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Enriched cereal bars are more effective in increasing plasma quercetin compared with quercetin from powder-filled hard capsules

Published online by Cambridge University Press:  20 July 2011

Sarah Egert*
Affiliation:
Department of Nutrition and Food Science, Nutritional Physiology, University of Bonn, Endenicher Allee 11-13, 53115Bonn, Germany Department of Human Nutrition, Institute of Human Nutrition and Food Science, Christian-Albrechts-University Kiel, Kiel, Germany
Siegfried Wolffram
Affiliation:
Institute of Animal Nutrition and Physiology, Christian-Albrechts-University Kiel, Kiel, Germany
Beate Schulze
Affiliation:
Department of Food Technology, Institute of Human Nutrition and Food Science, Christian-Albrechts-University Kiel, Kiel, Germany
Peter Langguth
Affiliation:
Department of Biopharmaceutics and Pharmaceutical Technology, Institute of Pharmacy, Johannes Gutenberg-University, Mainz, Germany
Eva Maria Hubbermann
Affiliation:
Department of Food Technology, Institute of Human Nutrition and Food Science, Christian-Albrechts-University Kiel, Kiel, Germany
Karin Schwarz
Affiliation:
Department of Food Technology, Institute of Human Nutrition and Food Science, Christian-Albrechts-University Kiel, Kiel, Germany
Berit Adolphi
Affiliation:
Schwartauer-Werke GmbH & Co. KGaA, Bad Schwartau, Germany
Anja Bosy-Westphal
Affiliation:
Department of Human Nutrition, Institute of Human Nutrition and Food Science, Christian-Albrechts-University Kiel, Kiel, Germany
Gerald Rimbach
Affiliation:
Department of Food Science, Institute of Human Nutrition and Food Science, Christian-Albrechts-University Kiel, Kiel, Germany
Manfred James Müller
Affiliation:
Department of Human Nutrition, Institute of Human Nutrition and Food Science, Christian-Albrechts-University Kiel, Kiel, Germany
*
*Corresponding author: S. Egert, fax +49 228 733217, email s.egert@uni-bonn.de
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Abstract

The flavonol quercetin, is one of the major flavonoids found in edible plants. The bioavailability of quercetin in humans may be influenced by the food matrix in which it is consumed as well as by its chemical and physical form. The objective of the present study was to investigate the biokinetics of quercetin from quercetin-enriched cereal bars and quercetin powder-filled hard capsules. In a randomised, single-blinded, diet-controlled cross-over study, six healthy women aged 22–28 years took a single oral dose of approximately 130 mg quercetin equivalents from either quercetin-enriched cereal bars (containing 93·3 % quercetin aglycone plus 6·7 % quercetin-4′-glucoside) or quercetin powder-filled hard capsules (100 % quercetin aglycone). Blood samples were drawn before and after quercetin administration over a 24 h period. The concentrations of quercetin and its monomethylated derivatives, isorhamnetin (3′-O-methyl quercetin) and tamarixetin (4′-O-methyl quercetin), were measured by HPLC with fluorescence detection after plasma enzymatic treatment. The systemic availability as determined by comparing the plasma concentration–time curves of quercetin was found to be five times and the cmax values six times higher after ingestion of 130 mg quercetin by quercetin-enriched cereal bars than after ingestion by quercetin capsules. In contrast, tmax did not differ significantly between the two treatments. The cmax values for isorhamnetin and tamarixetin were four and nine times higher after ingestion of quercetin by quercetin-enriched cereal bars than after ingestion by quercetin capsules. In conclusion, quercetin from quercetin-enriched cereal bars is significantly more bioavailable than from quercetin powder-filled hard capsules.

Type
Full Papers
Copyright
Copyright © The Authors 2011

Quercetin (3,3′,4′,5,7-pentahydroxyflavone) is one of the major flavonoids, ubiquitously distributed in edible plants(Reference Erdman, Balentine and Arab1). Epidemiological studies, together with data from animal models and some clinical trials, may suggest a role of flavonoids in general and of quercetin in particular in the prevention of CVD and other age-related chronic diseases(Reference Graf, Milbury and Blumberg2). In plasma, quercetin is found in the form of glucuronidated, sulphated and methylated derivatives(Reference Manach, Williamson and Morand3). Rich sources of dietary quercetin are onions, unpeeled apples, berries, citrus fruits, tea (Camellia sinensis) and red wine(Reference Erdman, Balentine and Arab1). Daily dietary intake of the flavonol quercetin varies considerably. In Western populations, crude estimates of mean dietary intake appear to be 10–100 mg/d(Reference Erdman, Balentine and Arab1, Reference Scalbert and Williamson4). In some countries, quercetin is available as a dietary supplement with daily doses of 200–1200 mg quercetin (manufacturers' recommendations). In addition, quercetin may be used as a nutraceutical for functional foods within a concentration range of 0·008–0·5 % or 10–125 mg/serving(Reference Harwood, Danielewska-Nikiel and Borzelleca5). Rather high concentrations of quercetin in foods can be obtained through the addition of pure quercetin, but probably also by the enrichment of foods with sources naturally rich in quercetin.

