Green Tea Is a Poor Contributor to Tissue Folate in a Folate Depletion-Repletion Rat Model ()
1. Introduction
Folate has a role in the transfer and utilization of onecarbon groups and is involved in the de novo synthesis of nucleic acid bases and amino acids. Folate deficiency can lead to megaloblastic anemia [1], and low periconceptional folate status in women is related to an increased risk of fetal abnormalities such as neural tube defects (NTDs) [2]. In addition, low folate status leads to an increase in plasma homocysteine level, which is a risk factor for atherosclerosis, and impairs DNA synthesis and repair, resulting in increased DNA damage and consequently cancer initiation [3,4].
Folate naturally occurring in food (“natural folate”) mainly occurs in the polyglutamated form, but is converted to the monoglutamate form before absorption by deconjugation in the intestine. In contrast, synthetic folic acid (pteroylmonoglutamic acid), which is used for dietary supplementation and in fortified food, is the most oxidized and stable form, and is highly bioavailable. The bioavailability of folic acid is estimated to be, on average, about 2 times that of natural folate, but this varies depending on the food [1,5]. Excess intake of folic acid is of concern due to the possibility masking of vitamin B12 deficiency [1], increasing the risk of cancer growth when a tumor is present [4], and childhood asthma when taken in late pregnancy [6]. Generally, it is desirable to obtain folate from food because this approach minimizes excessive intake of this important vitamin. However, bioavailability of natural folate from foods is reported to vary greatly [5] due to differences between foods in the form of folate present, the food matrix in which it exists, and the presence of factors affecting its absorption and metabolism.
Intake of green tea (Camellia sinensis) has attracted a great deal of attention because it has been suggested to have health benefits in terms of protecting against vascular disease and some types of cancer due to the presence of catechins [7]. Green tea also contains natural folate and is regarded as one of the sources of folate, along with vegetables and fruit, in the Japanese diet [8]. However, green tea catechins including (−)-epigallocatechin gallate (EGCg) are reported to inhibit uptake of folic acid by Caco-2 cell monolayers [9] and inhibit dihydrofolate reductase (DHFR) activity in vitro [10]. Dihydrofolate reductase is an important enzyme because it catalyzes the reduction of folic acid to 7,8-dihydrofolate (DHF) and 5,6,7,8-tetrahydrofolate (THF), which acts as a coenzyme for several one-carbon group transfer reactions after its conversion to 5,10-methylenetarthydrofolate and 5-methyltetrahydro-folate [10]. A cross-sectional study reported a correlation between low serum folate concentration and high consumption of green tea or oolong tea during pregnancy [11]. Further, intake of green tea extract at 0.9 g/day has been shown to decrease maximum concentration and area under the blood concentration time curve of folic acid in human subjects [12]. On the other hand, consumption of green tea catechin (approximately 670 mg/day) did not influence plasma folate concentration in healthy men, and only high-dose green tea catechins (0.5% in diet) simultaneously added to folic acid in the diet decreased serum folic acid level in rats [13]. Accordingly, it remains unclear whether 1) natural folate in green tea is bioavailable, and 2) EGCg at the low dose found in green tea attenuates folic acid utilizetion in vivo. In this study, we examined the above questions in a modified folate depletion/repletion rat model [14].
2. Materials and Methods
2.1. Chemicals and Diet
Folic acid and EGCg were obtained from Wako Pure Chemical Ltd. (Osaka, Japan). For the folate microbeological assay, folinic acid calcium salt pentahydrate, Lactobacillus rhamnosus (strain ATCC 27773) and folic acid casei medium were obtained from Fluka (Buchs, Switzerland), the American Type Culture Collection (Rockville, MD, USA), and Becton Dickinson (Sparks, MD, USA), respectively. A folate-deficient diet (Dyets version of the Clifford/Kuory folate-deficient amino acid rodent diet, #517777) was purchased from Dyets (Bethlehem, PA, USA). This diet is composed of folate-free amino acids with the recommended amount of vitamins except folate, and the addition of 1% succinylsulfathiazole to minimize intestinal folate synthesis. Powdered green tea (matcha), spinach, and chicken liver were purchased at local grocery stores (Tokyo, Japan). The spinach and chicken liver were lyophilized, ground finely with a mortar and pestle, and stored at −80˚C until use. Total folate content in food samples (μg/g dry weight) was 10.2 in powdered green tea, 23.2 in freeze-dried spinach, and 57.0 in chicken liver. Food samples or folic acid were added to the folate-deficient diet at a folate concentration of 800 μg/kg diet. The percentage of food sample in the diet was 7.8% for powdered green tea, 3.4% for freeze-dried spinach, and 1.4% for chicken liver. The catechin content in powdered green tea was 22 mg/gand these catechins were composed of 50% EGCg, 14% (−)-epicatechin gallate, 13% (−)-epigallocatechin, 13% (+)-catechin, 6% (−)-epicatechin, and 3% (−)-catechin gallate.
