activity and cell membrane fatty acid composition. Cells were incubated for 21 h without (*) or with 60 μm-fatty acids. Fatty acids used were oleic (■), linoleic (□), arachidonic (⋄), docosapentaenoic (●), α-linolenic (○), eicosapentaenoic (▾) and docosahexaenoic (▲) acids. Total lipid fatty acid composition was obtained by GC, as reported in Table 1. Unsaturation index (UI) was obtained by multiplying the relative molar content of each fatty acid by its number of double bonds, then adding up all obtained values. Values on PUFA content (a) or UI (b) and SRE-luc activity are means, with standard deviations represented by horizontal and vertical bars, respectively. SRE-luc activity negatively correlated with PUFA content (r − 0·79; P = 0·02) and UI (r − 0·83; P < 0·01).

To evaluate the intracellular distribution of NEC in HepG2 cells, filipin staining followed by fluorescence microscopy was performed in control and 60 μm-fatty acid–BSA-supplemented cells. In control cells, NEC appeared to be mainly localised at the cell periphery, in proximity to the PM, with a low intracellular staining intensity (Fig. 3(a)). The relative distribution of cholesterol was not affected by any of the supplemented PUFA, as illustrated for EPA in Fig. 3(b). Cholesterol is continuously transported from the PM to intracellular membranes, and vice versa. To estimate the effect of PUFA on the flow of cholesterol from the PM to intracellular membranes, we used U18666A, an inhibitor of cholesterol export from endo- and lysosomes(Reference Härmälä, Pörn and Mattjus25). In the presence of U18666A, filipin staining at the cell periphery was markedly reduced (Fig. 3(c)). Simultaneously, intracellular staining appeared as small clusters of bright spots, indicating that NEC is confined to intracellular organelles. The NEC that accumulated in the intracellular organelles apparently reflects the amount of NEC that has been transported from the PM during incubation with U18666A. When cells were co-incubated with U18666A and EPA (Fig. 3(d)), intracellular staining increased further and the cell periphery also stained strongly (compare Fig. 3(c) and (d)). Compared with U18666A alone, the number and size of the intracellular staining spots were markedly increased. The increased intracellular accumulation of NEC in EPA-supplemented cells indicates increased flow of cholesterol from the PM to endo- and lysosomes.

Fig. 3 Effect of EPA and U18666A on non-esterified cholesterol distribution in HepG2 cells. Cells were incubated for 21 h without (a, c) or with 60 μm-bovine serum albumin-bound EPA (b, d), and without (a, b) or with U18666A (2 μg/ml) (c, d), and then stained for non-esterified cholesterol by filipin. Data are representative of three independent experiments.

Discussion

It is 40 years since Keys & Parlin(Reference Keys and Parlin27) developed predictive equations to quantify the effects of fatty acids and dietary cholesterol on plasma cholesterol concentrations, and dietary PUFA were reported as important regulators of cholesterol metabolism. It is widely accepted that PUFA modulate the expression of genes involved in lipid metabolism, and SREBP have emerged as key mediators of this regulation. Nevertheless, the exact mechanism(s) by which PUFA interact with SREBP is still unclear, as well as the effectiveness of different n-6 and n-3 PUFA. To clarify this, we supplemented HepG2 cells with both n-6 and n-3 PUFA, while the monounsaturated OA was used for comparison.

The degree of incorporation of supplemented PUFA and their metabolites appeared to be an important determinant of their inhibitory effect on SREBP activity. In fact, the more they were incorporated into total cellular lipids, the lower was SREBP activity. This is further illustrated by the inverse correlation between SREBP activity and the unsaturation index of cellular lipids. It is therefore evident that suppression of SREBP activity by PUFA in HepG2 cells depends on the degree of their enrichment in cellular lipids. Supplementation with 60–120 μm-PUFA reduced SREBP activity in the order EPA = LA = ARA≫ALA = DHA = docosapentaenoic acid. In a recent review Jump et al. (Reference Jump, Botolin and Wang28) indicated DHA as the most active PUFA in modulating hepatic gene transcription and the most potent suppressor of SREBP-1 nuclear abundance. Actually, in rat primary hepatocytes, DHA was more effective than EPA but ineffective below 100 μm in reducing nSREBP-1 protein(Reference Botolin, Wang and Christian16). Worgall et al. (Reference Worgall, Sturley and Seo29) found that LA, ARA, ALA and docosapentaenoic acid were similarly effective in HepG2 cells at 300 μm; EPA and DHA were not included in this study. In rat hepatoma cells, ARA, EPA and DHA (150 μm) were more effective in suppressing nSREBP-1 protein than LA and ALA (300 μm)(Reference Le Jossic-Corcos, Gonthier and Zaghini30). These differences in efficacy may be due to the different experimental models or the different PUFA:albumin ratios used. In addition, the reporter assay used in the present study does not discriminate between SREBP isoforms, and some PUFA may also suppress nSREBP-2.

Supplemented PUFA were not only incorporated into cell lipids as such, but they were also converted to longer and more unsaturated species by the HepG2 cells. This is in contrast to Yu-Poth et al. (Reference Yu-Poth, Yin and Kris-Etherton31) but in agreement with El-Badry et al. (Reference El-Badry, Graf and Clavien32). In accordance with this last paper, we found these processing activities to be higher for n-3 than n-6 PUFA, as indicated by the higher product:precursor ratios for 18 : 3n-3 than 18 : 2n-6.