A prerequisite for the physiological effects of quercetin is its bioavailability. A considerable number of studies have dealt with determining the bioavailability of quercetin in human subjects(Reference Manach, Williamson and Morand3). It has been reported that isolated quercetin glucosides are absorbed better than quercetin administered in non-glucosidic forms, with no difference between the 3′-O-glucoside and 4′-O-glucoside(Reference Olthof, Hollman and Vree6). Furthermore, Hollman et al. (Reference Hollman, de Vries and van Leeuwen7) showed in healthy ileostomy volunteers that quercetin absorption was approximately two times higher when it was ingested as quercetin glucosides originating from fried onions compared with quercetin aglycone administered as a pure substance (quercetin dihydrate) in capsules. In contrast, Wiczkowski et al. (Reference Wiczkowski, Romaszko and Bucinski8) found that when provided along with natural sources (e.g. shallot preparations), quercetin aglycone was significantly more bioavailable than its glucosides in human subjects.

Onion skins are rich sources of quercetin aglycone(Reference Wiczkowski, Romaszko and Bucinski8) and may be suitable for the enrichment of several foods with quercetin. However, at present it is not known to what extent quercetin from foods enriched with onion skins or with extracts from onion skins is absorbed and whether food components or the matrix affects its bioavailability.

The present pilot study was designed to investigate in healthy normal-weight volunteers the systemic availability of quercetin from cereal bars enriched with quercetin derived from onion skin extract and in comparison from pure quercetin powder-filled hard capsules, consumed in combination with quercetin-free cereal bars. A dosage of approximately 130 mg quercetin was chosen, since it has been shown to lower resting systolic blood pressure, pulse pressure and plasma concentrations of oxidised LDL in our previous placebo-controlled cross-over study in overweight patients with a high CVD risk phenotype(Reference Egert, Bosy-Westphal and Seiberl9, Reference Egert, Boesch-Saadatmandi and Wolffram10). With both treatments, cereal bars and capsules, quercetin was administered as quercetin aglycone. In addition, the food matrix with which quercetin was ingested was the same; only the vehicle that contained the quercetin aglycone differed (cereal bar v. capsule).

Subjects and methods

Subjects

A total of six non-smoking German women aged 22–28 years participated in the present study. They were in good health as determined by a basic examination (body weight and height, blood pressure/pulse, medical anamneses and blood analyses; baseline characteristics are presented in Table 1). BMI ranged between 20 and 23 kg/m2. Exclusion criteria were overweight, metabolic and endocrine diseases, malabsorption syndromes, smoking, pregnancy/lactation, alcohol abuse, use of dietary supplements or any form of medication (with the exception of oral contraceptives, which were taken by all women). All subjects were asked to maintain their regular lifestyles and usual extent of physical activities throughout the study. The study was conducted according to the guidelines laid down in the Declaration of Helsinki, and all procedures involving human subjects were approved by the ethics committee of the Medical Faculty of the Christian-Albrechts-University of Kiel, Germany. Written informed consent was obtained from all subjects.

Table 1 Baseline characteristics of the participants

(Mean values with their standard errors, n 6)

Study design

Run-in phase

The participants refrained from quercetin-rich food for 1 week. For this purpose, a list of food items rich in quercetin (e.g. unpeeled apples, grape products, fruit juice, citrus fruits, berries, onions, broccoli, French beans, kale, tea and red wine) was given to each participant, and they were instructed to avoid such products. Compliance with these dietary restrictions was controlled by a self-completed standardised 3 d dietary record. No deviation from the low-quercetin diet occurred as shown by the records. Accordingly, the concentrations of quercetin were very low (0·08 (sem 0·01) μmol/l) in fasting plasma samples taken at baseline (see later).