2.2. Animals
Male Wistar rats purchased from Japan Clea (Tokyo, Japan) were housed individually in wire bottomed cages in a room maintained at a constant temperature of 23˚C ± 1˚C with a 12-hour light-dark cycle. Following the experiments, the rats were euthanized with sodium pentobarbital, blood was taken from the abdominal aorta with a heparinized syringe, and the liver, femurs, and tibiae were removed. Bone marrow cell samples were prepared from the femurs and tibiae according to a method reported previously [15]. All procedures were in accordance with the National Institute of Health and Nutrition guidelines for the Care and Use of Laboratory Animals, and they were approved by the ethical committee of the National Institute of Health and Nutrition.
2.3. Folate Depletion/Repletion Model
The folate depletion/repletion procedure was performed as reported previously [14] with the exception that the present study used a shorter 7-day repletion period, in order to determine the initial difference in how folate in diverse test samples is incorporated into the body. Rats (4 - 5 weeks old) were given ad libitum access to a folate-deficient diet for 4 weeks, and then given the same diet with supplementary folic acid or food samples for 7 days (each group consisted of 5 - 6 rats). A preliminary study showed that plasma folate transiently increased from 0.5 to 6 hours after an excess folic acid administration (330 μg/kg body weight), but returned to the basal level at 8 hours. Based on this finding, blood and tissue samples were taken 24 hours after each intragastric gavage administration of folic acid, or after overnight fasting when dietary folate supplementation was given. During the study, body weights and dietary intakes were measured every day.
There were 4 parts to the study (Figure 1). In the timedependent study, the folate-depleted rats (n = 6) were administered folic acid daily by intragastric gavage. The folic acid was dissolved in 0.1 M sodium bicarbonate at a dose of 330 μg/kg body weight, and blood was taken every day 24 hours after each folic acid administration. In the dose-response study, the folate-depleted rats were divided into 4 groups (n = 5 - 6) to be administered one of 4 doses of folic acid daily (0, 4, 40, or 400 μg/kg body weight/day) by intragastric gavage. In the dietary folate supplementation study, the folate-depleted rats were divided into 5 groups (n = 5 - 6): one group underwent monitoring of folate status in the depletion phase, and the other 4 were fed a diet containing powdered green tea, spinach, chicken liver, or folic acid. Folate intake in each group was adjusted from the amount of food intake during the previous days (about 11.5 g/day), and the calculated dose was set at 40 μg/kg body weight. The powdered green tea diet contained about 1.73 g of total catechins/kg diet, and the estimated total catechin dose was approximately 90 mg/kg body weight. In the study to evaluate the effect of EGCg on folic acid absorption, folate-depleted rats were divided into 3 groups (n = 5 - 6) to be given folic acid (31 μg/kg body weight), EGCg (8 mg/kg body weight), or folic acid with EGCg (folic acid 31 μg and EGCg 8 mg/kg body weight) daily by intragastric gavage.
2.4. Analytical Methods
For hematocrit measurements, blood was transferred to a capillary tube and centrifuged at 10,000 g for 10 minutes. Plasma was prepared by centrifugation at 1500 g for 15 minutes at 4˚C. Whole blood and plasma were immediately mixed with 0.5% ascorbic acid to stabilize folate and stored at −80˚C until folate analysis. The liver and bone marrow cell samples were homogenized or sonicated with 9 volumes of folate extraction buffer (50 mM phosphate buffer, 0.5% ascorbic acid, final pH 6.1). Total folate concentration in the plasma and conjugase-treated liver and bone marrow samples was analyzed using the microbiological assay described elsewhere [16]. Erythrocyte folate concentration was calculated using the following formula: [whole blood folate-{plasma folate x (1- hematocrit)}]/hematocrit. Plasma homocysteine was measured by HPLC using a fluorescence detector [17]. Protein was measured using a BCA protein assay kit (Pierce, Rockford, IL, USA). Folate content in food samples was determined by microbiological assay with the tri-enzyme treatment method [18]. The catechin content in powdered green tea was analyzed by the HPLC method [19].
