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Effects of dietary strawberry powder on blood lipids and inflammatory markers in obese human subjects

Published online by Cambridge University Press:  09 November 2011

Susan J. Zunino*
Affiliation:
United States Department of Agriculture, Agricultural Research Service, Western Human Nutrition Research Center, 430 West Health Sciences Drive, Davis, CA95616, USA
Mardi A. Parelman
Affiliation:
Department of Nutrition, University of California, Davis, One Shields Avenue, Davis, CA95616, USA
Tammy L. Freytag
Affiliation:
United States Department of Agriculture, Agricultural Research Service, Western Human Nutrition Research Center, 430 West Health Sciences Drive, Davis, CA95616, USA
Charles B. Stephensen
Affiliation:
United States Department of Agriculture, Agricultural Research Service, Western Human Nutrition Research Center, 430 West Health Sciences Drive, Davis, CA95616, USA
Darshan S. Kelley
Affiliation:
United States Department of Agriculture, Agricultural Research Service, Western Human Nutrition Research Center, 430 West Health Sciences Drive, Davis, CA95616, USA
Bruce E. Mackey
Affiliation:
United States Department of Agriculture, Agricultural Research Service, Pacific West Area, 800 Buchanan Street, Albany, CA94710, USA
Leslie R. Woodhouse
Affiliation:
United States Department of Agriculture, Agricultural Research Service, Western Human Nutrition Research Center, 430 West Health Sciences Drive, Davis, CA95616, USA
Ellen L. Bonnel
Affiliation:
Department of Nutrition, University of California, Davis, One Shields Avenue, Davis, CA95616, USA
*
*Corresponding author: Dr S. J. Zunino, fax +1 530 752 5271, email [email protected]
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Abstract

Obesity is a strong risk factor for the development of CVD, hypertension and type 2 diabetes. The overall goal of the present pilot study was to feed strawberries, in the form of freeze-dried powder, to obese subjects to determine whether dietary strawberries beneficially altered lipid profiles and reduced blood markers of inflammation compared with a control intervention. A total of twenty healthy subjects (thirteen females and seven males) aged between 20 and 50 years with a BMI between 30 and 40 kg/m2 completed the present 7-week double-blind, randomised, cross-over trial. Each subject received a prepared diet 7 d/week for 7 weeks consisting of approximately 35 % of energy from fat, 20 % protein, 45 % carbohydrate and 14 g fibre. Blood was collected on days 1 and 8 for baseline information. After the first week, subjects were randomly assigned to the strawberry powder (equivalent to four servings of frozen strawberries) or control (strawberry-flavoured) intervention for 3 weeks. For the remaining 3 weeks, subjects crossed over to the opposite intervention. Blood was collected again at the end of weeks 3, 4, 6 and 7. A comprehensive chemistry panel, lipid profile analyses and measurement of inflammatory mediators were performed for each blood draw. A 3-week dietary intervention with strawberry powder reduced plasma concentrations of cholesterol and small HDL-cholesterol particles, and increased LDL particle size in obese subjects (P < 0·05). Dietary strawberry powder reduced risk factors for CVD, stroke and diabetes in obese volunteers, suggesting a potential role for strawberries as a dietary means to decrease obesity-related disease.

Type
Full Papers
Copyright
Copyright © The Authors 2011

Obesity constitutes a serious public health problem in the USA as well as in other parts of the world(Reference Flegal, Carroll and Ogden1, Reference Nguyen and El-Serag2). Obesity rates have steadily risen over the past 20 years, and >30 % of US adults are obese according to a recent analysis of the 2007–8 National Health and Nutrition Examination Survey data(Reference Flegal, Carroll and Ogden1). Health care expenses associated with obesity have reached nearly 147 billion dollars(Reference Finkelstein, Trogdon and Cohen3). Obesity is a strong risk factor for the development of a number of chronic diseases which include hypertension, CVD and stroke, and the metabolic syndrome leading to insulin resistance and type 2 diabetes mellitus(Reference Samartin and Chandra4). Hypercholesterolaemia and dyslipidaemia are prominent in obese individuals. The development of type 2 diabetes in obese individuals further increases the risk of CVD due to metabolic disturbances resulting from insulin resistance and increased levels of inflammatory molecules. Atherosclerotic plaque formation can be initiated by an injury to the endothelial cell lining in the arterial wall by hypertension and subendothelial accumulation of oxidised, or otherwise modified, LDL(Reference Libby5). As a consequence of this damage, immune cells such as monocytes and T-lymphocytes enter the subendothelium and macrophages engulf the modified LDL creating foam cells, which eventually build up to form the plaques. The inflammation mediated by activated immune cells leads to the continued migration of macrophages and T-lymphocytes into the plaques, remodelling of the arterial wall and eventual blockage of the blood vessel.