Treatment period

The study was conducted in a single-blinded (blind participants), diet-controlled cross-over design. The six women were randomly assigned to treatment group A or B (n 3 and 3, respectively). Group A ingested two quercetin-enriched cereal bars (approximately 130 mg quercetin equivalents) plus six placebo capsules with a glass of water (200 ml); group B ingested two quercetin-free cereal bars (‘placebo cereals bars’) plus six quercetin capsules (approximately 130 mg quercetin equivalents) with 200 ml water during the first period of the treatment. After a break of 2 weeks (including a 1-week run-in period), group A ingested two placebo cereals bars plus six quercetin capsules during the second treatment and group B consumed two quercetin-enriched cereal bars plus six placebo capsules. The products were given in the morning after a 12 h overnight fast.

A standardised breakfast (white bread, butter and cheese and 200 ml water) was offered 120 min after the quercetin bolus. Lunch (pasta, cheese sauce, ice cream and 200 ml water) was served 240 min after quercetin administration, and dinner (white bread, butter, cheese, yogurt and water) was served at 600 min after quercetin administration. All foods were weighed to the nearest gram, contained only minor amounts of flavonoids and were provided at the study site. The participants were only allowed to drink water. Food and water intake was documented in a dietary record.

Blood samples were collected before (baseline) quercetin administration and 30, 60, 90, 120, 180, 240, 300, 360, 420, 480 and 1440 min after the dose. Blood was obtained by an indwelling cannula for samples up to 8 h and thereafter by venipuncture.

Study products

The study products used are not commercially available and were specifically made for the present biokinetic study. The quercetin and placebo capsules were prepared in a Good Manufacturing Practice (GMP)-certificated facility (Department of Biopharmaceutics and Pharmaceutical Technology, Johannes Gutenberg-University Mainz, Germany). The hard gelatine capsules were filled with 25 mg quercetin dihydrate powder (Voigt Global Distribution, Inc., Lawrence, KS, USA), mannitol and the flow-regulating excipient silicium dioxide. The quercetin content of the quercetin capsules was constant for a shelf-life of 3 years. The placebo capsules contained only mannitol and silicium dioxide.

The cereal bars were produced by Schwartauer Werke (Bad Schwartau, Germany). The main ingredients of the formulations were milk chocolate, glucose–fructose syrup, popped cereals (meal), almonds and cereal flakes. Enrichment with quercetin was achieved by mixing the onion skin extract (Rudolf Wild GmbH & Company KG, Heidelberg-Eppelheim, Germany) with almonds, cereal flakes and popped cereals before adding the viscous sugar binder. Finally, the cereal bars were partly coated with milk chocolate.

The quercetin content of the cereal bars was constant for a stated shelf-life of 12 months. Placebo cereal bars were prepared and packaged in an identical form to the enriched cereal bars to allow the blind protocol. The nutritional content of two cereal bars (2 × 25 g) was 940 kJ energy, 3·8 g protein, 29·4 g carbohydrate, 15·6 g sugar, 9 g fat, 4 g SFA, 2·2 g dietary fibre and 0·1 g Na. Quercetin-enriched cereal bars and placebo cereal bars were comparable with respect to appearance, texture, taste, acceptability and palatability.

The particle size X50 of quercetin dihydrate (capsules) was 11·9 μm. The X50 of the onion skin extract (cereal bars) averaged 22·5 μm. For the determination of particle size, a laser diffraction sensor (Helos; Sympatec GmbH, Clausthal-Zellerfeld, Germany) equipped with a cuvette was used. For the measurement of the particle size, an aliquot of the powder was dispersed in an inert oil (MCT (medium-chain TAG) oil; Gustav Hees Oleochemische Erzeugnisse GmbH, Stuttgart, Germany) until an optical density of 5 % was obtained. Analyses were performed in triplicate.

HPLC analyses of quercetin in cereal bars and capsules

The quercetin content of the capsules and cereal bars was determined by HPLC-diode-array detection analysis. For the determination of the content of the cereal bars, approximately 1 g of the homogenised sample was weighed into an extraction tube and 10 ml of a mixture of 80 % acetone and 20 % aqueous 0·1 % citric acid solution were added. Extraction was performed using ultrasonication. The samples were centrifuged (8750 g, 3 min, 20°C) and the supernatant was collected. The extraction was repeated three times using 5 ml of the extraction solvent for each extraction step. The supernatants were combined and filled to a total volume of 25 ml. For the capsules, the content of one capsule was dissolved in 100 ml of a mixture of 80 % acetone and 20 % aqueous 0·1 % citric acid solution. Before HPLC analysis, the samples were filtered through a paper filter. Analyses were carried out in duplicate.

