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Effects of similar intakes of marine n-3 fatty acids from enriched food products and fish oil on cardiovascular risk markers in healthy human subjects

Published online by Cambridge University Press:  15 September 2011

Bente Kirkhus*
Affiliation:
Nofima AS, Norwegian Institute of Food, Fisheries and Aquaculture Research, Osloveien 1, 1430Ås, Norway Mills DA, Oslo, Norway
Amandine Lamglait
Affiliation:
Mills DA, Oslo, Norway
Karl-Erik Eilertsen
Affiliation:
Faculty of Biosciences, Fishery and Economics, University of Tromsø, Tromsø, Norway
Eva Falch
Affiliation:
Mills DA, Oslo, Norway
Trond Haider
Affiliation:
Link Medical Research AS, Oslo, Norway
Hogne Vik
Affiliation:
Aker BioMarine Antarctic AS, Oslo, Norway
Nils Hoem
Affiliation:
Aker BioMarine Antarctic AS, Oslo, Norway
Tor-Arne Hagve
Affiliation:
Department of Medical Biochemistry, Oslo University Hospital, Rikshospitalet, Oslo, Norway Center of Laboratory Medicine, Akershus University Hospital, Lørenskog, Norway
Samar Basu
Affiliation:
Department of Public Health and Caring Sciences, Uppsala University, UppsalaSE-755 85, Sweden Laboratoire de Biochimie, Biologie Moléculaire et Nutrition, Faculté de Pharmacy, Université d'Auvergne, 28 Place Henri-Dunant, 63001Clermont-Ferrand, France
Elisabeth Olsen
Affiliation:
Denomega Nutritional Oils, Sarpsborg, Norway
Ingebjørg Seljeflot
Affiliation:
Department of Cardiology, Oslo University Hospital, Ullevål, Oslo, Norway
Lena Nyberg
Affiliation:
Skånemejerier, Malmø, Sweden
Elisabeth Elind
Affiliation:
Faculty of Health, Nutrition and Management, Akershus University College, Kjeller, Norway
Stine M. Ulven
Affiliation:
Faculty of Health, Nutrition and Management, Akershus University College, Kjeller, Norway
*
*Corresponding author: Dr B. Kirkhus, fax +47 64 97 03 33, email [email protected]
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Abstract

There is convincing evidence that consumption of fish and fish oil rich in long-chain (LC) n-3 PUFA (n-3 LCPUFA), EPA (20 : 5n-3) and DHA (22 : 6n-3) reduce the risk of CHD. The aim of the present study was to investigate whether n-3 LCPUFA-enriched food products provide similar beneficial effects as fish oil with regard to incorporation into plasma lipids and effects on cardiovascular risk markers. A parallel 7-week intervention trial was performed where 159 healthy men and women were randomised to consume either 34 g fish pâté (n 44), 500 ml fruit juice (n 38) or three capsules of concentrated fish oil (n 40), all contributing to a daily intake of approximately 1 g EPA and DHA. A fourth group did not receive any supplementation or food product and served as controls (n 37). Plasma fatty acid composition, serum lipids, and markers of inflammation and oxidative stress were measured. Compared with the control group, plasma n-3 LCPUFA and EPA:arachidonic acid ratio increased equally in all intervention groups. However, no significant changes in blood lipids and markers of inflammation and oxidative stress were observed. In conclusion, enriched fish pâté and fruit juice represent suitable delivery systems for n-3 LCPUFA. However, although the dose given is known to reduce the risk of CVD, no significant changes were observed on cardiovascular risk markers in this healthy population.

Type
Full Papers
Copyright
Copyright © The Authors 2011

The health benefits of long-chain (LC) n-3 PUFA (n-3 LCPUFA) of marine origin, in particular EPA (20 : 5n-3) and DHA (22 : 6n-3), are well documented, indicating protective effects on CVD, autoimmune and mental disorders(Reference Harris1Reference Appleton, Rogers and Ness5). n-3 LCPUFA appear to reduce the risk of CVD through a wide range of beneficial effects, including anti-atherothrombogenic effect and reduction in serum TAG, whereas there are some inconsistencies regarding the effects on arrhythmia, hypertension and inflammation(Reference Valagussa, Franzosi and Geraci6Reference Myhrstad, Retterstol and Telle-Hansen17). However, n-3 LCPUFA are prone to oxidation, which may lead to increased susceptibility to oxidation and atherogenicity of LDL-cholesterol, and increased risk of CVD(Reference Suzukawa, Abbey and Howe18Reference Turner, McLean and Silvers20). High levels of F2-isoprostanes, formed from the free radical-induced peroxidation of membrane-bound arachidonic acid (AA, 20 : 4n-6), have been associated with higher cardiovascular risk(Reference Basu21Reference Kim, Hyun and Jang24). Still, the role of n-3 LCPUFA in oxidative stress is unclear.

