Recruitment of subjects

Healthy non-smoking adults aged 18–50 in the surroundings of Wageningen in the Netherlands were recruited for participation in the screening for the study by posters and advertisements in local newspapers. Written and verbal information was provided and informed consent forms were signed. The screening's examination included a health and lifestyle questionnaire, a FFQ⁽Reference Feunekes, van Staveren and de Vries²²⁾, weight measurement (precise to 0·1 kg) and height measurement (precise to 0·5 cm), and haematological analyses of blood, liver enzymes, creatinine, alkaline phosphatase and cholesterol. Exclusion criteria were as follows: haematological abnormalities, history of chronic diseases, including cancer, renal insufficiency, liver disease, diagnosed gastrointestinal disorders, surgery of gastrointestinal tract, use of (oral) drugs suspected of interfering with fat-soluble vitamin absorption, pregnancy, BMI < 18 or >25 kg/m², smoking, abnormal dietary pattern, excessive alcohol consumption (>40 g/d), and consumption of carotenoids/vitamin/mineral supplements 6 weeks before and during the study. Subjects with low serum β-carotene ( < 0·28 μmol/l) and/or low serum retinol ( < 1·07 μmol/l) concentrations were also excluded from participation. Twenty-eight volunteers participated in the screening, and twenty-four subjects were selected to form two groups, which were matched for sex, age, BMI and habitual energy intake. The subject characteristics at baseline are shown in Table 1. The study was conducted at the Division of Human Nutrition, Wageningen University, the Netherlands. The research protocol was approved by the Medical-ethical Committee on Research Involving Human Subjects, Region Arnhem-Nijmegen, the Netherlands.

Table 1 Characteristics of the subjects at baseline*

(Mean values and standard deviations)

* Groups 1 and 2 were matched for sex, age, BMI and habitual energy intake. There were no differences between groups (two-tailed t tests for independent samples).

Study design

The study was designed as a cross-over intervention with two controlled diets in twenty-four healthy subjects. Each subject followed two diets for 3 weeks each; one diet containing vegetables low in β-carotene with supplemental β-carotene in salad dressing oil (‘oil diet’) and the other diet containing vegetables high in β-carotene (‘mixed diet’). The subjects consumed capsules each day for 6 weeks during both diets. The capsules contained a mean of 55 μg/d [¹³C₁₀]β-carotene and 55 μg/d [¹³C₁₀]retinyl palmitate in oil (relative to their daily energy intake). On days 0, 1, 21, 22, 42 and 43 fasting blood samples (13 ml each) were obtained, and then kept in the dark at 4°C for 30 min before being centrifuged at 3000 rpm for 10 min at 4°C to separate cells from serum. Serum was stored at − 80°C until analysis. Fasting was defined as not consuming any food or energy-containing drinks for 12 h prior to the blood sampling. On days 19, 20 and 21 and also on days 40, 41 and 42, complete 72 h faeces were collected directly after defecation at home (according to instructions), stored on dry ice ( − 79°C) in plastic bags with labels, and then transported to the − 80°C freezer at the research centre. The concentrations of carotenoids and retinol in duplicate diets, serum and in faeces were measured by HPLC, and the isotopic enrichments of retinol with [¹³C₅]retinol and [¹³C₁₀]retinol and of β-carotene with [¹³C₁₀]β-carotene were measured using LC–MS.

