Subjects and study design

The present study was part of a larger intervention study investigating the effects of FO-supplementation in combination with a high or low 18 : 2n-6 intake on tissue PUFA-incorporation⁽Reference Damsgaard, Frokiaer and Lauritzen²⁸⁾, CVD risk markers and cytokine production in healthy young men. The study ran from October 2005 to February 2006. Healthy male subjects aged 18–40 years were recruited by notes at universities throughout Copenhagen. Subjects were invited to participate in the study if they matched the following inclusion criteria: BMI 18·5–27 kg/m²; non-smokers or infrequent smokers ( ≤ 5 cigarettes a week); daily consumption of butter, margarine and/or oil, and home-made cooking ≥ 5 times per week. Volunteers were excluded if they suffered from chronic diseases or serious allergic symptoms, were taking medication or dietary supplements, exercised more than 7 h weekly or had donated blood within the last 2 months. Ethical permission for the study was obtained from the Ethical Committee of the Municipalities of Frederiksberg and Copenhagen (Journal No. KF 01 267804). The study was registered in the clinical trial database of the US National Institutes of Health (ClinicalTrials.gov, NCT00266292). Informed written consent was obtained from all subjects enrolled in the study.

The design of the study was as follows: a screening visit, a 2-week run-in period, a baseline visit, an 8-week intervention period, an endpoint visit and a washout visit 8 weeks post-intervention⁽Reference Damsgaard, Frokiaer and Lauritzen²⁸⁾. The sub-study described in the present paper ended after the subjects had completed the endpoint visit and therefore does not contain any washout data. The following sections describe only measurements relevant to this particular sub-study.

The study had a randomised-parallel 2 × 2-factorial design in which the subjects were randomly assigned to daily supplementation with capsules containing either FO or olive oil (OO, control) for 8 weeks. Subjects were also randomly assigned to household use of oil and fat spreads with either a high or a low 18 : 2n-6 content supplied by sunflower oil/Becel (S/B) and rapeseed oil/Kaergaarden (R/K), respectively. The randomisations were performed in two steps: first, notes were drawn from one envelope for the capsule intervention and second, within each capsule group notes were drawn for the oil and fat spread intervention. Thus, the subjects were randomly allocated in a double-blind fashion to one of four intervention groups: (1) OO-capsules and S/B, (2) OO-capsules and R/K, (3) FO-capsules and S/B or (4) FO-capsules and R/K.

Capsules (in a defined surplus), fat spreads and oils specified by the randomisation were supplied to the subjects on the day of their baseline visit. The subjects were instructed to consume ten capsules per day (equal to 5 ml/d) with FO (Bio-Marin) or OO (both kindly provided by Pharma Nord, Vejle, Denmark). Each FO-capsule contained 333 mg n-3 PUFA (NEFA, approximately 166 mg EPA and 119 mg DHA). The OO was given as TAG, but the capsules were matched for fat content. The S/B groups were supplied with sunflower oil (kindly provided by Aarhus United Denmark A/S, Aarhus, Denmark) and margarine (Becel 60, kindly provided by Unilever Denmark A/S Foods, Brøndby, Denmark) with a high content of 18 : 2n-6, whereas the R/K groups were supplied with rapeseed oil (also a gift from Aarhus United Denmark A/S) and a butter product containing two-thirds butter and one-third rapeseed oil (Kaergaarden Light, kindly provided by Arla Foods amba, Viby, Denmark) with a low content of 18 : 2n-6. Both the margarine and the butter products contained 60 g fat/100 g product. Prior to the intervention period, all subjects were provided with butter (Lurpak, also a gift from Arla Foods amba) and OO (Oleificio R.M. s.p.a., Lucca, Italy) for a 2-week run-in period. The purpose of this was to reset the fatty acid composition of the tissue marker. There were no restrictions concerning the amount of fat spreads or oil ingested, but it was intended that the intake of fat and energy remained constant during the study. The average energy intake and the dietary composition were determined by 4 d weighed dietary records: (1) prior to the run-in period and (2) at the end of the 8-week intervention period. The mean length of the intervention was 56 d (range 50–65 d).

