Human vitamin E requirements assessed with the use of apples fortified with deuterium-labeled {alpha}-tocopheryl acetate

19th International Congress of Nutrition

HOME

HELP

FEEDBACK

SUBSCRIPTIONS

ORIGINAL RESEARCH COMMUNICATION

Human vitamin E requirements assessed with the use of apples fortified with deuterium-labeled ${alpha}$ -tocopheryl acetate¹^,2^,3

Richard S Bruno¹, Scott W Leonard¹, Su-il Park¹, Yanyun Zhao¹ and Maret G Traber¹

¹ From the Department of Food Science and Technology, Oregon State University, Corvallis, OR

² Supported in part by a grant to MGT (NIH DK59576) and by theNational Institute of Environmental Health Sciences (NIH P30ES00210).

³ Reprints not available. Address correspondence to MG Traber,571 Weniger Hall, Linus Pauling Institute, Oregon State University,Corvallis, OR 97331. E-mail: maret.traber{at}oregonstate.edu.

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
SUBJECTS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Background: Little is known about factors that modulate dietary ${alpha}$ -tocopherol bioavailability.

Objectives: The study aimed to assess the efficacy of vitaminE–fortified apples as a low-fat vitamin E delivery system,the influence of fat on vitamin E absorption, and human vitaminE requirements by using plasma ${alpha}$ -tocopherol kinetics at a dosageof ${alpha}$ -tocopherol found in food.

Design: Apples fortified with deuterium-labeled ${alpha}$ -tocopherylacetate were consumed by 5 participants at a breakfast containing0%, 6%, or 21% kcal from fat in 3 sequential trials. The trialswere separated by a 2-wk washout period. Blood samples wereobtained up to 72 h, and plasma was analyzed for labeled andunlabeled ${alpha}$ -tocopherol.

Results: Compared with observations in the 0% fat trial, themaximum observed plasma d₆- ${alpha}$ -tocopherol concentrations (C_max)and the areas under the curve increased 2- and 3-fold duringthe 6% and 21% fat trials, respectively. The mean (±SD)estimated percentage d₆- ${alpha}$ -tocopherol absorbed increased from10 ± 4% during the 0% fat trial to 20 ± 3% and33 ± 5% during the 6% and 21% fat trials, respectively.The mean time to C_max (9 ± 2 h), fractional disappearancerates (0.022 ± 0.003 pools/d), and half-lives (32 ±4 h) did not differ significantly between the trials. With theuse of fractional disappearance rates and baseline plasma ${alpha}$ -tocopherolconcentrations, the estimated daily plasma ${alpha}$ -tocopherol effluxwas 13–14 mg. The estimated rate of ${alpha}$ -tocopherol deliveryto tissues was 5 mg/d.

Conclusions: Given an estimated 33% absorption, the amount ofdietary vitamin E needed daily to replace irreversible lossesis $≤$ 15 mg. These estimates support the current human vitaminE requirements despite the claims that the median amount ofvitamin E that Americans consume is 7 mg/d.

Key Words: ${alpha}$ -Tocopherol • vitamin E requirements • bioavailability • deuterium • biokinetics • dietary fat

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
SUBJECTS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Because of the widespread problem of obesity (1, 2), Americansare being counseled to reduce their total energy and fat intakes.However, Maras et al (3) indicated that most persons obtaindietary vitamin E from high-energy, high-fat foods that arenot particularly ${alpha}$ -tocopherol–rich. When persons are instructedto decrease their fat intake as part of weight management, theyincur a ${approx}$ 50% reduction in vitamin E intake (4). Indeed, vitaminE is one of the most difficult nutrients to obtain; only 8%of men and 2% of women in the United States had vitamin E intakesfrom food (3) that met the 2000 Estimated Average Requirementof 12 mg ${alpha}$ -tocopherol/d (5). Low-fat foods fortified with vitaminE might be a solution that allows consumers to eat more ${alpha}$ -tocopherol–densefoods.

Fresh-cut fruit and vegetables can be fortified with micronutrientswith the use of vacuum impregnation without otherwise changingthe physiochemical food properties. This is a technique usedby the food industry to fortify the functional composition ofhigh-porosity foods. We have used vacuum impregnation to incorporatemicronutrients, such as ${alpha}$ -tocopherol (6) or zinc and calcium(7), into low-fat, low-energy foods.