Adipose tissue is a source of the inflammatory cytokines IL-6, TNF-α and IL-1β which stimulate the production of acute-phase proteins, such as C-reactive protein (CRP), fibrinogen and serum amyloid A(Reference Hotamisligil, Arner and Caro6Reference Fain11). Increased levels of serum CRP and serum amyloid A have been linked to an increased expression of endothelial adhesion molecules and chemoattractants that promote recruitment of immune cells into the arterial wall(Reference O'Brien and Chait8, Reference Pickup12). Soluble intercellular adhesion molecule-1 (ICAM-1) and soluble vascular adhesion molecule-1 (VCAM-1) both increase in the blood of obese humans, and are associated with an increased risk of CVD(Reference Straczkowski, Lewczuk and Dzienis-Straczkowski13, Reference Shai, Pischon and Hu14). IL-8, one of the chemoattractant molecules involved in atherosclerosis, can be produced by adipocytes, and circulating concentrations of IL-8 increase in obesity(Reference Kim, Park and Kawada15). Obesity leads to a prothrombotic state from the increased production of fibrinogen and other coagulation factors(Reference Faber, de Groot and Visseren9). Adipose tissue produces the hormone leptin, the obese (Ob) gene product, and elevated plasma levels of leptin are strongly associated with insulin-resistant states found in obesity, type 2 diabetes and hypertension(Reference Otero, Lago and Lago16). Increased leptin production in obese individuals can enhance the inflammatory processes associated with the development of atherosclerotic plaques and has been linked to the development of other chronic inflammatory diseases(Reference Otero, Lago and Lago16, Reference Lago, Gómez and Lago17).

Epidemiological and clinical studies have shown a positive association between dietary berries and reduced CVD risk (reviewed in Basu et al. (Reference Basu, Rhone and Lyons18)). Strawberries are a fibre- and Zn-rich food that contain abundant amounts of vitamin C and antioxidant polyphenols(Reference Hannum19, 20). Fibre is well known to reduce serum cholesterol and the risk of CVD(Reference Erkkilä and Lichtenstein21). Plasma Zn is inversely correlated with inflammation and atherosclerosis, and obese individuals generally present with decreased plasma Zn concentrations(Reference Bao, Prasad and Beck22Reference Yang, Choi and Chun24). Strawberries contain high levels of flavonoid antioxidants including catechins, anthocyanins, and the flavanols quercetin and kaempferol, all of which have anti-inflammatory abilities(Reference Hannum19). In the present pilot study, the overall goal was to determine whether dietary strawberries fed in the form of freeze-dried powder to obese subjects would reduce risk factors for CVD and other health problems known to be associated with morbidity and mortality of obese individuals. The specific hypothesis was that dietary strawberries would reduce cholesterol due to the increased intake of fibre, and beneficially alter lipid profiles and reduce blood markers of inflammation.

Methods

Subject recruitment

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 University of California Davis, Institutional Review Board. Written informed consent was obtained from all subjects. Healthy male and female subjects who participated in the present study were 20–50 years old with a BMI of 30–40 kg/m2. Subjects were recruited by advertisements, flyers and press releases, and screened by telephone questionnaire for health history, lifestyle, physical activity levels and dietary habits. For screening purposes, blood pressure, complete blood count and differential leucocyte counts were measured at the Western Human Nutrition Research Center (WHNRC). The pathology laboratory at the University of California Davis Medical Center (UCDMC) measured blood lipids and performed chemistry panels. All samples sent to the UCDMC pathology laboratory were coded and de-identified. Inclusion criteria for the present study were blood pressure, blood cell counts and blood chemistry profiles within the normal range, and commitment to the dietary intervention and scheduled testing. Exclusion criteria were vegetarianism, current use of tobacco products, drinking more than one alcoholic beverage per d (29·6 ml distilled liquor, 88·7 ml wine and 354·9 ml beer), use of cholesterol-lowering medications, steroids for asthma or other conditions, thyroid-regulating drugs or weight-loss products. Subjects with mildly or moderately elevated total cholesterol ( < 6·5 mmol/l) or TAG ( < 3·4 mmol/l) were not excluded. Subjects taking oral contraceptives were not excluded.