In the literature, recommended daily intakes of n-3 LCPUFA vary from 200 mg to 1 g EPA and DHA(Reference Kris-Etherton and Hill25). Recent evidence shows that the intake of EPA and DHA is inversely related to cardiovascular risk in a dose-dependent manner up to about 250 mg/d in healthy populations, and intake of 1 g/d is associated with a marked protection from sudden cardiac death(Reference Mozaffarian2, Reference Valagussa, Franzosi and Geraci6, Reference Rupp, Wagner and Rupp26, 27). A growing market for n-3 LCPUFA-fortified foods may provide recommended amounts for people whose diet is inadequate. However, whether consumption of such products provides the same health benefits as fish consumption or fish oil supplementation has to be established. There is an ongoing discussion about the preferred ‘delivery system’ for n-3 fatty acids, i.e. food v. supplement, with respect to bioavailability and physiological function. The molecular form of the lipids, the food matrix and possible interactions with other food components may have an impact on the absorption and incorporation of EPA and DHA into plasma lipids. Some studies have indicated that fish consumption is more effective in increasing serum concentrations of n-3 LCPUFA than fish oil(Reference Visioli, Rise and Barassi28, Reference Elvevoll, Barstad and Breimo29), whereas others have shown almost identical increases when comparing equal intakes of EPA and DHA from fish and capsules(Reference Harris, Pottala and Sands30). In a single-meal study, fish oil incorporated into food products was absorbed differently from the same fish oil in capsules, and the rate of absorption varied depending on the food matrix(Reference Schram, Nielsen and Porsgaard31). Both level and type of emulsifiers and phospholipids in foods may influence lipid bioavailability(Reference Mun, Decker and McClements32); still, it is unclear whether steady-state levels of plasma EPA and DHA, obtained after regular daily intake, are also influenced by the food matrix.

In a previous intervention study, intake of fish pâté enriched in EPA and DHA indicated efficient incorporation into blood lipids and favourable effects on inflammatory markers(Reference Elvevoll, Eilertsen and Brox33). In the present study, the same fish pâté and n-3 LCPUFA-enriched fruit juice were compared with fish oil with regard to incorporation into plasma lipids and effects on cardiovascular risk markers, e.g. serum lipids, plasma fatty acid profile, and markers of inflammation and oxidative stress. The aim was to investigate whether n-3 LCPUFA-enriched food products provide similar beneficial effects as fish oil when consuming 1 g/d EPA and DHA, a recommended intake known to reduce the risk of CVD.

Experimental methods

Participants

Participants were recruited by local advertising in the community of Akershus, Norway. Men and women, aged 18–70 years, with normal to slightly increased cholesterol and TAG levels (total cholesterol < 7·5 mmol/l and TAG < 4·0 mmol/l) and C-reactive protein ( < 10 mg/l) were included. Exclusion criteria were regular fatty fish consumption (>1/week of salmon, trout, herring, sardine and mackerel), diagnosis of familial hypercholesterolaemia, secondary hyperlipidaemia, chronic rheumatoid disease, coronary, peripheral or cerebrovascular disease within the previous 3 months of inclusion, BMI ≥ 30 kg/m2, hypertension ( ≥ 160/100 mmHg), use of medication to lower serum lipids, blood pressure and inflammation, pregnancy and lactation. Subjects who used n-3 LCPUFA supplements regularly were asked to terminate the use of supplements 2 months before inclusion (n 19). The 2 months washout period was considered appropriate based on the reduced level of EPA and DHA in serum cholesteryl esters reported previously during washout after n-3 supplementation(Reference Katan, Deslypere and vanBirgelen34). The study was conducted according to the guidelines in the Declaration of Helsinki and approved by the regional Ethics Committee. Written informed consent was obtained from all participants. A validated FFQ(Reference Andersen, Nes and Lillegaard35) was used in order to check the background diet of the subjects. All subjects, including the control group, were instructed by a nutritionist not to change their habitual diet (including changes in fatty fish intake and use of n-3 supplements), to keep a stable weight and not to change their lifestyle during the intervention period. The intervention period did not include summer or Christmas holidays.