Immediately after extraction, the extracts were analysed by HPLC-diode-array detection on an Agilent HP 1100 instrument (Agilent Technologies, Waldbronn, Germany) equipped with a Nucleodur Sphinx RP-C18 column (125 × 4 mm; 5 μm, Machery & Nagel, Düren, Germany) using 0·5 % aqueous formic acid (solvent A) and 100 % acetonitrile (solvent B) at a flow rate of 1 ml/min with gradient elution: 0–15 min, 10 % B; 15–20 min, 10–28·5 % B; 20–25 min, 28·5–34 % B; 25–30 min, 34–44 % B; 30–34 min, 44–80 % B and 34–38 min, 80–10 % B. Analytes were detected at 365 nm and quantified using quercetin aglycone for calibration.

In addition, the declared quercetin content of the capsules of 22·03 mg quercetin aglycone (anhydrous) was verified by UV spectroscopy using a sample size of twenty quercetin capsules. The content of each capsule was dissolved in 35 ml acetone. The solution was transferred to a 100 ml volumetric flask and filled to volume with demineralised water, and 50 μl of this solution was added to an acetone–water mixture (35:65) and absorbance was measured at 374 nm.

Dietary analysis

Dietary records were analysed using the computer-based nutrient calculation program EBISpro (University of Hohenheim, Stuttgart, Germany), based on the German Nutrient Database Bundeslebensmittelschlüssel (Max Rubner-Institute, Karlsruhe, Germany).

Nutritional status

Body height was measured to the nearest 0·5 cm with a stadiometer during the basic examination. Body composition (fat mass and fat-free mass) and body weight were determined on each treatment day after an overnight fast by air displacement plethysmography using the BOD POD Body Composition System (Life Measurements Instruments, Concord, CA, USA)(Reference Bosy-Westphal, Danielzik and Becker11).

Blood sampling, processing and analysis

For the determination of plasma concentrations of quercetin and its metabolites, blood was drawn into tubes containing lithium heparin (Sarstedt, Nümbrecht, Germany). After each sampling, blood was immediately centrifuged (2000 g, 15 min, 4°C) and the plasma was stored at − 75°C until analysis. All samples from one participant were measured within one analytical run. The analyses were conducted without the knowledge of the treatment groups.

On each treatment, additional fasting blood was taken to determine serum total cholesterol, LDL-cholesterol, HDL-cholesterol and TAG concentrations as well as plasma glucose concentrations, liver and kidney function markers in serum and haematological markers in blood.

Fasting blood concentrations of glucose, lipids as well as liver and kidney function markers were measured on a VITROS 950 Chemistry System autoanalyser (Ortho-Clinical Diagnostics, Neckargemünd, Germany) with the manufacturer's assay kits, quality controls and reagents. Haematological parameters (leucocyte count, erythrocyte count, platelet count, Hb concentration, haematocrit, mean corpuscular volume, mean corpuscular Hb and mean corpuscular Hb concentration) were determined by a CELL-DYN 3700 autoanalyser (Abbott Diagnostics Europe, Wiesbaden, Germany). The CV for all automated measurements were below 5 %.

Plasma quercetin and its metabolites

Analyses of plasma concentrations of quercetin and of the monomethylated derivatives isorhamnetin (3′-O-methyl quercetin) and tamarixetin (4′-O-methyl quercetin) were performed by HPLC with fluorescence detection as described previously(Reference Bieger, Cermak and Blank12). All samples were treated enzymatically with β-glucuronidase/sulfatase type H-2 (crude enzyme extract from Helix pomatia; Sigma-Aldrich AG, Taufkirchen, Germany) before the extraction of the flavonols. Authentic flavonols (Carl Roth GmbH, Karlsruhe, Germany) were used as external standards. The limit of detection was 5–7 nmol/l. Inter-analysis and inter-day variances were within 5 %.

Biokinetic calculations

Plasma flavonol concentrations obtained at different time points (T30–T1440) were corrected for individual baseline flavonol concentrations (T0). Maximum plasma concentrations (c max) and times to achieve maximum plasma concentrations (t max) were obtained directly by the visual inspection of each participant's plasma concentration time profile. The area under the plasma concentration–time curve (AUC) was determined according to the linear trapezoidal rule.