Seventy-five subjects were invited to a screening visit at which height, weight, hip- and waist-circumference were measured and the subjects were instructed in how to perform the dietary records. Eight subjects dropped out during the run-in period due to the workload of attendance and one subject was rejected at the baseline visit due to intense discomfort during blood sampling. This left us with sixty-six men enrolled in the study, of which sixty-four completed the intervention period. The reasons for drop-out were discomfort swallowing the oil capsules (n 1) and the workload of attendance (n 1). Furthermore, six subjects were left out from this sub-study, four because no endpoint oxidative bursts were measured and two because the baseline neutrophil count failed (equipment error). Drop-outs and data collection failures were evenly distributed across the four intervention groups. Data are reported only for those subjects with a complete dataset (n 58). Furthermore, one analysis run stopped (for an unknown reason), which resulted in a loss of three subjects in all statistical tests of the area under the curve (AUC) and desensitisation (Des) oxidative burst variables (n 55). The baseline characteristics of the subjects in each of the intervention groups are shown in Table 1. Age, height, weight, BMI and waist/hip ratio did not differ between the groups.

Table 1 Baseline characteristics of the subjects in the four intervention groups (n 58)

R/K, rapeseed oil/Kaergaarden; S/B, sunflower oil/Becel.

† Between-group comparisons were performed using one-way ANOVA and Kruskal–Wallis tests with significance established at P < 0·05. No significant differences were observed for any of the variables.

‡ Percentiles: 25th to 75th.

Fasting blood samples were collected at the baseline and endpoint visits. The subjects were asked to follow standardised fasting conditions before each visit. These were: no food for 12 h or more (except from 0·5 litre water), lack of strenuous physical activity for 36 h, no smoking for 1 week and no medicine for 24 h. Moreover, the subjects were told to eat the same meal the evening before all visits and to re-schedule their visit if they were ill or had a cold. These criteria were checked at every visit.

Experimental procedures

On the days of examination, body weight and waist/hip ratio were determined. The subject filled out a questionnaire on dietary habits, illnesses, use of medication and smoking. Blood (80–110 ml) was drawn from fasting males after 10 min of rest and analysed for: oxidative burst, cell count, Hb concentration and the fatty acid composition of peripheral blood mononuclear cells (PBMC).

Compliance was assessed by counting returned capsules and measuring tissue fatty acid composition of the PBMC. The mean daily consumption of capsule oils was 4·5 (sd 0·5) ml/d (range 3·0–5·5 ml/d), equivalent to 89 % compliance. No difference in compliance was observed between the intervention groups. The fatty acid composition in the total lipid fraction from PBMC was determined as a biomarker of the resulting changes in tissue composition.

Measuring fatty acid composition of the tissue

PBMC were isolated from blood sampled with Na-heparin and fatty acid composition was determined by GLC as described elsewhere⁽Reference Damsgaard, Frokiaer and Lauritzen²⁸⁾. Fatty acids are given as area percentage (FA%), comparable to g/100 g.

Neutrophil counts and Hb concentration

Neutrophil count was determined by leucocyte size differentiation carried out on a Sysmex KX-21 automated haematology analyser (Sysmex Corporation, Kobe, Japan) on venous blood collected in EDTA tubes using the appropriate control. At the same time the Hb concentration was measured. Intra- and interassay CV for Hb were 0·7 % (n 12) and 0·6 % (n 25), respectively. Prior to the study intra-individual variation in neutrophil count was determined to 17·5 % measured on three independent days in five individuals.

Measurement of oxidative burst

Prior to the study all stock solutions were portioned and frozen at − 20°C. Zymosan A, a proteoglycan isolated from Saccharomyces cerevisiae (Sigma-Aldrich, St Louis, MO, USA), was suspended to 1 mg/ml in Hank's Balanced Salt Solution with CaCl₂+MgCl₂ (Invitrogen, Carlsbad, CA, USA) and portioned in aliquots of 300 μl, and luminol (5-amino-2,3-dihydro-1,4-phthalazinedione; Across Organics, NJ, USA) was dissolved to 5 mg/ml in dimethyl sulphoxide (Sigma-Aldrich) and portioned in aliquots of 100 μl.

Blood, sampled in Na-heparin tubes for assessment of oxidative burst, was stored at 37°C and oxidative burst was determined within 2 h after sampling by chemiluminescence: 90 μl whole blood diluted 1:9 in pre-warmed (37°C) Hank's Balanced Salt Solution was loaded on ninety-six-well LumiNunc™ polystyrene plates (Nunc, Roskilde, Denmark), which were preloaded with a 1:10 diluted stock solution of luminol (10 μl) with Hank's Balanced Salt Solution in a final concentration of 142 μm/well. The diluted blood samples were stimulated with 100 μl pre-warmed (37°C) zymosan at two different final concentrations (5 and 0·5 μg/ml). Chemiluminescence (relative light units/s) was measured in a thermostat-regulated (37°C) ninety-six-well Orion II Microplate luminometer (Berthold Detection Systems, Pforzheim, Germany). The microplate was read for 1 s/well with a 2 min delay, a cycle repeated for a total of seventy-five rounds. Unstimulated control samples (blanks) were analysed in duplicate and stimulated samples in sextuplicate.