Our fluorescence microscopy studies are consistent with an increased flow of NEC from the PM to intracellular membranes in PUFA-supplemented HepG2 cells. It is conceivable that incorporation of PUFA displaces cholesterol from the PM, thus increasing NEC flow to intracellular membranes. In the PM cholesterol is associated with sphingomyelin(Reference Worgall, Sturley and Seo29). In HL-60 cells and human neutrophils, the increase in PUFA concentration stimulates neutral sphingomyelinase activity(Reference Jayadev, Linardic and Hannun33, Reference Robinson, Hii and Poulos34). Treatment of cultured cells with sphingomyelinase, thereby degrading the major raft sphingolipids, leads to a rapid increase in intracellular cholesterol content and subsequent inhibition of SREBP maturation(Reference Simons and Ikonen35). In control cells, NEC appeared to be mainly localised at the cell periphery, in proximity to the PM, with a low intracellular localisation. The similar staining pattern observed in PUFA-supplemented cells argues against a major re-distribution of NEC from the PM to intracellular membranes. However, cholesterol in the PM is continuously turning over and it is estimated that the entire PM cholesterol pool cycles to the endoplasmic reticulum and back with a half-time of 40 min(Reference Liscum and Munn36). Therefore, suppression of SREBP activity may result from subtle increases in intracellular NEC not detectable by filipin staining. However, in the presence of U18666A, which inhibits NEC basal movements, the increased accumulation of NEC in intracellular organelles strongly suggests increased trafficking of cholesterol between the PM and intracellular compartments. Hence, it may be the NEC dynamics in the intracellular membranes rather than the NEC concentration that affects the post-translational maturation of SREBP.

Taken together, our data suggest that both n-3 and n-6 PUFA suppress SREBP activity in HepG2 cells via the increased flow of NEC from the PM to intracellular membranes, in proportion to their accumulation in cellular lipids. Besides, the regulation of SREBP activity by PUFA may also involve other mechanisms, such as sphingomyelin hydrolysis and consequent ceramide production(Reference Worgall, Johnson and Seo37), PPAR activation(Reference König, Koch and Spielmann38), and accelerated degradation of nSREBP by a 26S proteasome-dependent pathway(Reference Botolin, Wang and Christian16), mechanisms that may or may not be secondary to PUFA incorporation into cellular membranes. Lowering of liver SREBP-1 protein levels by PUFA-enriched oil feeding has been consistently reported for rats and mice(Reference Botolin, Wang and Christian16, Reference Sekiya, Yahagi and Matsuzaka39Reference Xu, Cho and O'Malley40), suggesting that our findings may hold also in vivo. Although additional studies are needed to elucidate how PUFA control SREBP activity, and thereby lipid metabolism, our data may contribute to the further development of PUFA as nutritional therapeutic agents for management of cholesterol and lipid homeostasis.

Acknowledgements

The authors would like to thank Dick H. W. Dekkers, Christina H. Lim and Ben C. Tilly for their helpful discussion, and Granarolo SpA (Bologna, Italy) for the financial support.

Part of the present study was supported by grants from the Programma Marco Polo, University of Bologna (M. di N.), the Dutch Heart Foundation (grant no. 2001B174) and Granarolo SpA (Bologna, Italy).

M. Di N. and D. v. D. performed the analysis. A. J. M. V. and A. B. designed and supervised the study, and wrote the paper.

All authors state that there is no conflict of interest associated with the present study.

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Figure 0

Table 1 Fatty acid composition (mol %) of HepG2 cells in the control condition and after PUFA supplementation†(Mean values and standard deviations for three independent experiments)

Figure 1

Fig. 1 Effect of n-6 and n-3 PUFA supplementation on sterol regulatory element–luciferase (SRE-luc) activity. HepG2 cells were incubated for 21 h with different concentrations of n-6 (a) and n-3 (b) fatty acids, and the effect on SRE-luc activity was determined. Fatty acids used were linoleic acid (□), arachidonic acid (⋄), docosapentaenoic acid (●), α-linolenic acid (○), EPA (▾) and DHA (▲). The effects of PUFA were compared with similar concentrations of oleic acid (■). Data are expressed as percentage of control from three separate experiments each performed in quadruplicate. Values are means, with standard deviations represented by vertical bars. Mean value was significantly different from that of the control cells: * P < 0·05, ** P < 0·01, *** P < 0·001.

Figure 2

Fig. 2 Correlations (—) between sterol regulatory element–luciferase (SRE-luc) activity and cell membrane fatty acid composition. Cells were incubated for 21 h without (*) or with 60 μm-fatty acids. Fatty acids used were oleic (■), linoleic (□), arachidonic (⋄), docosapentaenoic (●), α-linolenic (○), eicosapentaenoic (▾) and docosahexaenoic (▲) acids. Total lipid fatty acid composition was obtained by GC, as reported in Table 1. Unsaturation index (UI) was obtained by multiplying the relative molar content of each fatty acid by its number of double bonds, then adding up all obtained values. Values on PUFA content (a) or UI (b) and SRE-luc activity are means, with standard deviations represented by horizontal and vertical bars, respectively. SRE-luc activity negatively correlated with PUFA content (r − 0·79; P = 0·02) and UI (r − 0·83; P < 0·01).

Figure 3

Fig. 3 Effect of EPA and U18666A on non-esterified cholesterol distribution in HepG2 cells. Cells were incubated for 21 h without (a, c) or with 60 μm-bovine serum albumin-bound EPA (b, d), and without (a, b) or with U18666A (2 μg/ml) (c, d), and then stained for non-esterified cholesterol by filipin. Data are representative of three independent experiments.