Although vacuum impregnation of fresh apples with vitamin Eincorporates substantial amounts of ${alpha}$ -tocopherol, little is knownabout ${alpha}$ -tocopherol bioavailability from this low-fat matrix.In most foods, vitamin E is associated with fats and oils (8).Intestinal ${alpha}$ -tocopherol absorption is dependent on the same processesthat enable fat digestion, uptake into the enterocyte, and secretionin chylomicrons (9). Therefore, we hypothesized that ${alpha}$ -tocopherolbioavailability from vitamin E–fortified apples couldbe significantly enhanced by the simultaneous ingestion of dietaryfat. To test this hypothesis, deuterium-labeled vitamin E–fortifiedapples, which were designed so that a serving contained approximatelythe vitamin E daily value (30 IU) (5), were consumed with abreakfast that contained increasing amounts of fat followedby a controlled lunch in 3 sequential trials. Importantly, becausethe amount of vitamin E consumed was in the range for dietaryintakes, we also estimated human vitamin E requirements basedon ${alpha}$ -tocopherol turnover kinetics.

SUBJECTS AND METHODS

TOP
ABSTRACT
INTRODUCTION
SUBJECTS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials
HPLC-grade methanol was obtained from Fisher (Fair Lawn, NJ).Ascorbic acid, butylated hydroxy toluene, and potassium hydroxidewere obtained from Sigma-Aldrich (St Louis, MO). Vitamin E standards,including unlabeled (d₀) RRR- ${alpha}$ -tocopherol, labeled (d₆) RRR- ${alpha}$ -tocopherylacetate (d₆- ${alpha}$ -tocopheryl acetate), and d₀- ${gamma}$ -tocopherol, were giftsfrom James Clark of Cognis Nutrition and Health, LaGrange, IL.The isotopic purity of the d₆- ${alpha}$ -tocopheryl acetate was determinedto be 89% by liquid chromatography–mass spectrometry (LC-MS);the remainder was d₅- ${alpha}$ -tocopheryl acetate. d₉-all rac- ${alpha}$ -Tocopherylacetate, which was used as an internal standard, was providedby Carolyn Good of General Mills (Minneapolis, MN) and was synthesizedby Isotec Inc (Miamisburg, OH).

Study participants and protocol
The protocol for the present study was approved by the InstitutionalReview Board for the Protection of Human Subjects of the OregonState University, and all participants provided written consent.Healthy, nonsmoking, normolipidemic volunteers (n = 5; 3 menand 2 women) were selected on the basis of age (range: 18–35y; ± SD: 26.6 ± 6.2y), no nutritional supplement use (>6 mo), and exercise status(<5 h/wk of aerobic activity). To verify the participants'health status, a serum chemistry profile was conducted at theGood Samaritan Regional Medical Center in Corvallis, OR. Allparticipants had body mass indexes (BMIs; ± SD: 23.0 ± 2.0 kg/m²) and serum chemistries(not shown) within normal limits.

The participants sequentially completed each of the 3 trials,which were separated by a 2-wk washout period. During each trial,the participants consumed a serving of apples ( ${approx}$ 80 g) that wasfortified with 22 mg d₆- ${alpha}$ -tocopherol (see below for vacuum impregnationand deuterated vitamin E quantitation). The participants ingestedthe fortified apples alone (0 g fat; 0% kcal from fat) duringtrial 1, with a low-fat breakfast (2.4 g fat; 6% kcal from fat)consisting of a bagel with 30 g low-fat cream cheese duringtrial 2, or with a regular-fat breakfast (11.0 g fat; 21% kcalfrom fat) consisting of a bagel with 30 g regular-fat creamcheese during trial 2 (see Table 1 for complete dietary details).Lunch was controlled on the first day of each trial and wasconsumed between 1130 and 1230. Lunch (1300 kcal, 53 g fat,36% kcal from fat) consisted of a turkey sandwich with lettuceand tomato (no mayonnaise), 236 mL orange juice (Minute Maid;Coca-Cola Company, Houston, TX), and 30 g chips (Sun Chips;Frito-Lay, Dallas, TX). Other food (ie, snacks after 1500, dinner,etc) was consumed ad libitum. To estimate additional nutrientintakes until 0700 the following day, all participants completeda food record that was analyzed with the use of FOOD PROCESSOR(version 7.9; Salem, OR).

View this table:
[in this window]
[in a new window]

TABLE 1. Dietary intakes during the first day of each trial¹

After an overnight fast of ${approx}$ 12 h and immediately before consumingthe breakfast (t = 0 h), a blood sample was obtained from eachparticipant from the antecubital vein into blood collectiontubes containing 0.05 mL 15% K₃ EDTA (Vacutainer; Becton Dickinson,Franklin Lakes, NJ). After breakfast, blood samples were obtainedat 3, 6, 9, 12, 24, 36, 48, and 72 h. Tubes were kept on icefor <30 min before the plasma isolation. Plasma was separatedby centrifugation (500 x g, 15 min, 4 °C; Beckman TJ-6,Palo Alto, CA), divided into aliquots that were put into cryovials,frozen in liquid nitrogen, and stored at –80 °C untilanalyzed.