Study design

The study was part of a larger study, which has been published previously(Reference Ulven, Kirkhus and Lamglait36). It was a single-centre intervention study with an open, randomised, parallel-group design conducted at the Akershus University College, Kjeller, Norway. Intervention products to be tested were n-3 LCPUFA-enriched fish pâté, n-3 LCPUFA-enriched fruit juice and concentrated fish oil in capsules. In total, 369 phone calls were received and 207 subjects were invited to a screening visit (visit 1). Subjects eating fatty fish regularly more than once per week were excluded at the phone interviews. Screening of subjects (n 199) was performed within 3 weeks before inclusion in order to identify subjects who satisfied the eligibility criteria (n 179). The evaluation conducted at screening included assessment of C-reactive protein and serum lipids. Demographic information (age, sex and ethnicity), concomitant medication and medical history were registered, and a brief physical examination (weight, height and blood pressure) was conducted. Subjects who satisfied the eligibility criteria (n 179) were randomised into four study groups. Before the baseline visit (visit 2), nine subjects were lost, whereas eleven subjects dropped out during the study period. In the n-3 LCPUFA-enriched fruit juice group, two subjects did not manage to consume the product, in the n-3 LCPUFA-enriched fish pâté group there were five dropouts (two did not manage to eat the product, two got clinical symptoms such as stomach pain and nausea and one was lost to follow-up) and in the control group four subjects were lost to follow-up. A total of 159 subjects finished the study, and they had consumed either 500 ml n-3 LCPUFA-enriched fruit juice (n 38), 34 g n-3 LCPUFA-enriched fish pâté (n 44) or three capsules of fish oil (n 40) daily for 7 weeks in order to obtain an intake of approximately 1 g/d EPA and DHA (Table 1). A control group that did not receive any products (n 37) was included to account for seasonal variation. The participants were advised to include fish pâté and fruit juice in meals where they commonly used bread or a beverage and the capsules to be consumed at breakfast or other regular meals. All products were delivered free of charge. At the end of the 7-week intervention period, the subjects met for a final visit (visit 3). Blood and urine samples were collected at visits 2 and 3 for assessments of efficacy. A change in concomitant medication and smoking habits from baseline and clinical symptoms during the intervention period were registered in the case report form at each visit. In total, eighteen subjects were using a stable dose of hormonal contraceptives before and during the study, and eight subjects were using drugs against allergies. The number of subjects taking medication was equally distributed among the study groups. The total number of smokers was eighteen. The number of cigarettes per d varied among the subjects (from 1 up to 20 per d), but the number was stable for each subject before and during the study. Compliance was ensured through regular telephone contact with the participants and monitored by collecting leftover study products and empty containers at visit 3. Compliance was satisfactory in all groups; 94 % in the fish pâté group, 100 % in the juice group and 100 % in the fish oil group.

Table 1 Fatty acid composition of the study products (percentage of fatty acids)

AA, arachidonic acid; DPA, docosapentaenoic acid.

Products

Fish pâté was based on a commercial product manufactured by Mills DA, Oslo, Norway. The main ingredients were farmed Atlantic salmon (Salmo salar), rapeseed oil, water and fish oil (refined cod-liver oil; Denomega Nutritional Oils, Sarpsborg, Norway). Fish oil was added to increase the contents of DHA and EPA to about twice the natural content. The product was gently processed under carefully controlled conditions, high-temperature pasteurised and packed in Al tubes. Fruit juice was based on concentrates of fruits and berries, with no sugar added. It was developed and delivered by Mills DA, in collaboration with Skånemejerier, Malmø, Sweden, where it was produced by adding fish oil (refined cod-liver oil; Denomega Nutritional Oils) through a patented technique (patent no. Norge 325446, ‘Lipid composition and use thereof’). Fish oil capsules (Peter Møllers Dobbel, Axellus, Norway) were a commercial food supplement of concentrated fish oil (TAG). The capsules were made of gelatine softened with glycerol. All intervention products were obtained from large-scale production and subjected to regular in-house quality tests, including routine sensory analysis and analysis of peroxide value. Sensory analysis was performed by a panel consisting of company employees specially trained to detect oxidative attributes such as rancidity. The participants were told to keep the food products refrigerated in order to ensure oxidative stability throughout the shelf-life period. Fish oil capsules were stored at room temperature. The fatty acid composition of the study products is presented in Table 1. Fatty acid content was analysed by The Norwegian Institute for Food and Environmental Analysis Inc. (Oslo, Norway) using a modified Caviezel method(Reference Pendl, Bauer and Caviezel37). Lipids were extracted using a modified Bligh & Dyer method(Reference Bligh and Dyer38). Fatty acid concentrations were determined by GLC of fatty acid methyl esters on a fused-silica wall-coated capillary column (Chrompack CP-Wax-52 CB, 25 mm × 0·25 mm) in a Perkin-Elmer Auto System XL (Perkin Elmer Inc., Waltham, MA, USA).