Figure 1. Animal treatment in this study. Rats were sacrificed at the time point shown as an arrow.
2.5. Statistical Analyses
Data are presented as the mean ± standard deviation (SD) for individual groups. Data were analyzed by one-way analysis of variance followed by Dunnett’s multiple comparison test. Pearson’s correlation coefficient was used to determine the association between tissue folate and plasma total homocysteine. These statistical analyses were performed using GraphPad Prism version 5.01 (GraphPad Software, Inc., San Diego, CA, USA). Values of p < 0.05 were considered significant.
3. Results
3.1. Confirmation of the Folate Depletion/Repletion Rat Model
Rats were fed a folate-deficient diet for 4 weeks to minimize the background level of plasma folate, and they were then given folic acid at 330 μg/kg body weight/day by intragastric gavage, daily for 7 days. Before administration of folic acid (on day 0 of repletion), plasma folate levels decreased to about 10% of those in the control diet rats. Levels then increased with the consecutive daily administration of folic acid, by 4-fold on day 5 and by 7-fold on day 7 (data not shown). Next, folate-depleted rats (maintained on the folate-deficient diet for 4 weeks) were intragastrically administered various doses of folic acid (0, 4, 40, or 400 μg/kg body weight/day) for 7 days. Changes in body weight during the experimental period are shown in Figure 2. Final body weight was significantly higher in rats given high doses of folic acid. The administration of folic acid increased folate levels in plasma, liver, and bone marrow in a dose-dependent manner and decreased plasma homocysteine level (Figure 3). Plasma total homocysteine level was negatively
Figure 2. Changes in body weight in rats fed a folate-deficient diet followed by repletion with various doses of folic acid. Rats fed a folate-deficient diet for 4 weeks were intragastrically given various doses of folic acid while maintaining the same folate-deficient diet for 7 days. ■: Depletion phase, ◆: 0 µg/kg body weight/day, △: 4 µg/kg body weight/day, ○: 40 µg/kg body weight/day, ▲: 400 µg/kg body weight/day. Values are mean ± SD, n = 5 - 6.
Figure 3. Dose-dependent repletion effect of folic acid on body weight, folate level in tissues, and homocysteine level in plasma in a folate depletion/repletion rat model. Rats fed a folate-deficient diet for 4 weeks were intragastrically given various doses of folic acid (0, 4, 40, or 400 μg/kg body weight/day) for 7 days. (a) Body weight; (b) plasma folate level; (c) erythrocyte folate level; (d) liver folate level; (e) bone marrow folate level; (f) plasma total homocysteine level. Values are mean ± SD, n = 5 - 6. aSignificantly different from 0 μg/kg body weight/day group (p < 0.05).
correlated with folate level in plasma, liver, and bone marrow (r = −0.75, −0.74, −0.86, respectively, p < 0.05 for all), but not with erythrocyte folate level, which was only significantly increased at the highest dose of folic acid (i.e., 400 μg/kg body weight/day). Significant changes in folate and homocysteine levels were detected at a folic acid dose of 40 μg/kg body weight/day or greater.
3.2. Absorption of Powdered Green Tea Folate Relative to Folate in Spinach and Liver, and to Folic Acid
Diets containing either natural folates or folic acid (with the dose of folate set at 40 μg/kg body weight/day) were given to folate-depleted rats to cause folate repletion. Repletion with folic acid increased plasma and liver folate levels, and decreased plasma homocysteine levels when compared with those in the depletion phase (Table 1). Repletion with natural folate increased folate levels in the plasma and liver, but not in the bone marrow. In contrast to liver and plasma folate levels, bone marrow folate level was further diminished in the rats fed the powdered green tea and chicken liver diets. No significant increase in erythrocyte folate level was detected following the treatments (data not shown). When compared to the folic acid group, relative changes in folate levels among plasma, liver, and bone marrow in the depletion phase ranged from 27% to 88% in the spinach group, −13% to 42% in the chicken liver group and −61% to 21% in the powdered green tea group.