Statistical analysis

Statistical analyses were performed using the SPSS statistical software package (version 17; SPSS, Inc., Chicago, IL, USA). All data were log-transformed before statistical analyses. The differences between the mean values of c max, t max and AUC were analysed with the use of the paired Student's t test. Changes between the baseline (0 min) and the following time points among the two treatment groups were tested for significance by repeated-measures ANOVA. Differences were considered significant at P < 0·05. Unless otherwise indicated, the results are reported as mean values with their standard errors.

Results

Control variables

No adverse effects of the quercetin intakes were reported. The dietary records did not show significant differences between the two treatment groups in mean daily intakes of energy (9·1 MJ/d), protein (14·8 % of energy intake), carbohydrates (46·6 % of energy intake), fat (37·5 % of energy intake), SFA and unsaturated fatty acid, cholesterol, antioxidants (vitamin E, 1·4 mg/MJ; vitamin C, 15·6 mg/MJ) or dietary fibre before the treatment (data not shown).

Fasting serum lipids, glucose, biomarkers of liver and kidney function and haematological parameters were all within normal ranges, and no significant differences were observed between the treatment groups (data not shown).

Quercetin content of the study products

Based on individual component analysis, quercetin-enriched cereal bars contained 67 mg quercetin equivalents/25 g (containing 93·3 % quercetin aglycone plus 6·7 % quercetin-4′-glucoside). Thus, the participants ingested a total dose of 134 mg quercetin equivalents (two cereal bars). The quercetin capsules contained 22 mg quercetin aglycone per capsule leading to a total intake of 132 mg quercetin aglycone (six capsules).

Plasma quercetin

The group mean plasma quercetin concentration–time curve for the six women after consuming a single dose of approximately 130 mg quercetin from quercetin-enriched cereal bars and quercetin capsules, respectively, is shown in Fig. 1. In all participants, plasma quercetin increased 30 min following oral administration. This is consistent with in vitro digestion experiments, in which capsules and cereal bars were completely dispersed within the first digestion media simulating a fasting stomach fluid (data not shown).

Fig. 1 Plasma appearance and disappearance curves of quercetin after the ingestion of quercetin from quercetin-enriched cereal bars (■) and quercetin powder-filled hard capsules (● circle; n 6). Values are means, with their standard errors represented by vertical bars. Plasma concentrations differ significantly over time between the two treatment groups (P < 0·001 for time effect and P < 0·001 for time × treatment interaction in repeated-measures ANOVA). The last two data points are connected by a dashed line, because elimination processes during this time cannot be reliably determined.

The plasma quercetin concentration was consistently higher after the consumption of the quercetin-enriched cereal bars compared with quercetin intake from capsules. There was a high inter-individual variation in plasma concentration time profiles among the participants (Fig. 1). The participants who were the highest and the lowest quercetin absorbers after ingestion of the quercetin-enriched cereal bars were also the highest and the lowest absorbers after the intake of the quercetin capsules (data not shown).

Table 2 shows a summary of the results of the plasma kinetic analyses. Significant differences in the biokinetic parameters between the two treatments existed with respect to AUC and c max. The systemic availability as determined by comparing the plasma concentration–time curves of quercetin was found to be five times and c max six times higher after ingestion of 130 mg quercetin by quercetin-enriched cereal bars than after ingestion of quercetin powder-filled capsules. In contrast, t max did not differ significantly between the two treatments. Inter-individual variability of c max values for plasma quercetin was 24·6 % (cereal bars) and 25·0 % (capsules).

Table 2 Biokinetic variables of plasma quercetin, isorhamnetin and tamarixetin concentrations in women after a single oral dose of quercetin from quercetin-enriched cereal bars and quercetin capsules

(Mean values with their standard errors, n 6)

AUC, area under the plasma concentration–time curve; c max, the maximum plasma concentration; t max, the time to reach the maximum.

* Paired t test was used to assess differences between the variables.

Plasma isorhamnetin and tamarixetin

Following supplementation with quercetin, low amounts of isorhamnetin and tamarixetin were also apparent (Figs. 2 and 3). The plasma concentrations of isorhamnetin and tamarixetin were consistently higher after the consumption of the quercetin-enriched cereal bars compared with quercetin intake from capsules. There also was a high inter-individual variation in plasma concentration time profiles among the participants (Figs. 2 and 3). In all participants, tamarixetin was not detected in fasting plasma samples at baseline. The c max values for isorhamnetin and tamarixetin were four and nine times higher after the ingestion of quercetin by quercetin-enriched cereal bars than after the ingestion of quercetin capsules (Table 2). In contrast, t max values did not differ significantly between the two treatments (Table 2).