Labeled (d₆-) and unlabeled (d₀-) ${alpha}$ -tocopherol and unlabeled ${gamma}$ -tocopherol were extracted from the plasma (10) and analyzedby LC-MS as previously described (11, 12). Plasma total cholesteroland triacylglycerol concentrations were measured with kits obtainedfrom ThermoDMA (Louisville, CO), and the analyses were performedin accordance with the manufacturer's instructions.

Vacuum impregnation of apples with vitamin E
To emulsify and stabilize the labeled ${alpha}$ -tocopheryl acetate inthe water-based vacuum impregnation solution, a mixture (1:1:0.3,by wt) of 0.8 g d₆- ${alpha}$ -tocopheryl acetate, 0.8 g acetylated monoglyceride(Grindsted Acetem 50–00 pk; Danisco, New Century, KS),and 0.24 g polysorbate 80 (Integra, Renton, WA) was heated to70 °C followed by the addition of 200 g 70 °C 20% high-fructosecorn syrup solution (Western Family Foods Inc, Portland, OR).The solution was then homogenized (Polytron PT 10–35;Kinematica AG, Littau, Switzerland) for 90 s at 10 000 rpm.

Fuji apples (Washington State, fall 2004 crop) were washed withdistilled water, and cylindrical apple chunks (15 mm heightx 15 mm diameter pieces, without the skin) were obtained witha sterile stainless steel tubular cork borer and a knife. Theapple cylinders were cut in the axial direction. The pieceswere immediately immersed into distilled water to avoid contactwith air.

The goal was to enrich the apples with ${approx}$ 30 mg vitamin E/100 gapples. For treatment, freshly prepared apple pieces ( ${approx}$ 50 g)were immersed into 150 mL vacuum impregnation solution and placedin a chamber that was connected to a vacuum pump (Model 0211-P204;Gast Mfg Corp, Benton Harbor, MI). Vacuum pressure (100 mm Hg)was applied at room temperature for 15 min, then atmosphericpressure was restored for 30 min. The apples were removed fromthe solution, left to drain at room temperature for 15 min,then packed in 8" hinged clear shallow containers (Gourmet ClassicsDV 800S; Barrett Parkway, St Louis, MO). The packed sampleswere stored at 2 °C and 88% relative humidity until consumedwithin 48 h.

Apple pieces were pooled from various enrichment sessions andmixed thoroughly, and then aliquots were obtained for analysis.The d₆- ${alpha}$ -tocopherol enrichment of the apple pieces was measuredwith the use of LC-MS (11). The exact weight of apples thatwas necessary for delivery of 22 mg (± SD: 21.89 ± 0.34 mg) d₆- ${alpha}$ -tocopherol per servingwas calculated on the basis of the apple vitamin E concentrationof each batch of apples for each trial.

Mathematical and statistical analysis
Areas under the curve (AUCs) of plasma d₆- ${alpha}$ -tocopherol concentrationswere calculated for each person for each trial with the trapezoidalrule. Time to maximal concentration (T_max) and maximal concentrations(C_max) were identified by visual inspection of the data. ${alpha}$ –Tocopherolfractional disappearance rates (FDRs) and half-lives were calculatedfrom the plasma d₆- ${alpha}$ -tocopherol concentrations, as previouslydescribed (13).

Statistical comparisons between the treatments were performedwith GRAPHPAD PRISM (version 4; GraphPad Software, San Diego,CA). The statistical significance of treatment effects on AUC,T_max, and C_max was evaluated by a one-way analysis of variancewith repeated measures followed by Tukey's post hoc test whena significant main effect (P < 0.05) was observed. Data arereported as means ± SDs throughout the text; means ±SEs are shown in the figures.

The C_max increment that was dependent on dietary fat was estimatedby calculating the linear relation between the plasma d₆- ${alpha}$ -tocopherolC_max and fat ingested for each participant, then the slopesand intercepts were averaged. The amount absorbed was estimatedby multiplying the C_max with the plasma volume, which convertedthe value from µmol to mg. The fractional absorption wasestimated from the amount absorbed divided by the dose administered(22 mg d₆- ${alpha}$ -tocopherol).

No significant differences in plasma total cholesterol or triacylglycerolconcentrations were observed between dietary treatments. Becauseit was suggested that plasma tocopherol concentrations shouldbe adjusted for lipid concentrations (14), we performed the ${alpha}$ -tocopherol kinetic analyses with and without adjustment forcirculating lipid concentrations. After adjustment for lipids,we nonetheless observed no significant differences in the resultsand, therefore, have presented the ${alpha}$ -tocopherol concentrationsand analyses without adjustment for circulating lipids.