3.3. Effect of EGCg on Folic Acid Utilization
Influence of low-dose EGCg on folic acid utilization was evaluated in the folate depletion/repletion rat model. The folate-depleted rats were given intragastrically either folic acid (31 µg/kg body weight), EGCg (8 mg/kg body weight), or folic acid with EGCg, on a daily basis. Folic acid administration increased folate concentration in plasma, liver, and bone marrow and decreased plasma homocysteine level (Figure 4). Such changes resulting from folic acid treatment were also detected in the presence of EGCg, suggesting that EGCg at the tested dose did not influence utilization of folic acid.
4. Discussion
In the present study, we showed that natural folate from green tea was less bioavailable than folate from other sources in a folate depletion/repletion rat model. Food folate bioavailability estimated based on the increase in plasma and liver folate concentration would be only 17% - 21% for green tea folate, 27% - 42% for chicken liver folate, and 57% - 88% for spinach folate, when compared to folic acid as a reference. Our estimation of spinach folate bioavailability is comparable to that reported by Clifford [20], who showed that bioavailability of folate in spinach is 70% - 90% of that of folic acid in a depletion/repletion rat model. The present findings suggest that green tea is a poor source of folate and in fact could negatively impact folate status. The present study supports an epidemiological study that showed an association between low plasma folate level and high consumption of green tea [21].
It is important to define the system by which the bioavailability of green tea folate is estimated. In our system, rats were fed a folate-deficient diet for 4 weeks and then given test samples for 7 days, and folate bioavailability was estimated from the increase in the concentration of folate in plasma, liver, and bone marrow and the decrease in the concentration of plasma homocysteine. The folate-depletion period is the same as that described in previous reports [14], but our repletion time was shorter (7 days versus 4 weeks). We considered the 7-day repletion period useful to detect initial differences in how folate in diverse test samples is incorporated into the body, and to minimize the effect of substances other than folate in test food samples, particularly those with in
Table 1. Effect of folate repletion from powdered green tea relative to spinach, chicken liver, and folic acid in a folate depletion/repletion rat model.
Rats fed a folate-deficient diet for 4 weeks were divided into 5 groups: one group was killed to monitor the folate levels in the depletion phase, and the other 4 groups were given the same folate-deficient diet supplemented with one of 4 test foods/substances (folic acid as a reference, powdered green tea, spinach, and chicken liver) for 7 days. The folate intake dose was set at 40 μg/kg body weight/day. Values are the means ± SD, n = 5 - 6. aSignificantly different from folic acid (p < 0.05).
Figure 4. Influence of EGCg on repletion of folic acid in a folate depletion/repletion rat model. Rats fed a folate-deficient diet for 4 weeks were intragastrically given either folic acid (31 µg/kg body weight), EGCg (8 mg/kg body weight) or folic acid + EGCg, while maintaining the same folatedeficient diet for 7 days. (a) Plasma folate level; (b) liver folate level; (c) bone marrow folate level; (d) plasma total homocysteine level. Values are mean ± SD, n = 5 - 6. aSignificantly different from folic acid group (p < 0.05).
low folate concentration. In the case of powdered green tea, the folate concentration in the test diet was 7.8%. In the present study, the repletion effect with folic acid was consistently observed among plasma, liver, and bone marrow, while that with test food samples differed among these tissues. Changes in bone marrow folate status appeared delayed compared with those in plasma and liver, particularly for powdered green tea, which caused further depletion of bone marrow folate following the 7-day repletion period. These findings suggest that changes in bone marrow folate may be more evident later than examined here, and that green tea is not a good source of folate. Although we did not validate our test system against a human model, our rat model provides a practical initial approach to elucidating the bioavailability of green tea folate.