Diets and compliance

Menus were designed for twelve levels of energy intake ranging from 7 to 18 MJ/d. The subjects were allocated to an energy intake level close to their habitual energy intake, which was estimated from a FFQ⁽Reference Feunekes, van Staveren and de Vries²²⁾. The ‘oil diet’ and the ‘mixed diet’ were designed according to the guidelines of ‘good nutrition’ from the Dutch Nutrition Board in The Hague, the Netherlands. Both diets were typical western diets with respect to the contribution of carbohydrates, proteins and fats to the energy intake (57, 13 and 30, respectively; Table 2). The menu was changed daily on a 3-week cycle; 90 % of energy was provided; all food was weighed out for each subject. The remaining 10 % of energy had to be chosen from a list of low-fat food items, which did not contain carotenoids or retinol, which had to be recorded in a diary. The diaries were inspected at least twice weekly. Body weight was recorded twice weekly and energy intake was adjusted, when necessary, to limit changes in weight to less than 2 kg. During weekdays, subjects consumed all their capsules and hot meal at noon at the research centre under supervision. Foods for their other meals and snacks (bread; margarine; meat and cheese; honey, jam, or sprinkles; fruit; milk and/or yoghurt; cookies) were packed for consumption at home, as was food for the weekends. The hot meal contained potatoes/pasta/rice, cooked vegetables, salad with salad dressing, a piece of meat and dessert. The salad dressing for the ‘oil diet’ was supplemented with synthetic β-carotene (all-trans β-carotene, 30 % suspension in vegetable oil; Hoffmann-La Roche, Switzerland). The margarine was prepared by special order (Unilever, the Netherlands) and was not supplemented with retinol or β-carotene as is normally the case with margarine in the Netherlands. The ratio of β-carotene provided by fruits to vegetables was 1:2·4 in the ‘oil diet’ and 1:8·2 in the ‘mixed diet’. The fruits were orange, apple, grapes, banana and melon. The cooked vegetables in the ‘oil diet’ were French beans, beetroots, snow peas, white cabbage, cauliflower, ratatouille, red cabbage and Chinese cabbage. The cooked vegetables in the ‘mixed diet’ were carrots in combination with French beans, green beans, snow peas, green peas, endive, leek, savoy cabbage and broccoli. Each vegetable originated from one batch and was analysed before the study to ensure the β-carotene content of each daily diet was similar. Each subject kept a diary for monitoring compliance to the diet, compliance to the intake of the capsules, compliance to fasting instruction, compliance to faeces collection, illnesses, medication used and the daily choice of low-fat food items. The composition of both diets was calculated using the Dutch Food Composition Table⁽²³⁾. In order to analyse the nutrient content, duplicate diets of the 11 MJ menu were collected every day and stored at − 20°C in non-transparent buckets. On a weekly basis, seven diets were pooled, mixed thoroughly with 2·5 ml 20 % butylhydroquinone/kg food, and stored at − 20°C until analysis. The individual energy and nutrient intakes during the study were calculated by using the food composition data of the selected food items and the analysed values of the duplicate diets and adjusted to the individual energy intake level.

Table 2 Composition of the two controlled diets during the 6-week crossover intervention study*

* Energy and nutrient intakes were calculated by using the calculated data of the freely selected food items (10 % of energy) and of the analysed values of the duplicate diets (90 % of 11 MJ) and adjusted to the individual energy intake level.

Chemical analysis of duplicate diets, vegetables and salad dressings

Duplicate samples of the meals were analysed for fat, protein, dietary fibre, moisture, ash, retinol and carotenoids at the Division of Human Nutrition. The fat concentration was measured gravimetrically after Soxhlet extraction with petroleum ether–diethyl ether (1:1, v/v)⁽²⁴⁾. The protein concentration was measured as total nitrogen by the Kjehldahl method, multiplied by 6·25⁽²⁴⁾. Dietary fibre was measured according to the Prosky procedure⁽²⁴⁾. The moisture level was determined after drying for 10 h in a vacuum oven at 80°C, and the ash content was determined using a dry ashing procedure in a muffle furnace for 10 h at 550°C⁽Reference Osborne and Voogt²⁵⁾. Available carbohydrates were calculated by difference.

For the analysis of the dietary retinol and carotenoids, food samples were homogenized and extracted with tetrahydrofuran. After evaporation of the solvent, the residue was saponified overnight at room temperature in 5 % ethanolic KOH containing 0·2 % pyrogallol. After addition of dichloromethane, KOH was extracted four times using water. The dichloromethane layer was filtered by using a water filter (597 HY ½; Schleicher & Schuell) and evaporated to dryness under nitrogen at 35°C. The residue was dissolved in methanol–tetrahydrofuran (1:1, v/v) and analysed by HPLC on a Vydac 201TP54 reversed-phase column (C₁₈; 5 μm; 300 Å; 4 × 250 mm) using gradient elution with a mixture of methanol, tetrahydrofuran, water and triethylamine, as described elsewhere⁽Reference Hulshof, van Roekel-Jansen and van de Bovenkamp²⁶⁾. The elution of retinol was monitored at 326 nm, and carotenoids were measured at 450 nm. The samples of the vegetable batches and duplicate salad dressings were analysed for concentrations of carotenoids by HPLC⁽Reference Hulshof, Chao and van de Bovenkamp²⁷⁾. All sample preparations were carried out under subdued yellow light to avoid degradation of the carotenoids.