RESULTS

TOP
ABSTRACT
INTRODUCTION
SUBJECTS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Dietary fat intakes
The participants consumed vitamin E–enriched apples atbreakfasts that varied in amounts of fat, followed by a lunchthat contained a constant amount of fat (1300 kcal, 53 g fat,36% kcal from fat). During the first 24 h of each trial, theparticipants' daily fat intakes did not differ significantly,although there was some variability in the carbohydrate andprotein intake between trials largely due to the differencesin breakfast composition (Table 1).

Plasma unlabeled and deuterium-labeled ${alpha}$ -tocopherols
Compared with the 0% fat trial, plasma d₆- ${alpha}$ -tocopherol C_max doubledand tripled during the 6% and 21% fat trials, respectively (Figure1, Table 2). The increasing breakfast fat also increased themean (±SD) maximum percentage plasma d₆- ${alpha}$ -tocopherol absorbedfrom the total (labeled plus unlabeled) ${alpha}$ -tocopherol consumedfrom 8 ± 3% during the 0% fat trial to 14 ± 2%and 22 ± 6% for the 6% and 21% fat trials, respectively.

View larger version (32K):
[in this window]
[in a new window]

FIGURE 1.. Plasma labeled ${alpha}$ -tocopherol time course. The participants (n = 5) ingested vitamin E–fortified apples (22 mg d₆- ${alpha}$ -tocopherol/serving) after a breakfast that contained 0%, 6%, or 21% fat (percentage of total kcal). Each trial was separated by a 2-wk washout period. Plasma d₆- (labeled) and d₀- (unlabeled) ${alpha}$ -tocopherol ( ${alpha}$ -T) concentrations ( ± SE; analyzed by liquid chromatography–mass spectrometry) are shown at each time point for each trial.

View this table:
[in this window]
[in a new window]

TABLE 2. Plasma ${alpha}$ -tocopherol kinetics¹

Mean (±SD) plasma d₆- ${alpha}$ -tocopherol T_max (9 ± 2 h)did not significantly differ between the 3 trials, nor did eitherFDR (± SD for all trials:0.52 ± 0.07 pools/d) or the corresponding half-lives(± SD for all trials: 32 ±4 h). Additionally, FDRs were not significantly correlated withfat intake. The AUC is often used as a measure of bioavailability.Compared with the 0% dietary fat trial, the plasma d₆- ${alpha}$ -tocopherolAUC (0–72 h) doubled in the 6% fat trial and tripled inthe 21% fat trial, increasing from a mean (±SD) 68 ±42 µmol/L · h during the 0% fat trial to 124 ±29 and 209 ± 57 µmol/L · h for the 6% and21% fat trials, respectively (P < 0.05 between each of thetrials). Given the lack of change in T_max and FDR between thetrials, the increase in bioavailability with increased fat intakeresulted from an increase in vitamin E absorption.

Vitamin E absorption was estimated from each participant's plasmad₆- ${alpha}$ -tocopherol C_max. The mean (±SD) percentage d₆- ${alpha}$ -tocopherolabsorbed increased from 10 ± 4% in the absence of fatto 20% ± 2.5% during the 6% fat trial and 33 ±5% with the 21% fat trial (Table 2). These data show that ${alpha}$ -tocopherolabsorption was enhanced by the simultaneous consumption of increasingamounts of dietary fat.

Importantly, d₆- ${alpha}$ -tocopherol was absorbed from the apples inthe absence of fat. The increment in C_max that was dependenton dietary fat was also estimated (Figure 2). In the absenceof fat, the average (±SD) C_max was 2.0 ± 0.8 µmol/L,which is equivalent to 2.7 ± 1.0 mg d₆- ${alpha}$ -tocopherol absorbed.With each gram of fat consumed, C_max increased by 0.33 µmol/L,which is equivalent to an increase of 0.43 mg d₆- ${alpha}$ -tocopherolabsorbed. The data estimated from the disappearance curves weresimilar to the C_max actually measured for the participants (Figure1).

View larger version (23K):
[in this window]
[in a new window]

FIGURE 2.. Plasma labeled ${alpha}$ -tocopherol maximum concentration (C_max) as a function of breakfast fat content. Plasma d₆- ${alpha}$ -tocopherol C_max during each of the dietary treatments was linearly related to fat intake in each of the participants. Plasma d₆- ${alpha}$ -tocopherol C_max was significantly (P < 0.0001) correlated with dietary fat consumption; each ingested gram of dietary fat resulted in a corresponding increase in plasma d₆- ${alpha}$ -tocopherol C_max of 0.33 µmol/L (linear regression: y = 0.33x + 2.17; R² = 0.72) or an increase of 0.43 mg/g fat consumed.