Study design and dietary intervention

The study was a 7-week double-blind, randomised, cross-over trial. Each subject received a prepared diet of three meals per d, 7 d/week for the duration of the study. Menu rotation was every 4 d. Energy intake was prescribed per individual based on the Mifflin–St Jeor equation(Reference Mifflin, St Jeor and Hill25) corrected for an appropriate activity factor. The background diet consisted of approximately 35 % energy from fat (animal and plant), 20 % protein, 45 % carbohydrate and 14 g fibre, which typifies the average American diet (National Health and Nutrition Examination Survey III)(26, 27) and was low in fruits and vegetables (less than four servings per d). The subjects came to the WHNRC for breakfast and dinner Monday to Friday (except for holidays), and received a packaged lunch for those days. For weekends and holidays, all meals were packaged and given to the subjects to consume. The subjects were asked to return all uneaten foods. Intervention with strawberries, in the form of strawberry powder, occurred at breakfast and dinner and was supervised, except for weekends and holidays. The California Strawberry Commission (Watsonville, CA, USA) provided the strawberry powder that was produced from individually quick frozen kosher, conventional (non-organic) whole strawberries. The strawberries were supplied by Anacapa Foods (Watsonville, CA, USA) and Frozsun Foods (Watsonville, CA, USA). The powder was prepared and packaged by Van Drunen Farms (Momence, IL, USA) by a commercial food freeze-drying process with a moisture content of approximately 5 %. The strawberry powder was maintained at − 20°C during the study. The mixture of strawberries used to generate the powder contained the University of California public cultivars Camarosa (37 %), Ventana (13 %) and Diamante (13 %), and two proprietary varieties (37 %) in production in 2004. In the present study, one serving of frozen strawberries (80 g) was used to calculate the amount of powder needed per serving. The subjects consumed the equivalent of four servings of strawberries per d. The strawberry intervention consisted of two servings of strawberry powder mixed as a milkshake, in yogurt, cream cheese, or water-based, sweetened beverage. The control intervention was the same drinks or food products with strawberry flavouring and red food colour (McCormick & Company, Hunt Valley, MD, USA). The flavourings were imitation strawberry extract (McCormick) and Kool-Aid strawberry artificial flavour (Kraft Foods, Rye Brook, NY, USA). Additional energy from the strawberries was matched in the control drink by adding an equivalent amount of glucose, fructose and sucrose. In the first week of the study, subjects received prepared meals without intervention. Blood was collected on day 1 and at the end of the first week to obtain baseline information. After the first week, subjects were randomised into one of two groups. Group 1 received the strawberry intervention and group 2 received the control intervention for 3 weeks. For the remaining 3 weeks of the study, subjects crossed over to the opposite intervention. All subjects fasted 12 h before each blood draw. Blood was collected again at the end of weeks 3, 4, 6 and 7 during the study. Measurements for each blood draw included a complete blood count with the differential leucocyte count and a comprehensive chemistry panel. Body weights were measured daily and dietary energy adjusted when necessary to maintain the same body weight throughout the study. Blood pressure, heart rate and body temperature were measured at the time of screening and at each blood draw during the study.

Chemistry and lipid panels

For serum preparation, blood was collected in Vacutainer tubes (Becton Dickinson, Franklin Lakes, NJ, USA), allowed to clot for 30 min at room temperature, and centrifuged at 4°C, 10 min, 1300 g. Serum samples were sent by courier to the UCDMC pathology laboratory the day of the blood draw. Alanine aminotransferase was added to the panel by the pathology laboratory midway through the study and analysed for ten subjects.