Blood sampling

Blood from venepuncture was collected after an overnight fast ( ≥ 12 h). Subjects were instructed to refrain from alcohol consumption and from vigorous physical activity the day before the blood sampling. Serum was obtained from silica gel tubes (BD Vacutainer, Plymouth, Devon, UK), kept at room temperature for at least 30 min until centrifugation at 1300 g for 12 min. Plasma was obtained from EDTA tubes (BD Vacutainer) kept on ice and centrifuged at 1300 g for 10 min at 10°C within 2 h. Samples were kept frozen ( − 80°C) until analysis.

Serum lipids and apolipoproteins

Analyses of serum total-, LDL- and HDL-cholesterol, TAG, apoA1, and apoB were performed at the routine laboratory at the Department of Medical Biochemistry at Oslo University Hospital, Rikshospitalet, Oslo, Norway (ISO 17 025 accredited), using standard methods (Modular System; Roche, Mannheim, Germany).

Plasma fatty acid composition and vitamin E (α-tocopherol)

Plasma fatty acid composition was analysed by Jurilab Limited, Kuopio, Finland, which used a slight modification of the method described by Nyyssonen et al. (Reference Nyyssonen, Kaikkonen and Salonen39). Plasma (250 μl) fatty acids and 25 μl of an internal standard (eicosane 1 mg/ml in isopropanol) were extracted with 6 ml of methanol–chloroform (1:2) and 1·5 ml of water were added. The two phases were separated by centrifugation and the upper phase was discarded. To the chloroform phase, 1 ml of methanol–water (1:1) was added, and this extraction was repeated twice. The chloroform phase was evaporated under N2. For methylation, the remainder was treated with 1·5 ml of sulphuric acid–methanol (1:50) at 85°C for 2 h. The mixture was diluted with 1·5 ml of water and extracted with light petroleum diethyl ether. The fatty acids from the diethyl ether phase were determined using a 6890 GC with an HP-5MS capillary column and interfaced with a 5973 mass selective detector with electron impact ionisation (Agilent Technologies, Palo Alto, CA, USA). For retention time and quantitative standardisation, fatty acids purchased from Nu-Chek-Prep (Elysian, MN, USA) were used.

Plasma α-tocopherol was analysed by Vitas AS, Oslo, Norway. Briefly, 100 μl of human plasma were diluted with 300 μl 2-propanol containing the internal standard tocol and butylated hydroxytoluene (BHT) as an antioxidant. After thorough mixing (15 min) and centrifugation (10 min, 4000 g at 10°C), an aliquot of 1 μl was injected from the supernatant into the HPLC system. HPLC was performed with an HP 1100 liquid chromatograph (Agilent Technologies) with an HP1100 fluorescence detector, an emission wavelength of 295 nm and an excitation wavelength of 330 nm. Tocopherol isomers were separated on a 2·1 mm × 250 mm reversed phase column. The column temperature was 40°C. A two-point calibration curve was made from an analysis of a 3 % albumin solution enriched with a known concentration of tocopherols. Recovery is >95 %, the method is linear from at least 1 to 200 μm and the limit of detection is 0·01 μm.

Circulating inflammatory markers

Analysis of serum high-sensitivity C-reactive protein was performed at the routine laboratory at the Department of Medical Biochemistry at Rikshospitalet (ISO17025 accredited), using a standard method (Modular System; Roche). Plasma IL-6, TNFα, monocyte chemotactic protein-1, interferon-γ, soluble E-selectin and P-selectin, soluble intracellular adhesion molecule-1 and vascular cell adhesion molecule-1 were determined by Fluorokine® MAP kits from R&D Systems, Inc. (Minneapolis, MN, USA). Plasma leukotriene B4 was analysed as described previously(Reference Elvevoll, Barstad and Breimo29). Due to low sensitivity by the multiplex method, IL-6 and TNFα were measured using ELISA (R&D Systems).

Urinary F2 isoprostanes

Spot morning urine samples were analysed for 8-iso-PGF by a highly specific and validated RIA as described by Basu(Reference Basu40). The cross-reactivity of the 8-iso-PGF antibody with 15-keto-13,14-dihydro-8-iso-PGF, 8-iso-PGF, PGF, 15-keto-PGF, 15-keto-13,14-dihydro-PGF, thromboxane B-2, 11β-PGF, 9β-PGF and 8-iso-PGF, respectively, was 1·7, 9·8, 1·1, 0·01, 0·01, 0·1, 0·03, 1·8 and 0·6 %. The detection limit of the assay was 23 pmol/l. Glomerular filtration rate was assessed as equal to the clearance of creatinine and the urinary levels of 8-iso-PGF were adjusted according to creatinine concentration.