At baseline (t = 0 h), plasma unlabeled ${alpha}$ -tocopherol concentrationswere not significantly different between trials 1, 2, and 3( ± SD: 20.8 ± 2.9,21.1 ± 6.6, and 20.7 ± 3.6 µmol/L, respectively;Figure 1

and Table 2

), nor were plasma ${gamma}$ -tocopherol concentrationssignificantly different (1.2 ± 0.5, 1.1 ± 0.4,and 0.9 ± 0.3 µmol/L, respectively). During thecourse of the trials, no significant changes in either plasmatotal ${alpha}$ -tocopherol (Table 2

) or ${gamma}$ -tocopherol concentrations (notshown) were observed from baseline. Therefore, the baselined₀- ${alpha}$ - tocopherol concentrations were used to calculate the dailyplasma ${alpha}$ -tocopherol efflux as follows:

Formula 1 (1)
From the FDR (pool/d), the plasma pool size(calculated to be 4.5% body weight; in kg), and the baselineplasma d₀- ${alpha}$ -tocopherol concentration for each participant, themean (±SD) calculated plasma ${alpha}$ -tocopherol efflux was 13± 3 mg/d (means for each trial are given in Table 2).

Vitamin E requirements based on vitamin kinetics
Vitamin E requirements can be approximated from the presentstudy, given that the intakes of both dietary and supplementalvitamin E were relatively limited and did not appear to significantlychange plasma ${alpha}$ -tocopherol pool sizes. As shown in Figure 3,the rate of ${alpha}$ -tocopherol entering or leaving the tissues cannotbe specifically calculated with the present design; however,some estimates can be made. The range of total (d₀ + d₆) ${alpha}$ -tocopherolabsorbed was from 4.8 to 9.2 mg. The ${alpha}$ -tocopherol flux to tissues(k_t) appears to be an estimate of tissue ${alpha}$ -tocopherol requirements.Our previous study (16) suggested the tissue ${alpha}$ -tocopherol effluxrate was 0.191 pools/d, which is equivalent to a mean (±SD)5.1 ± 0.9 mg excreted from the body (on the basis ofthe present participants' baseline plasma ${alpha}$ -tocopherol concentrationsand plasma volumes). The mean (±SD) estimate for k_t of5 ± 1 mg/d is roughly equivalent to the rate of absorptionduring trial 1 (k_a = 4.8 ± 2.0 mg/d). The sum of these2 rates (10 ± 3 mg/d) is roughly equivalent to the estimatedefflux (k_e) of 15 ± 5 mg/d. Thus, at steady state, theabsorption of 5 ± 2 mg/d is sufficient to meet tissueneeds. If this value represents the amount of ${alpha}$ -tocopherol requiredby the tissues, and intestinal absorption of ${alpha}$ -tocopherol is33%, then the mean (±SD) dietary vitamin E requirementis ${approx}$ 15 ± 6 mg/d. This range of the estimated dietary vitaminE requirements confirms that the current Dietary RecommendedAllowance of 15 mg/d is substantially correct. However, mostAmericans' vitamin E intakes are well below this amount. Indeed,the mean (±SD) dietary intake of the participants inthe present study was 7 ± 3 mg ${alpha}$ -tocopherol/d withoutconsumption of the vitamin E–fortified apples; the fortifiedapples added 22 mg.

View larger version (20K):
[in this window]
[in a new window]

FIGURE 3.. Model of plasma ${alpha}$ -tocopherol kinetics. Only a portion of the vitamin E (in either the apples or diet) is absorbed (k_a) and incorporated into the plasma vitamin E pool. This plasma pool includes the liver, because vitamin E moves in a rapid equilibrium between the liver and plasma (15). Efflux (k_e) from the plasma pool can go to extrahepatic tissues (k_t) or can be excreted from the body (k_b). The design of the present study does not allow estimation of the rates of k_t or k_b. However, our previous estimates of vitamin E utilization (0.191 pools/d; 16) allowed us to estimate the k_t to equal 5 ± 1 mg/d from the plasma d₀- ${alpha}$ -tocopherol concentrations and volume. This rate is equivalent to the mean (±SD) rate of absorption during trial 1 (k_a = 4.8 ± 2.0 mg/d). The sum of these 2 rates (10 ± 3 mg/d) was roughly equivalent to the mean estimated efflux (k_e) of 15 ± 5 mg/d. (Note that k_e is somewhat higher, probably because it is influenced by excretion of newly absorbed ${alpha}$ -tocopherol.) Thus, at steady state, the mean absorption of 5 ± 2 mg/d is sufficient to meet tissue needs. A daily ${alpha}$ -tocopherol intake of 15 ± 6 mg is required when the fraction absorbed is 33%.

	DISCUSSION

TOP ABSTRACT INTRODUCTION SUBJECTS AND METHODS RESULTS DISCUSSION REFERENCES

The purpose of the present study was three-fold: 1) to assessthe efficacy of vitamin E–fortified apples as a low-fatvitamin E delivery system, 2) to assess the influence of faton vitamin E absorption, and 3) to assess human vitamin E requirementsfrom plasma ${alpha}$ -tocopherol kinetics at a dosage of ${alpha}$ -tocopherolfound in food.