Fig. 2 Plasma appearance and disappearance curve for isorhamnetin after ingestion of quercetin from quercetin-enriched cereal bars (■) and quercetin powder-filled hard capsules (●; n 6). Values are means, with their standard errors represented by vertical bars. Plasma concentrations differ significantly over time between the two treatment groups (P < 0·001 for time effect and P < 0·001 for time × treatment interaction in repeated-measures ANOVA). The last two data points are connected by a dashed line, because elimination processes during this time cannot be reliably determined.

Fig. 3 Plasma appearance and disappearance curves for tamarixetin after ingestion of quercetin from quercetin-enriched cereal bars (■) and quercetin powder-filled hard capsules (●; n 6). Values are means, with their standard errors represented by vertical bars. Plasma concentrations differ significantly over time between the two treatment groups (P < 0·001 for time effect and P < 0·001 for time × treatment interaction in repeated-measures ANOVA). The last two data points are connected by a dashed line, because elimination processes during this time cannot be reliably determined.

We did not calculate the AUC for isorhamnetin and tamarixetin because of the low and irregular plasma appearance and disappearance curves that made a reliable determination of the parameter impossible. Based on the c max values, the monomethylated derivatives of quercetin (isorhamnetin and tamarixetin) accounted for about 14 % (cereal bars) and 16 % (capsules) of total plasma flavonols ( = sum of quercetin (μmol/l)+isorhamnetin (μmol/l)+tamarixetin (μmol/l)).

Discussion

The aim of the present pilot study was to investigate the systemic availability of quercetin from cereal bars enriched with quercetin derived from onion skin extract and from powder-filled hard capsules, both applying equivalent amounts of quercetin (approximately 130 mg). We used this moderate supranutritional but non-pharmacological dose of quercetin, since our data should provide a rational basis for the development of functional foods. The quercetin dose represented ten- to fifteen-fold of the estimated daily quercetin intake in Germany of about 10 mg(Reference Linseisen, Radtke and Wolfram13, Reference Böhm, Boeing and Hempel14). Our data indicate that onion-derived quercetin from quercetin-enriched cereal bars is more effective at increasing plasma quercetin compared with quercetin from powder-filled hard capsules in a short-term protocol with a single-oral dose administration. This conclusion is based on the AUC values, which were significantly higher with quercetin from cereal bars than with quercetin from capsules.

The plasma profiles of quercetin after the ingestion of 130 mg quercetin from capsules were similar to our previous human study that investigated the kinetics of plasma quercetin from three different quercetin dosages (50, 100 and 150 mg quercetin dihydrate)(Reference Egert, Wolffram and Bosy-Westphal15). In accordance with previous human studies, we observed a relatively high inter-individual variance in plasma concentration–time curves of quercetin, isorhamnetin and tamarixetin following supplementation with quercetin(Reference Egert, Wolffram and Bosy-Westphal15Reference Moon, Wang and Dicenzo18), although our non-smoking female study population was very homogenous with respect to age, baseline plasma quercetin concentrations, body weight, BMI, fat mass and fat-free mass as well as lifestyle and physical activity. This variability in plasma kinetic profiles may be attributed to inter-individual differences in digestive transit time, preferential site of absorption and enteric bacterial metabolism of quercetin as reported in the literature for quercetin and other polyphenols(Reference Manach, Williamson and Morand3, Reference Williamson and Manach19, Reference Manach, Scalbert and Morand20) as well as to the intrinsic solubilisation capacity of each individual.

The c max values (Table 2) indicated that the gastrointestinal absorption rate of quercetin from quercetin-enriched cereal bars was higher than from quercetin powder-filled hard capsules, which were ingested in combination with quercetin-free cereal bars. One factor that could explain this finding might be the food matrix. There are a limited number of studies concerning the effect of food components on the absorption of quercetin. Piskula & Terao(Reference Piskula and Terao21) found that the solubility of quercetin in vehicles (propylene glycol, water and 25 % propylene glycol in water (v/v)) for administration to rats greatly affected the efficiency of quercetin absorption. Sri et al. (Reference Sri, Kondaiah and Ratna22) demonstrated that the bioavailability of quercetin can be enhanced by a factor of 3 when inclusion complexes are formed with hydroxyl propyl-β-cyclodextrin. Azuma et al. (Reference Azuma, Ippoushi and Ito23) indicated that a combination of lipids (phosphatidylcholine and soyabean oil) and emulsifiers (sucrose fatty ester) can elevate the absorption of quercetin aglycone in rat plasma. In pigs, Lesser et al. (Reference Lesser, Cermak and Wolffram24) showed that the oral bioavailability of quercetin aglycone from a test meal was enhanced by approximately 60 % by the addition of 15 % (w:w) fat to a low-fat standard pig diet. It was speculated that the enhancement of quercetin bioavailability may have been the result of improved solubility of the lipophilic quercetin aglycone in the intestinal tract and/or additional absorption of quercetin via the lymphatic system in the presence of fat. In humans, however, a typical Western-type diet is likely to contain sufficient dietary fat to facilitate the absorption of quercetin(Reference Lesser, Cermak and Wolffram25). Thus, the solubility and distribution of quercetin in bulk foods may be key factors for the bioavailability, because quercetin aglycone is not freely soluble in water.