Statistical methods

Statistical analyses were performed by LINK Medical Research AS (Oslo, Norway), an independent clinical research organisation contracted for partaking in the conduct of the project. Analyses were performed using SAS® for Windows (version 9.1; SAS Institute Inc., Cary, NC, USA). The nominal level for significance was 5 %. The power calculation was based on observed variations in TAG in a previous parallel study(Reference Elvevoll, Eilertsen and Brox33). Sample size calculations based on testing a null hypothesis of no difference, using a power of 0·80 and a significance level of 0·05, resulted in the need of including at least forty participants in each group (SAS® Power and Sample Size). This sample size was derived by using an estimated standard deviation of change from baseline of 0·485 mmol/l, and an assumed expected mean change of 0·30 mmol/l in all groups except the control group that was assumed to have a difference of zero. Due to the potential of participants dropping out of the study, it was decided to include fifty subjects per treatment. The participants were recruited during a period of 1 year. Due to a lower dropout rate than expected, only 179 subjects were recruited. Continuously distributed parameters were analysed by ANOVA. Box plots were checked for deviations between the groups that could severely affect the estimated P values. However, none was found. Whenever the ANOVA test resulted in rejecting the null hypothesis of no difference between the groups, the Scheffé multiple-comparison procedure based on CI was used(41). Within-group changes from baseline to the end of intervention were tested by paired Students t tests. All values are presented as means and standard deviations, unless otherwise stated. In order to detect potential associations between incorporation of DHA and EPA into plasma lipids, the plasma EPA:AA ratio and changes in cardiovascular risk markers, principal component analysis and cross-correlations were performed using Unscrambler® version 9.8 (Camo Inc., Oslo, Norway).

Results

Overall, 179 subjects were randomised into four groups, and 159 completed the study in accordance with the descriptions given in the protocol. Baseline demographics and clinical characteristics of the study groups are given in Table 2. No differences were observed between the groups. There were no changes in BMI and blood pressure during the intervention period.

Table 2 Baseline characteristics and plasma lipids

(Mean values and standard deviations)

BP, blood pressure.

* Based on the ANOVA test using means (percentage for sex).

Plasma fatty acid profile and serum lipids

Significant differences in change from baseline between the groups were seen for EPA, docosapentaenoic acid (22 : 5n-3), DHA and the EPA:AA ratio, demonstrating that the control group had a significantly (P < 0·05) smaller change than the three intervention groups (Table 3). Also, significant within-group increases in plasma levels of EPA, docosapentaenoic acid and DHA, and decreased levels of AA were seen in all intervention groups, and the EPA:AA ratio increased markedly (Table 3). EPA increased with 113, 144 and 145 %, respectively, in the fruit juice, fish pâté and fish oil capsule groups. The increases in DHA were somewhat lower, 31, 38 and 50 %, whereas AA decreased with 9, 2 and 7 %, respectively, in the fruit juice, fish pâté and fish oil capsule groups. Also, compared with the control group, the increases in EPA, docosapentaenoic acid and DHA were statistically significant, but pairwise comparisons between the three intervention groups gave no significant results. However, the lowest increase in EPA and DHA was observed in the fruit juice group that had the lowest intake (Table 1). There were only minor changes in other plasma fatty acids (Table 3).

Table 3 Fatty acid levels in plasma (μmol/l)

(Mean values and standard deviations)

* Test of within-group changes (paired t test).

Test of the null hypothesis of no difference in change from baseline between the groups (ANOVA).

Mean change from baseline was significantly different for control group than for the other three groups (P < 0·05).

The changes seen in the levels of total cholesterol, HDL-cholesterol, LDL-cholesterol and TAG were limited (Table 4). There was a trend showing an increase in HDL (5–7 %) in the fruit juice, fish pâté and fish oil capsule groups (P = 0·06–0·07). This was in accordance with an observed increase in apoA (P = 0·01–0·06; Table 3). Although a few within-group changes were statistically significant, no statistically significant differences in changes between the groups were observed.

Table 4 Serum lipids (mmol/l)

(Mean values and standard deviations)

* Test of within-group changes (paired t test).

Test of the null hypothesis of no difference in change from baseline between the groups (ANOVA).