Chemical analysis of retinol and carotenoids in serum and in faeces

Retinol and carotenoids in human serum were analysed using the HPLC method with absorbance detection described previously⁽Reference Khan, West and de Pee²⁸⁾. Briefly, to 500 μl serum, 500 μl sodium chloride (0·9 %, w/v in water) and 1·00 ml ethanol (containing retinyl acetate as an internal standard) were added, and then extracted twice with 2·0 ml portions of hexane. The hexane layers were pooled and evaporated to dryness under nitrogen at 35°C. The residue was dissolved in 250 μl methanol–tetrahydrofuran (3:1, v/v), and 25 μl were injected for each HPLC analysis. Separations were monitored at 326 nm (retinol) and 450 nm (carotenoids). Within- and between-run CV for the chemical analysis of retinol and carotenoids in serum were 1·6 and 1·9 % for retinol, 3·4 and 8·2 % for β-carotene, 4·6 and 7·0 % for α-carotene, and 3·6 and 11·4 % for β-cryptoxanthin.

Faeces samples of 72 h collection from each subject were pooled, homogenized and weighed. Sample preparation for the extraction of human faeces has been described by van Lieshout et al. ⁽Reference van Lieshout, West and van de Bovenkamp²⁹⁾. Briefly, an aliquot (2 g) was extracted in duplicate with 4 g Na₂SO₄, 0·5 g CaCO₃, 30 ml tetrahydrofuran containing 0·01 % butylated hydroxytoluene and 1 ml of an internal standard in tetrahydrofuran–methanol (3:1, v/v) containing a known amount of retinyl acetate (about 1 μg) in a 100 ml measuring cylinder, using a Polytron. The residue was triple extracted with 30 ml tetrahydrofuran. Retinol and carotenoids in the extracts of the faeces samples were analysed by HPLC using a reversed-phase C₃₀ column with internal and external standards and control samples as described elsewhere⁽Reference van Lieshout, West and van de Bovenkamp²⁹⁾. All sample preparations of both serum and faeces were carried out under subdued yellow light. The recovery of β-carotene was 89, 79 and 90 % measured three times in duplicate by spiking of β-carotene standard. The reproducibility (combined within- and between-run CV) was 7·1 % based on twelve analytical runs.

Capsule administration and measurement in serum and in faeces

The capsules contained 14·9, 20·1 or 25·7 μg [12,13,14,15,20,12′,13′,14′,15′,20′-¹³C₁₀]β-carotene and 14·1, 19·1 or 23·9 μg [8,9,10,11,12,13,14,15,19,20-¹³C₁₀]retinyl palmitate in oil (analysed values). The oily mixture for the capsules was prepared by dissolving the labelled β-carotene and retinyl palmitate in highly unsaturated sunflower oil (>82 % oleic acid and >9 % linoleic acid; Hozol; Contined BV, Bennekom, the Netherlands) and contained 63 μg/g [¹³C₁₀]β-carotene and 60 μg/g [¹³C₁₀]retinyl palmitate. all-rac-α-Tocopheryl acetate (Roche Vitamins, Deinze, the Netherlands) was added to the oil at levels of 91, 122 or 150 μg/capsule, respectively. The capsules used in the present study were made from bovine gelatin (Capsugel, Bornem, Belgium) and were filled with the oily mixture by electronic repetitive multipipetting with 240, 320 or 400 μl. These actions were carried out under subdued light. The ¹³C₁₀-labelled β-carotene and ¹³C₁₀-labelled retinyl palmitate were synthesized at ARC Laboratories (Apeldoorn, the Netherlands) as described previously⁽Reference Lugtenburg, Creemers and Verhoeven³⁰⁾ (isotopic incorporation >99 %, isomeric purity >93 % all-trans, chemical purity >98 %). These compounds were food grade according to criteria established by the European Pharmacopoeia and the Joint FAO/WHO Expert Committee on Food Additives. The individual amount of labelled β-carotene and labelled retinyl palmitate varied from 35 to 90 μg/d as it was related to the individual's estimated daily energy intake which varied from 7 to 18 MJ/d. For example, a subject who consumed 11 MJ/d received 55 (sd 0·5) μg [¹³C₁₀]β-carotene and 55 (sd 0·5) μg [¹³C₁₀]retinyl palmitate each day (one capsule of 15 (sd 0·2) μg and two capsules of 20 (sd 0·3) μg [¹³C₁₀]β-carotene and [¹³C₁₀]retinyl palmitate). Likewise, a subject who consumed 8 MJ/d received 40 (sd 0·4) μg/d, and a subject consuming 14 MJ/d received 70 (sd 0·7) μg/d each of labelled β-carotene and labelled retinyl palmitate. Concentrations of retinol and β-carotene in the capsules were analysed by HPLC with absorbance detection⁽Reference Khan, West and de Pee²⁸⁾. There is no known health risk associated with ingestion of stable isotope-labelled β-carotene or retinyl palmitate. The degree of isotopic enrichment in serum of retinol with [¹³C₅]retinol (derived from administered [¹³C₁₀]β-carotene) and with [¹³C₁₀]retinol and of β-carotene with [¹³C₁₀]β-carotene was measured by using LC–MS with atmospheric pressure chemical ionization (APCI LC-MS) as described previously⁽Reference van Breemen, Nikolic and Xu^31, Reference Wang, Xu and van Lieshout³²⁾. Signals for β-carotene were detected at mass-to-charge ratios (m/z) 537, for [¹³C₁₀]β-carotene at m/z 547, for retinol at m/z 269, for [¹³C₅]retinol at m/z 274 and for [¹³C₁₀]retinol at m/z 279. The sample preparation, accuracy and precision of the measurement of the degree of isotopic enrichment of β-carotene and of retinol in serum and in faeces have been described in Zhu et al. ⁽Reference Zhu, Wang and Pang³³⁾.