Plasma zinc measurements

Blood was collected into syringes containing Zn-free lithium heparin (S-Monovette for trace metal analysis; Sarstedt, Numbrecht, Germany), centrifuged at 1300 g, 4°C, 10 min, and stored at − 80°C before analysis. Plasma Zn concentrations were determined by inductively coupled plasma atomic emission spectrometry (ICP-AES) using a Vista AX CCD simultaneous ICP-AES analyser with an SPS5 autosampler (Varian, Inc., Walnut Creek, CA, USA). Zn standards and plasma samples were prepared in 1 m-HNO3 (Fisher Scientific, Pittsburg, PA, USA), centrifuged at 2200 g, 4°C, 15 min, and the supernatants recovered for ICP-AES analysis. Quality-control samples included a serum reference with known Zn value (Seronorm Trace Elements Serum LI; Accurate Chemical and Scientific Corporation, Westbury, NY, USA), and an internal quality-control plasma (Utak Laboratories, Inc., Valencia, CA, USA). Bovine liver standard, a certified reference material (no. SRM 1577b; National Institute of Standards and Technology, Boulder, CO, USA), was run as an ICP-AES Zn reference control. All blanks, standards and samples were run in duplicate.

Lipid particle analysis

Lipid size and particle analyses were performed on plasma samples using NMR at Liposcience, Inc. (Raleigh, NC, USA)(Reference Jeyarajah, Cromwell and Otvos28). Plasma was prepared using EDTA-Vacutainer tubes (Becton Dickinson) centrifuged at 4°C, 10 min, 1300 g. All plasma samples sent to Liposcience were frozen at − 80°C and shipped on dry ice.

Acute-phase proteins and inflammatory markers

Serum and plasma were prepared as described above and frozen at − 80°C until analysis of inflammatory markers. CRP was measured in serum using a high sensitivity test kit and Immulite instrumentation (Siemens Healthcare Diagnostics, Inc., Deerfield, IL, USA). Complement 3c was measured in serum on the Cobas Integra 400 Plus chemical analyser (Roche Diagnostics, Indianapolis, IN, USA) using kit reagents from Roche Diagnostics. Enzyme-linked immunosorbant assays were used to measure serum amyloid A (US Biological, Swampscott, MA, USA) and plasma fibrinogen (AssayPro, St Charles, MO, USA) following the manufacturers’ protocols. Plasma levels of IL-1β, IL-6, IL-8, TNF-α, leptin, soluble ICAM-1 and soluble VCAM-1 were measured using Milliplex detection kits (Millipore Corporation, St Charles, MO, USA) run on a Bioplex multiplex instrument (BioRad, Hercules, CA, USA). Samples were run in duplicate.

Antioxidant status

Serum was prepared as described above and measured for antioxidant status using the total antioxidant status (TAS) and oxygen radical absorbance capacity (ORAC) assays. TAS was measured on the Cobas Integra 400 Plus chemical analyser using reagents from Randox Laboratories (San Diego, CA, USA) and following the manufacturer's recommendations. ORAC values were measured using the method described by Prior et al. (Reference Prior, Hoang and Gu29). The radical generator 2,2′-azobis(2-methylproprionamidine)dihydrochloride (AAPH) and 6-hydroxy-2,5,7,8-tetramethylchroman-2-carboxylic acid (Trolox) were purchased from Sigma (St Louis, MO, USA). Fluorescein sodium salt was obtained from Acros Organics (Morris Plains, NJ, USA). The loss of the fluorescein signal due to oxidation was monitored for 2 h at 37°C on a SpectraMAX GeminiXS spectrofluorometer running SoftMAX PRO version 4.0 software (Molecular Devices, Sunnyvale, CA, USA). Trolox equivalents were calculated by comparing the areas under the curves (fluorescence intensity v. time) of Trolox standards to serum samples.

Butylated hydroxytoluene was added as a preservative to plasma used for 8-isoprostane analyses. Concentrations of free 8-isoprostane were measured by enzyme-linked immunoassay kits (Cayman Chemical Company, Ann Arbor, MI, USA) following the manufacturer's recommendations. Assays for TAS and 8-isoprostane were run in duplicate. ORAC assays were run in triplicate.