Erythrocyte folate level is well known as a stable indicator of body folate stores, and we confirmed this in the present study; erythrocyte folate level was quite stable even after 4 weeks of folate depletion. This stability is due to the relatively long life span of the erythrocyte (about 60 days in the rat [22]) after it emerges from the bone marrow and enters the bloodstream. On the other hand, the concentration of folate in bone marrow, which, like the liver, contains high amounts of folate [23], clearly changed due to depletion and repletion of folic acid, indicating that folate was taken up by the developing erythrocytes in the bone marrow. The results indicate that an increase in bone marrow folate is a good indicator of the availability of both folic acid and natural folate. Moreover, an increase in the concentration of tissue folate was accompanied by a decrease in the concentration of plasma homocysteine when the repletion was performed with folic acid, but such a correlation was not observed with the food samples, particularly powdered green tea. This may be due to contributions of other substances within food samples that affect the metabolism of homocysteine. For example, tea catechin has been shown to reduce plasma homocysteine by increasing its catabolism in mice [24].
The reduced bioavailability of green tea folate might be related to the chemical structure of folates and the presence of reactive catechins in green tea. Wang et al. [25] reported that green tea catechins inhibited pancreatic phospholipase A2 and intestinal absorption of lipids in ovariectomized rats. Similarly, tea catechins, particularly EGCg, might also inhibit folate conjugase, an enzyme needed to absorb natural folate. We did not clarify the chemical structure of folates within green tea, and it is possible that the folate might be in a highly polyglutamated form that needs to be broken down by conjugase into monoglutamate for uptake from the intestinal tract. In a randomized double-blind controlled study, intake of high-dose tea catechin (1069 mg/day) for 1 week as a capsule with normal diet in volunteers aged 40 - 63 years was associated with a decrease in folate levels and increase in total homocysteine levels in serum [26]. Therefore, inhibition of folate conjugase by tea catechin could be a mechanism of action that explains the reduced supply of natural folate in green tea.
An inhibitory effect of EGCg on dihydrofolate reducetase (DHFR) may be also involved in the reduced bioavailability of green tea folate. In Caco-2 cells, EGCg was shown to inhibit DHFR [10], which reduces folic acid to DHF and THF after absorption in the small intestine [5,12]. In a rat study in which animals were fed 2 mg folic acid with various doses of green tea catechins for 42 days, Augustin et al. [13] reported that the plasma concentration of 5-methyl-tetrahydrofolate was reduced by the intake of green tea catechins (5 g/kg diet), but not when catechin dose was less than at 1 g/kg diet. In our present study, powdered green tea samples contained catechin at 1.73 g/kg diet. Thus, an inhibitory effect of tea catechin on DHFR may be another mechanism by which folate uptake into tissues is reduced during repletion with powdered green tea. In green tea, the content of EGCg is approximately 6 - 13 mg/100 mL [27]. If we consider a higher intake, such as 6 bottles of 500 mL of green tea beverage, this equates to an estimated EGCg intake of 8 mg/kg body weight. In the present study, pure EGCg at a dose of 8 mg/kg body weight did not affect the increase in tissue folate or decrease in plasma homocysteine when repletion was performed with folic acid, suggesting that absorption of folic acid is unaffected by low-dose EGCg. Therefore, folic acid supplementation of bottled green tea beverages may be a practical approach to minimize any negative effect of EGCg on folate status.
Periconceptional use of folic acid supplements is well known to reduce the risk of NTDs in infants [28]. In addition, serum folate levels were inversely related to tea consumption during pregnancy in Japan [11], and daily tea drinking during the periconceptional period was associated with an elevated risk of NTDs in a Chinese population [29]. Some young Japanese women who may become pregnant consume a green tea beverage with a high-strength tea catechin content for weight loss. Hence, infants born to these women may be at risk for NTDs. As shown in the present study, low-dose EGCg did not affect the supplementary effect of folic acid. Thus, it may be necessary to fortify with folic acid beverages containing tea catechin to counteract the negative effect of green tea on folic acid status.
In conclusion, we showed that natural folate in green tea was less bioavailable than that in other food sources, but EGCg at the dose found in green tea did not affect the uptake of folic acid into tissues in a folate depletion/repletion model. Our rat in vivo assay model with a 7-day repletion phase after 4 weeks’ depletion appears suitable to study the different bioavailability of folate in food samples compared with folic acid.
5. Acknowledgements
This study was financially supported in part by a research grant from the Ministry of Health, Labour and Welfare, Japan.
Abbreviations
EGCg: epigallocatechin gallate;
DHFR: dihydrofolate reductase;
DHF: 7,8-dihydrofolate;
THF: 5,6,7,8-tetrahydrofolate;
NTDs: neural tube defects.
NOTES