Inflammatory markers

There were no significant changes in the serum inflammatory markers high-sensitivity C-reactive protein, IL-6, TNFα, leukotriene B4, monocyte chemotactic protein-1, intracellular adhesion molecule-1, vascular cell adhesion molecule-1, E-selectin and P-selectin (Table 5). A significant within-group increase was observed for interferon-γ in the fruit juice, fish pâté and fish oil capsule groups, but there were no significant differences between the groups (Table 5).

Table 5 Serum high sensitive C-reactive protein (hsCRP) and plasma inflammatory markers

(Mean values and standard deviations)

ICAM, intracellular adhesion molecule; MCP-1, monocyte chemotactic protein-1; INFγ, interferon-γ.

* Test of within-group changes (paired t test).

Test of the null hypothesis of no difference in change from baseline between the groups (ANOVA).

Markers for oxidative stress

No significant changes in the urine levels of F2-isoprostane between the study groups were observed (Table 6). The plasma level of vitamin E (α-tocopherol) decreased in all groups, including the control group. When calculated in relation to the level of serum TAG, the decrease was statistically significant only in the fish pâté group (Table 6). No significant changes in the plasma levels of α-tocopherol were observed between the groups.

Table 6 Markers of oxidative stress

(Mean values and standard deviations)

* Test of within-group changes (paired t test).

Test of the null hypothesis of no difference in change from baseline between the groups (ANOVA).

Principal component analysis and cross-correlation

Principal component analysis and cross-correlations revealed no convincing associations between incorporation of DHA and EPA into plasma lipids and markers of inflammation and oxidative stress, or between the plasma EPA:AA ratio and markers of inflammation and oxidative stress (data not shown).

Discussion

The present randomised, parallel designed intervention study showed that intake of n-3 LCPUFA in the form of TAG from fortified foods and concentrated fish oil capsules contributed equally to significant increases in plasma concentrations of EPA and DHA. Still, no significant effects were observed in parameters associated with CVD such as serum lipids and markers of inflammation or oxidative stress.

The increase in plasma EPA varied from 113 to 145 % among the intervention groups, whereas the increase in DHA varied from 31 to 50 %. However, differences between the groups were not significant, indicating that fish oil capsules, enriched fruit juice and fish pâté represent equivalent sources of dietary EPA and DHA. The assumption that fish intake is more effective in increasing plasma levels of EPA and DHA than fish oil(Reference Visioli, Rise and Barassi28, Reference Elvevoll, Barstad and Breimo29) was not confirmed in the present study (Table 3). About 50 % of the intake of EPA and DHA in the fish pâté group originated from fish (salmon) and should therefore contribute to higher levels in plasma. However, the present results suggest that incorporation of EPA and DHA into plasma lipids, measured after 7 weeks of supplementation, is independent of the food matrix. This is in accordance with other studies of fortified foods, including foods added with microencapsulated fish oil(Reference Mantzioris, Cleland and Gibson42Reference Earnest, Hammar and Munsey48). In the present study, the incorporation of EPA and DHA into plasma lipids was somewhat lower, still not significantly lower, in the fruit juice group than in the fish oil group (Table 3), although intakes were quite similar (Table 1). As compliance was satisfactory in all groups, we have no explanation for the lower incorporation of EPA and DHA after consumption of fruit juice and further research is needed to confirm whether components in fruit juice influence the uptake of fatty acids. Moreover, it cannot be excluded that small variations in product content could have influenced the results. The present results also show that the increase in plasma EPA is larger than the increase in plasma DHA in all groups, despite similar intakes of EPA and DHA (Table 1). This is in accordance with previous studies(Reference Visioli, Rise and Barassi28, Reference Elvevoll, Barstad and Breimo29, Reference Elvevoll, Eilertsen and Brox33, Reference Katan, Deslypere and vanBirgelen34, Reference Metcalf, James and Mantzioris45), and may be explained by a more strict biological regulation of DHA levels.

The increase in plasma EPA and DHA observed in the intervention groups seemed to be paralleled by a decrease in AA (Table 3), resulting in a marked increase in the EPA:AA ratio. Elevated blood levels of n-3 LCPUFA and the EPA:AA ratio, and, in particular, a high percentage of EPA and DHA in erythrocyte membranes (omega-3 index) have been associated with a reduced risk of sudden cardiac death(Reference Harris1, Reference Rupp, Wagner and Rupp26, Reference Albert, Campos and Stampfer49, Reference von Schacky and Harris50). However, despite a marked increase in plasma n-3 LCPUFA and the EPA:AA ratio in the present study, no significant effects were observed in parameters known to be associated with CVD such as serum lipids, markers of inflammation and oxidative stress. Neither did multivariate analyses reveal any strong associations between the EPA:AA ratio and any of the measured parameters. The omega-3 index was not measured in the present study, but future studies should examine whether n-3 LCPUFA-enriched food products providing a daily dose of 1 g EPA and DHA is sufficient to achieve the recommended omega-3 index associated with a reduced risk of CVD(Reference Harris1, Reference von Schacky and Harris50).