Five variables were used to define the kinetics of the mean chemiluminescence response curve (Fig. 1): (1) time to half peak height (T½P), (2) peak height, (3) AUC, (4) slope between 40 and 60 % of peak height (α_40–60 %) and (5) Des. All variables, except for AUC were calculated with Microsoft Excel 2000 (Windows XP; Microsoft Corp., Redmond, WA, USA) based on linear mathematical principles. AUC was determined with GraphPad Prism version 4.00 (GraphPad Prism, San Diego, CA, USA) based on integral calculation. Prior to the study, the inter-day variation of the oxidative burst variables was determined: blanks 2·4 %, peak height 25·9 %, AUC 29·6 %, T½P 3·8 %, Des 48·5 % and α_40–60 % 35·4 % based on three independent days in five individuals. Data were analysed with the Statistical Package for the Social Sciences software version 13.0 (SPSS Inc., Chicago, IL, USA). Data are only shown for the 5 μg/ml zymosan-stimulated samples. The results of the 0·5 μg/ml zymosan-stimulated samples were similar, but the responses were smaller.

Fig. 1 Illustration of the luminol-enhanced chemiluminescence-detected oxidative burst response in whole blood as a function of time, based on a randomly selected participant. ●, Non-stimulated mean response curve; ○, mean zymosan (Saccharomyces cerevisiae)-induced (5 μg/ml) response curve. The response kinetics of the oxidative burst was expressed by five selected variables: peak height (peak); area under the curve (AUC, ); time to half peak (T½P); desensitisation (Des) and the slope between 40 and 60 % of peak height (α_40–60 %). RLU, relative light units.

Statistical analyses

Data were checked for Gaussian distribution with Shapiro–Wilks test and visual inspection of histograms. Gaussian-distributed data are presented as means with their standard errors, whereas non-Gaussian-distributed data are presented as medians with 25th–75th percentiles. Baseline comparison between the four intervention groups were performed by one-way ANOVA and Kruskal–Wallis tests. Analyses of covariance (ANCOVA) were used for endpoint comparisons. Non-Gaussian-distributed dependent variables (peak height, AUC, Des, α_40–60 %) were log(10)-transformed before testing.

Statistical analysis was performed on the following: (1) the effect of the interventions on the fatty acid composition of PBMC, (2) the effect of the intervention on neutrophil count and oxidative burst, and (3) the association between the effect on oxidative burst and that on tissue fatty acid content. The three statistical procedures were as follows:

1. (1) The ANCOVA for the endpoint comparisons of PBMC fatty acid content (EPA, 22 : 5n-3, DHA and total n-3 PUFA) included fat type and capsule type as fixed factors and were adjusted for baseline values. All models were checked for interaction between the capsule and the oil/fat spread interventions.

2. (2) All oxidative burst variables at endpoint were checked for bivariate Spearman's correlation with the following covariates: neutrophil count (endpoint), changes in (Δ, endpoint value −  baseline value) neutrophil count, smoking (yes/no) and Δ Hb concentration. Correlating parameters (neutrophil count and Δ neutrophil count) were tested as covariates in the ANCOVA endpoint comparison of the oxidative burst variables, which also included fat type and capsule type as fixed factors (including check for fat × capsule interaction) and adjustment for baseline values. Covariates were successively removed, but those affecting the outcome (P < 0·05) were kept in the model (Δ neutrophil count).

3. (3) The dose–response relationship analysis of the oxidative burst variables were performed using multiple linear regression analysis including the following covariates: endpoint PBMC DHA content, baseline values and the covariates included in the oxidative burst variable ANCOVA.

Wilcoxon test and paired-sample t test were used to check for within-group changes during the intervention of non-Gaussian-distributed and Gaussian-distributed data, respectively. Associations between the estimated FO-consumption (from the count of returned capsules (ml/d)) and Δ PBMC content of total n-3 PUFA, DHA, 22 : 5n-3 and EPA was analysed using Pearson correlation analysis. Significance was established at P < 0·05.