Calculations

Isotopic enrichment levels of β-carotene were calculated as the signal measured by LC–MS at m/z 546 divided by the total signal at m/z 536 and 546. Enrichment levels of retinol were calculated as the signal at m/z 274 (or 279) divided by the total signal at m/z 269, 274 and 279. The vitamin A equivalency (μg) of β-carotene in oil relative to that of retinol in oil was calculated for each subject as the inverse ratio of the dose-corrected ratio of [¹³C₅]retinol to [¹³C₁₀]retinol in serum (by weight) as follows⁽Reference van Lieshout, West and Wang³⁴⁾:

(1)

A necessary condition for using equation 1 is to standardize strictly the daily nutrient intake during the 3-week intervention study.

A bio-efficacy of 100 % would mean that 1 μmol dietary β-carotene (537 μg) is absorbed and converted totally to retinol, thus yielding 2 μmol retinol (572 μg). Thus, the bio-efficacy (%) of β-carotene was calculated from the vitamin A equivalency (equation 1), as follows⁽Reference van Lieshout, West and Muhilal^1, Reference van Lieshout, West and Wang³⁴⁾:

(2)

For each diet the apparent absorption (%) of total β-carotene (both labelled and unlabelled) was calculated for each subject by subtracting the amount of β-carotene in faeces (72 h) from the amount consumed (72 h) and dividing the difference by the amount consumed multiplied by 100 as shown in Table 5. This apparent absorption multiplied by the estimated bioconversion (2 μg β-carotene in the enterocyte is equivalent to 1 μg retinol in the body) resulted in an estimated bio-efficacy and from that the estimated vitamin A equivalencies for β-carotene in the ‘oil diet’ and for β-carotene in the ‘mixed diet’.

Statistical analysis

Data are shown as means and 95 % CI or standard deviation (in the case of descriptive measures). Data of serum concentrations and enrichments were averaged for days 0 and 1, for days 21 and 22, and for days 42 and 43 for each subject. Two-tailed t tests for independent samples were performed to evaluate differences in baseline characteristics (haematological blood values, alanine aminotransferase, creatinine, alkaline phosphatase, cholesterol) between the two groups. ANOVA was used to test period effects with diet and order as mean effects in the model. Because the order of the two diets did not significantly contribute to the model, serum retinol and serum β-carotene concentrations at baseline and after each diet were compared between the two groups with a paired t test. To test whether the percentages of apparent absorption were significantly different between both diets, two-tailed independent sample t tests were performed. All tests were two-sided, and P values < 0·05 were considered significant. The computer package SPSS version 12.0 (SPSS Inc., Chicago, IL, USA) and Microsoft Office Excel 2003 (Microsoft Corp., Redmond, WA, USA) was used for all statistical calculations and data handling.