With respect to bioavailability of the vitamin E in fortifiedapples, the data showed that ${approx}$ 10% of the 22 mg d₆- ${alpha}$ -tocopherolwas absorbed in the absence of fat or other foods. Additionally,an increase of 1 g fat consumed increased ${alpha}$ -tocopherol absorptionby 0.43 mg. The 21% fat breakfast contained 11 g fat and resultedin a 33% ${alpha}$ -tocopherol absorption. This value is less than the45% absorption rate estimated in thoracic duct-cannulated rats(17) or the 55–79% rate estimated in humans when radioactivevitamin E was used to estimate absorption (18). Thus, it islikely that the percentage absorption would have been largerwith a higher fat breakfast, but additional studies are neededto estimate maximal absorption rates. These data also emphasizethe relatively poor absorption of vitamin E when it is consumedwithout fat, as was observed when vitamin E pills were consumedwithout food (13). Note that the ideal method for measuringvitamin E absorption would be to feed one labeled dose and injectanother labeled dose of vitamin E. The ratio of the consumeddose divided by the injected dose (which is assumed to be 100%)would yield the fraction absorbed (19). This method, however,depends on the availability of a preparation of vitamin E thatis acceptable for intravenous injection in humans, which doesnot currently exist; the only intravenous preparation had adverseeffects in premature infants (20).

The finding of increased absorption of ${alpha}$ -tocopherol in the presenceof dietary fat is consistent with results of other fat-solublenutrients. Compared with the bioavailability of lycopene administeredin steamed tomatoes, the bioavailability of lycopene increased3-fold when administered in oil (21). Carotenoid bioavailabilityis higher with full-fat salad dressing than with reduced-fatsalad dressing (22). Similarly, ingestion of avocado significantlyenhanced carotenoid absorption from salad and salsa (23). Inaddition, increasing dietary fat increases the absorption ofvitamin E from supplements (13, 24). Roodenberg et al (25) suggestedthat a 3% fat intake was sufficient for optimal vitamin E bioavailability.However, they measured bioavailability as increased plasma ${alpha}$ -tocopherolconcentrations after 1 wk of supplementation with 50 mg ${alpha}$ -tocopherolin 50 g of a low or high fat spread that accompanied a mealthat resulted in an intake of <6.5 g fat or <45 g fat.From our study, it was apparent that the fat amount that wasconsumed concurrently with vitamin E was critical for its absorption.Note that the vitamin E–fortified apples were consumedwith breakfast; the lunch eaten ${approx}$ 5 h later contained 36% fatand yet had no apparent effect on absorption. The vitamin Ein the study by Roodenberg et al (25) was dissolved in a spread;thus, it is difficult to estimate whether the amount of fatneeded for vitamin E absorption from a low-fat food is the sameamount needed to dissolve vitamin E into a micellarized form.As also noted from our study, no significant changes in totalplasma ${alpha}$ -tocopherol were detectable with the low doses we used;therefore, it is imperative to use labeled ${alpha}$ -tocopherol to detectchanges in bioavailability of vitamin E from dietary sources.

With respect to vitamin E kinetics, breakfast fat (0–21%)consumption had no significant influence on ${alpha}$ -tocopherol ratesof disappearance, half-lives, or T_max values during the 3 trialsin normolipidemic persons who consumed daily diets containing34–38% fat. Because the plasma vitamin E pool was essentiallyunchanged during each of the trials and between the trials,the absorbed d₆- ${alpha}$ -tocopherol dose did not significantly changeplasma vitamin E kinetics. The absorbed amounts were estimatedfrom the plasma d₆- ${alpha}$ -tocopherol C_max. These estimated amountsare the minimum quantities that had to be absorbed to achievethe observed plasma d₆- ${alpha}$ -tocopherol concentrations and, therefore,underestimate the fractional d₆- ${alpha}$ -tocopherol absorption becausethey do not take tissue distribution into account.

The daily ${alpha}$ -tocopherol requirement for normal healthy personswas estimated by the Food and Nutrition Board (5) with datafrom studies that were carried out in the 1950s that evaluatedthe amount of dietary vitamin E necessary to prevent peroxide-inducederythrocyte hemolysis in men who were depleted of vitamin E.The Estimated Average Requirement is 12 mg ${alpha}$ -tocopherol/d (5).The mean (±SD) ${alpha}$ -tocopherol requirement is ${approx}$ 15 ±2 mg/d when the amount required by the tissues is ${approx}$ 5 mg/d andabsorption is 33%; when absorption is 50%, the ${alpha}$ -tocopherol requirementis 10 ± 1 mg/d. This range of the estimated dietary vitaminE requirements (10–15 mg/d) confirms that the currentDaily Recommended Intakes are substantially correct. However,most Americans' vitamin E intakes are well below this amount(3), which reemphasizes the importance of enriching low-fatfoods with vitamin E as a means of increasing vitamin E intakesbecause the long-term consequences of suboptimal vitamin E intakesare unknown.