The fact that quercetin capsules were administered together with quercetin-free cereal bars indicates that not merely do the components of the cereal bar affect the absorption of quercetin, but that the manufacturing process of the quercetin-containing cereal bar might be a key factor in explaining the present findings. Intimate mixing of quercetin with the components (solid macroparticles) of the cereal bar resulted in a homogenous distribution of quercetin. The addition of a viscous binding matrix (glucose–fructose syrup and soft sugar) converted the whole mixture after cooling into a solid dispersion. Solid dispersions provide a large surface for compounds with low solubility and are utilised for pharmaceuticals to enhance bioavailability. In fact, the effective surface area is one of the important factors governing the dissolution rate of poorly soluble compounds. Solid dispersions are, in addition to micronisation and nanosizing technologies, a measure of enhancing the effective surface area available for dissolution(Reference Krishnaiah26).

On the other hand, the hard capsules were filled with a powder, rather than a solid dispersion, containing 25 mg quercetin dihydrate, and also did not contain flavonoid-solubilising excipients, which might have helped in the dissolution of the flavonoid from the dosage form. More advanced technologies, e.g. self-emulsifying systems in soft capsules and solid solutions/solid dispersions in glyceride-based matrices, might be developed to overcome the problem of poor bioavailability of quercetin powder from hard capsules.

After oral intake of quercetin from quercetin-enriched cereal bars and quercetin capsules, isorhamnetin and tamarixetin were also detected in human plasma. This finding is in accordance with our previous human kinetic study(Reference Egert, Wolffram and Bosy-Westphal15) and has also been found in pigs(Reference Ader, Wessmann and Wolffram27, Reference Cermak, Landgraf and Wolffram28). However, in contrast to mice and rats, in which nearly one-half of the absorbed amount of quercetin is methylated to isorhamnetin(Reference Boesch-Saadatmandi, Egert and Schrader29Reference Boesch-Saadatmandi, Loboda and Wagner32), the proportion of the methylated derivatives in human and pig plasma is rather low (approximately 15–20 % of total plasma flavonols). The finding that we detected the methylated quercetin metabolites in plasma samples shortly after the oral ingestion of quercetin indicates that these metabolites are derived from intestinal and/or hepatic metabolism by phase I enzymes, e.g. catechol-O-methyltransferase(Reference Zhu, Ezell and Liehr33), rather than being generated by microbial metabolisation.

To the best of our knowledge, the present study is the first to report that systemic availability of quercetin from quercetin-enriched cereal bars is significantly higher than that from quercetin capsules. The strengths of the present study are the randomised, blinded, diet-controlled cross-over design, the homogenous study population and the administration of equivalent amounts of quercetin (approximately 130 mg). However, the present study has some limitations. The quercetin-enriched cereal bars contained low amounts of quercetin-4′-glucoside (6·7 %), whereas the quercetin capsules were free of any quercetin glucosides. The mechanisms of gastrointestinal absorption of the hydrophobic quercetin aglycone and of the glycosylated, more hydropholilic quercetin glucosides, differ(Reference Manach, Scalbert and Morand20, Reference Kottra and Daniel34). Thus, the slightly different chemical composition of the quercetin profiles between cereal bar and capsule may have influenced the plasma appearance of quercetin. However, it seems unlikely that the low ‘impurity’ with quercetin-4′-glucoside explains the big differences in the plasma concentration time profiles between the two application forms. More importantly, the physical form of the quercetin administered was not the same for the two treatments as the quercetin was isolated in two different ways. Quercetin dihydrate used for the hard capsule was isolated by crystallisation. In the cereal bars, quercetin was added in the form of an extract, i.e. an isolation process was used that includes an evaporation or sublimation process of the extraction solvent, which may lead to an amorphous structure. In turn, different solubilisation characteristics for quercetin may result(Reference Krishnaiah26). In fact, an additional study showed that the systemic availability of approximately 100 mg quercetin from hard capsules containing the onion skin extract was approximately two-fold higher than from quercetin dihydrate hard capsules (B Schulze, S Egert, S Wolffram, K Schwartz and H Stöckmann, unpublished results).