There were no significant effects on serum lipids with the dose given (1 g/d EPA and DHA), confirming that higher intakes of 2–4 g/d may be needed to induce significant reductions in normolipaemic individuals(Reference Kris-Etherton and Hill25, Reference Harris51, Reference Kris-Etherton, Harris and Appel52). The reductions seem to depend on the baseline level and are more frequently observed in hypertriacylglycerolaemic persons and CVD patients(Reference Valagussa, Franzosi and Geraci6, Reference Harris51, Reference Seierstad, Seljeflot and Johansen53), which may explain why no change was observed in the present study, which included only healthy volunteers with normal TAG levels. Some studies have shown an increase in HDL-cholesterol levels after the intake of n-3 LCPUFA(Reference Harris51, Reference Balk, Lichtenstein and Chung54). In the present study, only a weak indication of positive modulation of HDL was observed (Table 4). The lack of the effects on LDL-cholesterol and serum cholesterol is as expected, assuming that n-3 LCPUFA have a minor effect on serum cholesterol(Reference Harris51). The lack of effect of the intervention products on serum cholesterol could also be confirmed using serum cholesterol-predictive equations(Reference Muller, Kirkhus and Pedersen55).

The urine levels of F2-isoprostane did not increase significantly in any of the study groups (Table 6), indicating no changes in oxidative stress. The α-tocopherol levels, on the other hand, tended to decrease from baseline in all groups, and more in the intervention groups compared with the control group, but no significant between-group variations were found. Some studies have shown that intakes of EPA and DHA may reduce oxidative stress(Reference von Schacky56), whereas others have indicated no effect(Reference Tholstrup, Hellgren and Petersen57), or even increased in vivo lipid peroxidation and increased oxidative stress(Reference Stalenhoef, de Graaf and Wittekoek58, Reference Harats, Dabach and Hollander59). The conflicting results may be due to differences in experimental design and different products used. Both dosage and balancing with appropriate intakes of antioxidants seem to be of major importance for the outcome.

We have no explanation for the observed increase in interferon-γ levels (Table 5). There was no effect on the great majority of the measured inflammatory markers, and this is in accordance with a large body of evidence indicating that healthy subjects are relatively insensitive to immunomodulation with n-3 LCPUFA even at intakes that substantially raise their concentrations in phospholipids of immune cells(Reference Schmidt, Arnesen and de Caterina60Reference Hallund, Madsen and Bugel64). A recent study by Micallef et al. (Reference Micallef, Munro and Garg65), however, has indicated that in healthy individuals, plasma n-3 fatty acid concentration is inversely related to high-sensitivity C-reactive protein concentration. No such correlation was found in the present study. Moreover, results from the present study are apparently in contrast to an identically designed previous study where intake of the same fish pâté resulted in significant decreases in inflammatory markers (IL-6, TNFα, leukotriene B4 and monocyte chemotactic protein-1) in lipopolysaccharide-stimulated whole blood(Reference Elvevoll, Eilertsen and Brox33). The different results may be due to healthy subjects generally having low levels of circulating inflammatory markers, which makes it hard to detect small changes, whereas with lipopolysaccharide stimulation, much higher measurable levels of the markers are obtained. The intervention period in both studies was 7 weeks, which should ensure sufficient incorporation of n-3 LCPUFA into the cell membranes(Reference Harris, Pottala and Sands30, Reference Katan, Deslypere and vanBirgelen34). Incorporation into the membranes of immune cells may influence their function and the way they respond to external signals(Reference Calder13, Reference Yaqoob66). Whether lipopolysaccharide stimulation is relevant with respect to the in vivo situation needs further investigation and future studies should test the hypothesis that exposure to pathological conditions, such as lipopolysaccharide stimulation, is necessary to reveal the immunomodulatory effects of n-3 LCPUFA associated with CVD prevention in healthy individuals.