Obesity and various chronic diseases are associated with increasedoxidative stress (26). Vitamin E intakes are low in most Americansdespite the obvious overconsumption of calories. We showed thatit is possible to fortify low-fat fruit (apples) with vitaminE and that the vitamin E from this fruit is bioavailable; wealso showed that a serving of vitamin E–fortified applesmeets the calculated tissue vitamin E requirements. The presentstudy emphasizes our lack of information about vitamin E requirementsin humans—even the fractional absorption of vitamin Eis not known with certainty. Appropriate studies that estimatebioavailability, such as those by Levine et al (19) for vitaminC, cannot be carried out because no injectable forms of vitaminE are available. Moreover, the present study showed that vitaminE bioavailability is greatly influenced by both the food matrixand the presence of dietary fat. Additional studies are neededto determine the amount of dietary fat necessary for optimalvitamin E absorption, because extrapolation of our data suggestthat vitamin E absorption would continue to rise with the additionalingestion of dietary fat, a finding that seems highly unlikely.Furthermore, more invasive experimental approaches will be necessaryto accurately determine the rates of vitamin E delivery to tissues.Collectively, these investigations will enable a more sensitiveformulation of human dietary vitamin E requirements.

ACKNOWLEDGMENTS

We thank our participants and Rajasekhar Ramakrishnan for insightfuldiscussions. We also thank the Natural Source Vitamin E Associationfor providing partial support for the purchase of the LC-MS.We thank James Clark of Cognis Nutrition and Health (LaGrange,IL) for the gifts of unlabeled (d₀) RRR- ${alpha}$ -tocopherol, d₆-RRR- ${alpha}$ -tocopherylacetate, and d₀- ${gamma}$ -tocopherol and Carolyn Good of General Millsfor providing the d₉-all rac- ${alpha}$ -tocopheryl acetate, which wasused as an internal standard (synthesized by Isotec Inc, Miamisburg,OH).