In conclusion, quercetin aglycone from quercetin-enriched cereal bars was more bioavailable than from quercetin hard capsules containing the flavonoid powder and solid fillers as excipients in human subjects. If the intake of quercetin and related flavonols can indeed be proven to reduce the risk of CVD, then the production of foods with a more highly bioavailable form of quercetin might become a realistic proposition. Modification of intestinal absorption by food factors may be a promising technique to control the physiological function and effectiveness of quercetin. However, the safety of a regular (long-term) intake of quercetin as an ingredient of functional foods also needs to be assessed.

Acknowledgements

We are indebted to Schwartauer-Werke GmbH & Company KGaA (Dr Sebastian Portius) for the production of the cereal bars; to Rudolf Wild GmbH & Company KG (Matthias Saß) for the supply of the onion skin extract and to A.C.T. FOODS GmbH, Kiel, Germany (Dr Heiko Stöckmann) for supporting the bioavailability testing of the onion skin extract. We thank Petra Schulz and Ute Hartung for valuable technical assistance. S. E., S. W., B. S., P. L., E. M. H., K. S., A. B.-W., G. R. and M. J. M. disclose that there are no conflicts of interest. B. A. is employed at Schwartauer-Werke GmbH & Company KGaA. The present study was financially supported by the German Federal Ministry of Education and Research (BMBF 0313856A) within the project ‘Functional Foods for Vascular Health – from Nutraceuticals to Personalised Diets’ and Schwartauer-Werke GmbH & Company KGaA. S. E., G. R. and M. J. M. designed the study; S. E. and M. J. M. conducted the study; P. L. produced the capsules; B. A. produced the cereal bars; A. B.-W. helped in collecting the clinical data; S. E., S. W., B. S., P. L., E. M. H. and K. S. analysed the data; S. E. performed the statistical analysis and wrote the first draft of the manuscript; S. W., B. S., P. L., K. S., G. R. and M. J. M. strongly contributed to the interpretation of the results. S. E. and M. J. M. had primary responsibility for the final content. All authors read and approved the final manuscript.

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Figure 0

Table 1 Baseline characteristics of the participants(Mean values with their standard errors, n 6)

Figure 1

Fig. 1 Plasma appearance and disappearance curves of quercetin after the ingestion of quercetin from quercetin-enriched cereal bars (■) and quercetin powder-filled hard capsules (● circle; n 6). Values are means, with their standard errors represented by vertical bars. Plasma concentrations differ significantly over time between the two treatment groups (P < 0·001 for time effect and P < 0·001 for time × treatment interaction in repeated-measures ANOVA). The last two data points are connected by a dashed line, because elimination processes during this time cannot be reliably determined.

Figure 2

Table 2 Biokinetic variables of plasma quercetin, isorhamnetin and tamarixetin concentrations in women after a single oral dose of quercetin from quercetin-enriched cereal bars and quercetin capsules(Mean values with their standard errors, n 6)

Figure 3

Fig. 2 Plasma appearance and disappearance curve for isorhamnetin after ingestion of quercetin from quercetin-enriched cereal bars (■) and quercetin powder-filled hard capsules (●; n 6). Values are means, with their standard errors represented by vertical bars. Plasma concentrations differ significantly over time between the two treatment groups (P < 0·001 for time effect and P < 0·001 for time × treatment interaction in repeated-measures ANOVA). The last two data points are connected by a dashed line, because elimination processes during this time cannot be reliably determined.

Figure 4

Fig. 3 Plasma appearance and disappearance curves for tamarixetin after ingestion of quercetin from quercetin-enriched cereal bars (■) and quercetin powder-filled hard capsules (●; n 6). Values are means, with their standard errors represented by vertical bars. Plasma concentrations differ significantly over time between the two treatment groups (P < 0·001 for time effect and P < 0·001 for time × treatment interaction in repeated-measures ANOVA). The last two data points are connected by a dashed line, because elimination processes during this time cannot be reliably determined.