Statistical analyses

The Statistical Analysis Systems statistical software package version 9.2 (SAS Institute, Cary, NC, USA) was used for statistical analyses using the Proc Mixed procedure to fit the cross-over model with the baseline values (blood draws 1 and 2) as the covariates. The means of the two baselines were used as covariates to account for a greater amount of variability among the subjects, and thus, reduced error and increased precision in the tests. The Means procedure was used for means and standard deviations. Data subsets were transformed using Box–Cox power transformations, if needed to conform to a normal distribution. When a carry-over effect was detected, an analysis was performed that included only the first 3-week intervention period of the study. We expected cholesterol to be reduced by dietary strawberry powder due to the addition of fibre to the diet from the powder(20). Therefore, a one-tailed test was used only for the analysis of total cholesterol. All data are presented as means and standard deviations to indicate variability of individual values, with significance at P < 0·05.

Results

Recruitment and study participation

The recruitment, screening and participation of subjects are shown in Fig. 1. The age, weight and BMI for female and male subjects who completed the screening process and the study are presented in Table 1. Of the thirty-one subjects who participated, eleven dropped out for the following reasons: dietary (dislike of provided meals, five subjects); medical (unrelated to the study, two subjects); personal (undisclosed, two subjects); schedule conflicts (two subjects). Energy was adjusted in the diets weekly if needed to maintain body weight throughout the study period. Compliance was assured at least 5 d/week of the study, since the subjects were fed the interventions at breakfast and dinner under supervision at the Center on weekdays.

Fig. 1 Recruitment, screening and participation of the study subjects. M, male; F, female.

Table 1 Age, weight and BMI of subjects completing screening and the study

(Mean values and standard deviations)

Vitals, blood chemistry and lipid panels

No differences were observed between the intervention groups for blood pressure, heart rates or body temperature. Blood chemistry and lipid parameters were measured for each blood draw by the pathology laboratory at the UCDMC (Table 2). Diet effects were observed for Na, CO2 and total cholesterol. Dietary strawberry powder reduced Na and CO2 concentrations in the blood compared with the control group (P < 0·05). There was a carry-over (order) effect for serum cholesterol into the second intervention period of the cross-over design, and intervention period 1 only was analysed for this parameter (ten subjects). Serum cholesterol was reduced in the subjects receiving the strawberry powder compared with the control group (P = 0·0438). There was no effect of blood draw (week 2 v. week 3) or a diet × blood draw interaction for any parameter shown in Table 2.

Table 2 Chemistry and lipid panels*

(Unadjusted mean values and standard deviations (n 20 except for alanine aminotransferase (ALT) and total cholesterol))

wk, Week; AST, aspartate aminotransferase.

a,b Mean values with unlike superscript letters in overall diet effect between the two intervention groups were significantly different (P < 0·05).

* Baseline data (blood draws 1 and 2) were used as covariates.

ALT was added to the chemistry panel by the UC Davis Medical Center during the second half of the study and analysis was performed for ten study subjects.

A carry-over (order) effect was observed for cholesterol and the data presented represent a one-tailed, period 1 analysis (n 10).

§ Wk 2 data represent 2 weeks of intervention (blood draws 3 and 5), and wk 3 data represent 3 weeks of intervention (blood draws 4 and 6) with the control diet (control) or the diet containing the strawberry powder (strawberry).

P value for the overall diet effect between the two intervention groups. No diet × blood draw interactions were found.

Lipid particle profiles by NMR analysis

Profiles of lipid particles were obtained for each blood draw (Table 3). There was evidence of a carry-over (order) effect for total HDL, small HDL particles, VLDL size, LDL size, HDL size, intermediate-density lipoprotein-cholesterol and small HDL-cholesterol, and intervention period 1 only was analysed for these parameters (ten subjects). All other parameters had an n 20. There was a diet effect for small HDL particle concentrations, LDL size and small HDL-cholesterol concentrations. Dietary strawberry powder reduced the concentrations of small HDL particles and small HDL-cholesterol, and increased the mean particle size of LDL (P < 0·05). There was no effect of blood draw (week 2 v. week 3) or a diet × blood draw interaction.