All authors participated in the study design. SWL, S-iP, andYZ prepared the deuterium-labeled vitamin E-fortified apples.RSB and SWL carried out the sample collection and analyses.RSB and MGT wrote the initial draft of the manuscript, and allauthors contributed to the editing and review of the manuscript.None of the authors had any conflicts of interest.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
SUBJECTS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Mokdad AH, Marks JS, Stroup DF, Gerberding JL. Correction: actual causes of death in the United States, 2000. JAMA 2005;293:293–4.[Free Full Text]
Mokdad AH, Marks JS, Stroup DF, Gerberding JL. Actual causes of death in the United States, 2000. JAMA 2004;291:1238–45.[Abstract/Free Full Text]
Maras JE, Bermudez OI, Qiao N, Bakun PJ, Boody-Alter EL, Tucker KL. Intake of alpha-tocopherol is limited among US adults. J Am Diet Assoc 2004;104:567–75.[Medline]
Mueller-Cunningham WM, Quintana R, Kasim-Karakas SE. An ad libitum, very low-fat diet results in weight loss and changes in nutrient intakes in postmenopausal women. J Am Diet Assoc 2003;103:1600–6.[Medline]
Food and Nutrition Board, Institute of Medicine. Dietary reference intakes for vitamin C, vitamin E, selenium, and carotenoids. Washington, DC: National Academy Press, 2000.
Park S-i, Leonard SW, Traber MG, Zhao Y. Vitamin E and mineral fortification in fresh-cut apples (Fuji) using vacuum impregnation. Nutr Food Sci 2005;35:393–402.
Xie J, Zhao Y. Nutritional enrichment of fresh apple (Royal Gala) by vacuum impregnation. Int J Food Sci Nutr 2003;54:387–98.[Medline]
Eitenmiller RR, Lee J. Vitamin E. Food chemistry, composition and analysis. New York, NY: Marcel Dekker, Inc, 2004.
Traber MG. Vitamin E. In: Ross AC, ed. Modern nutrition in health and disease. Baltimore, MD: Williams & Wilkins, 1999:347–62.
Podda M, Weber C, Traber MG, Packer L. Simultaneous determination of tissue tocopherols, tocotrienols, ubiquinols, and ubiquinones. J Lipid Res 1996;37:893–901.[Abstract]
Leonard SW, Bruno RS, Paterson E, et al. 5-nitro-gamma-tocopherol increases in human plasma exposed to cigarette smoke in vitro and in vivo. Free Radic Biol Med 2003;35:1560–7.[Medline]
Lauridsen C, Leonard SW, Griffin DA, Liebler DC, McClure TD, Traber MG. Quantitative analysis by liquid chromatography-tandem mass spectrometry of deuterium-labeled and unlabeled vitamin E in biological samples. Anal Biochem 2001;289:89–95.[Medline]
Leonard SW, Good CK, Gugger ET, Traber MG. Vitamin E bioavailability from fortified breakfast cereal is greater than that from encapsulated supplements. Am J Clin Nutr 2004;79:86–92.[Abstract/Free Full Text]
Gross M, Yu X, Hannan P, Prouty C, Jacobs DR Jr. Lipid standardization of serum fat-soluble antioxidant concentrations: the YALTA study. Am J Clin Nutr 2003;77:458–66.[Abstract/Free Full Text]
Traber MG, Ramakrishnan R, Kayden HJ. Human plasma vitamin E kinetics demonstrate rapid recycling of plasma RRR- ${alpha}$ -tocopherol. Proc Natl Acad Sci U S A 1994;91:10005–8.[Abstract/Free Full Text]
Bruno RS, Ramakrishnan R, Montine TJ, Bray TM, Traber MG. ${alpha}$ -Tocopherol disappearance is faster in cigarette smokers and is inversely related to their ascorbic acid status. Am J Clin Nutr 2005;81:95–103.[Abstract/Free Full Text]
Traber MG, Kayden HJ, Green JB, Green MH. Absorption of water-miscible forms of vitamin E in a patient with cholestasis and in thoracic duct-cannulated rats. Am J Clin Nutr 1986;44:914–23.[Abstract/Free Full Text]
MacMahon MT, Neale G. The absorption of alpha-tocopherol in control subjects and in patients with intestinal malabsorption. Clin Sci 1970;38:197–210.[Medline]
Levine M, Conry-Cantilena C, Wang Y, et al. Vitamin C pharmacokinetics in healthy volunteers: evidence for a recommended dietary allowance. Proc Natl Acad Sci U S A 1996;93:3704–9.[Abstract/Free Full Text]
Arrowsmith JB, Faich GA, Tomita DK, Kuritsky JN, Rosa FW. Morbidity and mortality among low birth weight infants exposed to an intravenous vitamin E product, E-Ferol. Pediatrics 1989;83:244–9.[Abstract/Free Full Text]
Tang G, Ferreira AL, Grusak MA, et al. Bioavailability of synthetic and biosynthetic deuterated lycopene in humans. J Nutr Biochem. 2005;16:229–35.[Medline]
Brown MJ, Ferruzzi MG, Nguyen ML, et al. Carotenoid bioavailability is higher from salads ingested with full-fat than with fat-reduced salad dressings as measured with electrochemical detection. Am J Clin Nutr 2004;80:396–403.[Abstract/Free Full Text]
Unlu NZ, Bohn T, Clinton SK, Schwartz SJ. Carotenoid absorption from salad and salsa by humans is enhanced by the addition of avocado or avocado oil. J Nutr 2005;135:431–6.[Abstract/Free Full Text]
Jeanes YM, Hall WL, Ellard S, Lee E, Lodge JK. The absorption of vitamin E is influenced by the amount of fat in a meal and the food matrix. Br J Nutr 2004;92:575–9.[Medline]
Roodenburg AJ, Leenen R, van het Hof KH, Weststrate JA, Tijburg LB. Amount of fat in the diet affects bioavailability of lutein esters but not of ${alpha}$ -carotene, ß-carotene, and vitamin E in humans. Am J Clin Nutr 2000;71:1187–93.[Abstract/Free Full Text]
Davi G, Falco A, Patrono C. Determinants of F2-isoprostane biosynthesis and inhibition in man. Chem Phys Lipids 2004;128:149–63.[Medline]

Received for publication October 17, 2005. Accepted for publication October 26, 2005.

This article has been cited by other articles:

M. G Traber
Heart disease and single-vitamin supplementation
Am. J. Clinical Nutrition, January 1, 2007; 85(1): 293S - 299S.
[Abstract] [Full Text] [PDF]

A. J Clifford, F. F de Moura, C. C Ho, J. C Chuang, J. Follett, J. G Fadel, and J. A Novotny
A feasibility study quantifying in vivo human {alpha}-tocopherol metabolism
Am. J. Clinical Nutrition, December 1, 2006; 84(6): 1430 - 1441.
[Abstract] [Full Text] [PDF]

This Article

Abstract

Full Text (PDF)

Purchase Article

View Shopping Cart

Alert me when this article is cited

Alert me if a correction is posted

Citation Map

Services

Similar articles in this journal

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via Google Scholar

Google Scholar

Articles by Bruno, R. S

Articles by Traber, M. G

Search for Related Content

PubMed

PubMed Citation

Articles by Bruno, R. S

Articles by Traber, M. G

Agricola

Articles by Bruno, R. S

Articles by Traber, M. G