A weakness of the study is that we cannot rule out that group sizes were too small to detect significant effects on markers of inflammation and oxidative stress. Another weakness is that the study was not blinded. The participants received very different products and this was difficult to hide. In order to avoid confounding factors such as effects of seasonal variation and whether participation itself affected the measured parameters, we included a control group that did not consume any marine n-3 supplements or changed their fatty fish intake during the study. A nutritionist carefully instructed them. Also, high baseline n-3 LCPUFA plasma concentrations could diminish the effects. Regular fatty fish consumers were therefore not included in the study and all participants were told to terminate their intake of n-3 LCPUFA supplements 2 months before inclusion(Reference Katan, Deslypere and vanBirgelen34). Hence, baseline values were somewhat lower in the present study. Still, plasma n-3 LCPUFA calculated as a percentage of total fatty acids were similar to other studies and the observed increases in n-3 LCPUFA were within the same range as observed by others(Reference Visioli, Rise and Barassi28, Reference Elvevoll, Eilertsen and Brox33, Reference Zhang, Wang and Li67, Reference Rosell, Lloyd-Wright and Appleby68).

In conclusion, the present study shows that concentrated fish oil in capsules, enriched fruit juice and fish pâté represent suitable delivery systems for EPA and DHA, i.e. the efficiency of the incorporation into plasma lipids was independent of the food matrix. Fruit juice and fish pâté were safe, well tolerated and highly palatable, representing feasible alternatives to meet the nutritional recommendations. Fruit juice can be advised for individuals who do not favour fish or fish oil capsules. The products effectively increase plasma n-3 LCPUFA content and the EPA:AA ratio. However, significant effects on serum lipids and markers of inflammation and oxidative stress were not observed in this healthy population.

Acknowledgements

The financial support from the Norwegian companies Aker BioMarine Antarctic AS, Oslo, Norway, Mills DA and Denomega Nutritional Oils AS and the Swedish company Skånemejerier, is highly appreciated. Fish pâté was carefully prepared and made available from Mills DA. Fruit juice was produced by Skånemejerier, and made available from Mills DA. Fish oil added to the products was delivered by Denomega Nutritional Oils. The authors also want to thank Ingunn Hagen Westgaard and Minna Nurminiemi, Link Medical Research AS, for their contribution to the interpretation and statistical analyses of the data, Professor Bjarne Østerud, Faculty of Health Sciences, University of Tromsø, Tromsø, Norway, for his contribution to the interpretation and analyses of plasma inflammatory markers, and Professor Jan I. Pedersen, Department of Nutrition, University of Oslo, Oslo, Norway, for valuable discussions and reading the manuscript. We also want to thank the volunteers who participated in the study. Conflict of interest: some of the authors are employed by the companies that delivered products to the trial. A. L. and E. F. are employees at Mills DA, Lena Nyberg at Skånemejerier, Hogne Vik and N. H. at Aker BioMarine Antarctic AS and E. O. at Denomega Nutritional Oils AS. B. K. worked for Mills DA when the project started. B. K. contributed to the design of the experiment, analysis and interpretation of the data and writing of the manuscript. A. L. contributed to the design of the experiment, product development, analysis and interpretation of the data and revising of the manuscript. K.-E. E. contributed to the design of the experiment, interpretation of the data and writing of the manuscript. E. F. contributed to the collection of the data, analysis and interpretation of the data and revising of the manuscript. T. H. contributed to the planning of the study design, statistical analyses of the data and revising of the manuscript. H. V. contributed to the planning of the study design, discussion and analysis of the study results, interpretation of the data, and writing of the manuscript. N. H. contributed to the initial planning of the study design and statistical analytical plan, interpretation of the data and revision of the manuscript. T.-A. H. contributed to the initial planning of the project, interpretation of some of the results and writing of the manuscript. S. B. contributed to the analysis and interpretation of the data and revising of the manuscript. E. O. contributed to the interpretation of the data and revising of the manuscript. I. S. contributed to consultation, discussion of the results and writing of the manuscript. L. N. contributed to the design of the experiment, interpretation of the data and revising of the manuscript. E. E. contributed to the conduction of the trial, collection of the data and writing of the manuscript. S. M. U. contributed to the conduction of the trial, collection of the data, analysis and interpretation of the data and writing of the manuscript.

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Figure 0

Table 1 Fatty acid composition of the study products (percentage of fatty acids)

Figure 1

Table 2 Baseline characteristics and plasma lipids(Mean values and standard deviations)

Figure 2

Table 3 Fatty acid levels in plasma (μmol/l)(Mean values and standard deviations)

Figure 3

Table 4 Serum lipids (mmol/l)(Mean values and standard deviations)

Figure 4

Table 5 Serum high sensitive C-reactive protein (hsCRP) and plasma inflammatory markers(Mean values and standard deviations)

Figure 5

Table 6 Markers of oxidative stress(Mean values and standard deviations)