Table 3 Lipid particle concentrations and size*

(Unadjusted mean values and standard deviations (n 20 except as noted in footnote ))

wk, Week; IDL, intermediate-density lipoprotein.

a,b Mean values with unlike superscript letters in overall diet effect between the two intervention groups were significantly different (P < 0·05).

* Baseline data (blood draws 1 and 2) were used as covariates.

A carry-over (order) effect was observed for total HDL, small HDL, VLDL size, LDL size, HDL size, IDL-cholesterol and small HDL-cholesterol, and the data presented for these parameters are from intervention period 1 (n 10). For all other parameters, n 20.

Wk 2 data represent 2 weeks of intervention (blood draws 3 and 5), and wk 3 data represent 3 weeks of intervention (blood draws 4 and 6) with the control diet (control) or the diet containing the strawberry powder (strawberry).

§ P value for the overall diet effect between the two intervention groups. No diet × blood draw interactions were found.

Inflammatory markers and antioxidant status

Plasma or serum was analysed for inflammatory markers and antioxidant status (Table 4). The acute-phase protein fibrinogen was slightly increased in subjects consuming the strawberry powder compared with the control diet (P < 0·05), but the concentrations remained within the normal range. There were no differences observed for the other inflammatory markers. There were no differences in antioxidant status between the two dietary groups as measured by the ORAC, TAS or 8-isoprostane assay. There was no effect of blood draw or a diet × blood draw interaction for these measurements.

Table 4 Inflammatory markers and antioxidant status in serum and plasma*

(Unadjusted mean values and standard deviations (n 20 except as noted in footnote ))

wk, Week; sICAM-1, soluble intercellular adhesion molecule 1; sVCAM-1, soluble vascular adhesion molecule 1; CRP, C-reactive protein; SAA, serum amyloid A; ORAC, oxygen radical absorbance capacity; TE, Trolox equivalents; TAS, total antioxidant status.

a,b Mean values with unlike superscript letters in overall diet effect between the two intervention groups were significantly different (P < 0·05).

* Baseline data (blood draws 1 and 2) were used as covariates.

A carry-over (order) effect was observed for sICAM-1, sVCAM-1 and ORAC and the data presented represent a period 1 analysis (n 10). For all other parameters, n 20.

Wk 2 data represent 2 weeks of intervention (blood draws 3 and 5), and wk 3 data represent 3 weeks of intervention (blood draws 4 and 6) with the control diet (control) or the diet containing the strawberry powder (strawberry).

§ P value for the overall diet effect between the two intervention groups. No diet × blood draw interactions were found.

Discussion

The goal of the present pilot study was to determine the potential of dietary strawberries in the form of freeze-dried powder to improve markers of health in obese human subjects who are at high risk for developing serious diseases, such as CVD, stroke and diabetes. Hypercholesterolaemia is common in obese individuals. In the present study, we did not specifically recruit individuals with elevated cholesterol, and the mean total cholesterol concentrations for our participants was 4·66 (sd 0·89) mmol/l at the time of screening. However, consumption of the strawberry powder (equivalent to four servings of frozen strawberries per d) reduced plasma concentrations of total cholesterol by about 4 % compared with the control diet. This reduction was observed by 2 weeks of feeding and was maintained through week 3. The relatively small decrease in total cholesterol in response to strawberry powder in the present study may be because of the normal cholesterol concentrations before the supplementation, and the short duration of the intervention periods. In general, it should be noted that the subjects in the present study were relatively healthy obese individuals. In recent studies, Basu et al. (Reference Basu, Wilkinson and Penugonda30, Reference Basu, Fu and Wilkinson31) fed strawberry powder for 4 or 8 weeks to subjects who had both the metabolic syndrome and elevated plasma cholesterol. The powder was mixed as a beverage and equivalent to about four servings of strawberries per d. After 4 weeks of the strawberry powder intervention, these authors observed a 5 % decrease in total plasma cholesterol(Reference Basu, Wilkinson and Penugonda30). In a separate study, a 10 % reduction in total cholesterol was observed after an 8-week intervention with the same serving size of strawberry powder(Reference Basu, Fu and Wilkinson31). Fibre is well known to reduce cholesterol(Reference Erkkilä and Lichtenstein21). Reduction in total cholesterol may have been at least partly due to the increased intake of fibre in the diet from the addition of the strawberry powder. Strawberries have approximately 2 g fibre/100 g fresh edible portion(Reference Hannum19, 20). In the present study, each subject received about 8 g of extra fibre per d during the 3 weeks on the strawberry-enriched diet. Taken together, these data suggest that prolonged consumption of strawberries may continue to improve the cholesterol-lowering effect of this fruit over time.

Basu et al. (Reference Basu, Wilkinson and Penugonda30, Reference Basu, Fu and Wilkinson31) noted a 6 and 11 % reduction in the concentration of LDL-cholesterol after 4- and 8-week interventions, respectively. Jenkins et al. (Reference Jenkins, Nguyen and Kendall32) also reported a reduction in LDL-cholesterol and in the ratio of total:HDL-cholesterol after feeding 454 g strawberries per d for 1 month. In the present study, concentrations of LDL-cholesterol were not different between the dietary groups. However, our analyses of lipid particles by NMR revealed a reduction in the concentration of small HDL particles and small HDL-cholesterol in subjects consuming the strawberry powder. These lipid fractions have been linked to health status. Evaluation of HDL particle sizes in patients with coronary artery disease revealed a significantly higher concentration of small HDL particles in the coronary artery disease group than in control subjects(Reference Cheung, Brown and Wolf33). Also, higher concentrations of small HDL-cholesterol have been observed in Asian Indian men who have a greater incidence of CVD compared with Caucasian men(Reference Bhalodkar, Blum and Rana34), suggesting a link between CVD risk and the presence of small HDL. Patients with acute ischaemic stroke had greater concentrations of small HDL particles, as well as small LDL particles, than healthy controls(Reference Zeljkovic, Vekic and Spasojevic-Kalimanovska35). Furthermore, both LDL and HDL particle distribution and size have been linked to the metabolic syndrome and insulin resistance. As part of the Genetics of Coronary Artery Disease in Alaska Natives study, analyses of lipid distribution in Alaskan Eskimos with the metabolic syndrome showed an increase in the concentration of intermediate-density lipoprotein and small HDL particles compared with subjects without the metabolic syndrome(Reference Rivellese, Patti and Kaufman36). In 2005, Festa et al. (Reference Festa, Williams and Hanley37) reported the NMR-generated lipid profiles of prediabetic subjects as part of the Insulin Resistance Atherosclerosis Study. An increase in the concentration of small HDL was observed in subjects who had become diabetic at follow-up compared with non-diabetic patients at the time of follow-up.

Although the present study showed no change in LDL concentrations between the dietary groups, the strawberry intervention increased the mean particle size of plasma LDL. Decreased LDL size is positively associated with an increased risk of developing CVD, the metabolic syndrome and type 2 diabetes(Reference Festa, Williams and Hanley37Reference Rizzo, Pernice and Frasheri40). Festa et al. (Reference Festa, Williams and Hanley37) showed that a reduction of 0·3–0·5 nm in the diameter of LDL was positively correlated with the development of type 2 diabetes. Smaller HDL and larger VLDL particle sizes have also been associated with an increased risk of CVD(Reference Lyons, Jenkins and Zheng41, Reference Arsenault, Lemieux and Despres42). There was a potential trend towards an increase in HDL particle size in the present study, and this difference may have attained significance if a carry-over effect had not been observed. The present data indicate that a 3-week intervention with strawberry powder was able to reduce plasma concentrations of small HDL particles and cholesterol and increase LDL particle size in healthy obese subjects, and, thereby, reduce risk factors for obesity-related disease.

There were no differences in inflammatory markers, plasma Zn or antioxidant status of the serum from our volunteers between the two dietary groups. Basu et al. (Reference Basu, Fu and Wilkinson31) observed a decrease in circulating VCAM-1 in subjects with the metabolic syndrome receiving freeze-dried strawberry powder for 8 weeks. In an epidemiological study over a 10·9-year follow-up period involving the Women's Health Study, women who consumed two servings or greater of strawberries per week v. none had a 14 % lower likelihood of an elevated CRP equal to or above 3 mg/l(Reference Sesso, Gaziano and Jenkins43). A 16-week study with progressive doses of cranberry juice resulted in decreased plasma concentrations of ICAM-1-1 and VCAM-1(Reference Ruel, Pomerleau and Couture44). However, Erlund et al. (Reference Erlund, Koli and Alfthan45) observed no changes in soluble ICAM-1 levels in the blood after feeding a combination of berry preparations (including strawberries) for 8 weeks. Strawberries have recently been shown to decrease plasma levels of CRP and IL-6 in response to a high-fat meal, indicating that dietary strawberries have the potential for modulating immediate inflammatory responses induced by dietary fat(Reference Edirisinghe, Banaszewski and Cappozzo46). In the present study, 3 weeks of dietary intervention with strawberries may not have been long enough to observe differences in inflammatory markers between the two dietary groups. Antioxidant status was shown to increase in several clinical trials with consumption of strawberries or other berries, in either postprandial or longer-term protocols (reviewed in Basu et al. (Reference Basu, Rhone and Lyons18)). Recent studies using oxidised LDL as a marker have shown that dietary strawberries increased serum antioxidant capacity both postprandially(Reference Burton-Freeman, Linares and Hyson47) and after 3 and 4 weeks of strawberry intake(Reference Jenkins, Nguyen and Kendall32, Reference Henning, Seeram and Zhang48). Using three different tests for antioxidant potential or oxidation status, no difference in serum antioxidant status was observed in the present study. However, the subjects fasted for approximately 12 h before each blood draw, and antioxidant potential may not have been maintained at a steady-state level in our volunteers under these conditions. The strengths of the present study included the control of dietary intake by feeding all foods to the participants and maintaining body weight throughout the study. Therefore, the variables of dietary and weight change were reduced with this protocol. The use of freeze-dried strawberry powder rather than fresh strawberries further reduced seasonal variations in the fruit during the study. Analysis of drying methods has shown comparable levels of phenolics, vitamin C and antioxidant activity between fresh and freeze-dried strawberries(Reference Wojdyło, Figiel and Oszmiański49). Furthermore, the cross-over design allowed the subjects to be their own controls, and the dietary effects of the strawberry powder were observed within a 3-week period. Some parameters that were measured showed a carry-over or order effect, so that only the first intervention period was used to evaluate significant effects. The study design would have been enhanced with a washout period between the cross-over intervention periods as well as longer intervention periods. Increasing the number of participants may also have enhanced the study outcomes. However, the alterations in lipid subfractions that were observed may represent a beneficial reduction in risk factors for CVD, stroke and the metabolic syndrome/diabetes in our obese volunteers, suggesting a role for strawberries as a dietary means to decrease obesity-related disease. The present study provides data to support larger and more demographically diverse clinical trials with strawberries and other fruits to define the roles they may play in reducing morbidity and mortality associated with obesity.

Acknowledgements

This study was supported by the United States Department of Agriculture (USDA) Current Research Information System project no. 5306-51 530-013-00D and 5306-51 530-018-00D, and a grant from the California Strawberry Commission. S. J. Z. is a member of the scientific advisory committee for the California Strawberry Commission. The authors report no conflict of interest. The authors’ contributions were as follows: S. J. Z., C. B. S., D. S. K. and E. L. B. designed the research; T. L. F. and L. R. W. conducted the research; S. J. Z., M. A. P. and B. E. M. analysed the data; S. J. Z. wrote the manuscript with input from all authors and had primary responsibility for the final content. All authors read and approved the final manuscript. USDA is an equal opportunity provider and employer.

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Figure 0

Fig. 1 Recruitment, screening and participation of the study subjects. M, male; F, female.

Figure 1

Table 1 Age, weight and BMI of subjects completing screening and the study(Mean values and standard deviations)

Figure 2

Table 2 Chemistry and lipid panels*(Unadjusted mean values and standard deviations (n 20 except for alanine aminotransferase (ALT)† and total cholesterol‡))

Figure 3

Table 3 Lipid particle concentrations and size*(Unadjusted mean values and standard deviations (n 20 except as noted in footnote †))

Figure 4

Table 4 Inflammatory markers and antioxidant status in serum and plasma*(Unadjusted mean values and standard deviations (n 20 except as noted in footnote †))