Susanne
Andres†
*a,
Ulf
Hansen†
a,
Birgit
Niemann
a,
Richard
Palavinskas
b and
Alfonso
Lampen
a
aDepartment of Food Safety, Federal Institute for Risk Assessment, Max-Dohrn-Str. 8-10, 10589 Berlin, Germany. E-mail: Susanne.Andres@bfr.bund.de
bDepartment of Safety in the Food Chain, Federal Institute for Risk Assessment, Max-Dohrn-Str. 8-10, 10589 Berlin, Germany
First published on 29th May 2015
Dietary supplements high in isolated isoflavones are commercially available for human consumption primarily to alleviate menopausal symptoms in women. The isoflavone composition, quantity and importantly their estrogenic potency are poorly standardised and can vary considerably between different products. The aim of this study was to analyse the isoflavone composition of 11 dietary supplements based on soy or red clover using the HPLC/MS/MS technique. Furthermore, we investigated the transactivational potential of the supplements on the estrogen receptors (ER), ERα and ERβ, performing luciferase reporter gene assays. As expected, we found that the isoflavone composition varies between different products. The measured total isoflavone contents in various supplements were mostly comparable to those claimed by the manufacturers in their product information. However expressing the isoflavone content as isoflavone aglycone equivalents, soy-based supplements had a clearly lower quantity compared to the manufacturer information. All supplements transactivated more or less ERα and ERβ with a preference for ERβ. The transactivational efficiency exceeded partly the maximal 17β-estradiol induced ER activation. While the different soy-based supplements revealed similar transactivation potential to both ERs, red clover-based supplements differed considerably. We conclude that different commercial dietary supplements based on soy or red clover vary in their isoflavone composition and quantity. They are estrogenically active, although especially the red clover-based supplements show considerable differences in their estrogenic potential to ERα and ERβ. Thus, different isoflavone-rich products cannot be necessarily compared regarding possible biological effects.
In contrast to Western populations, it is well-known that populations in Asia have a lower risk of developing certain diseases or disorders like cardiovascular diseases, menopausal disorders, osteoporosis or even cancer.9,10 Attention has been focused on their traditionally consumed soy-based nutrition including a high daily isoflavone intake of around 20 to 50 mg as possible biologically-active plant ingredients. Western populations have usually only a daily intake of less than 3 mg isoflavones.11
Numerous experiments and studies suggested possible health effects of isoflavones. Although there is no conclusive evidence for such benefits,12–15 there is great interest in increasing the isoflavone intake in Western populations with the promise of protecting against or mitigating certain diseases or disorders such as menopausal symptoms or osteoporosis. Thus, in particular peri- and postmenopausal women are the special target group for isoflavone-rich dietary supplements. In fact, consumers are overflowed with such over the counter supplements.
Available products contain mostly 40 to 50 mg isoflavones per tablet; occasionally, they have a higher isoflavone content of up to 100 or even 200 mg (cited by Mortensen et al.16). The real content of isoflavone-rich supplements is often not consistent with the isoflavone amount that is claimed by the manufacturers.17–21 Thus, the aim of our study was to determine the isoflavone composition of 11 soy- or red clover-based dietary supplements, available on the German market.
Besides the assumption of numerous beneficial health effects, research on isolated isoflavones also revealed potential adverse effects for instance on the reproductive system or even regarding possible tumour-promoting effects on estrogen-sensitive tissues such as the breast. Therefore, the safety of a long-term intake of isolated isoflavones at high doses has still to be elucidated especially for postmenopausal women.12,22–24
In particular, there are concerns due to the weakly estrogenic potential of isoflavones acting among others via the two estrogen receptors (ER), ER-α and ER-β. Activation of ER-α is associated with cell proliferation and with carcinogenicity in estrogen-sensitive tissues, while ER-β has a particular role in suppressing estrogenic signal mechanisms stimulated by ER-α. ER-β negatively regulates cellular proliferation and plays a protective role in normal breast tissue (reviewed by Andres et al.23). Based on in vitro and xenograft animal studies, it is hypothesized that isoflavones may promote primarily ER-mediated cell proliferation of estrogen-sensitive human cells at concentrations that are also present in the human plasma.23,25,26 However, isoflavones at low concentrations (≤1 μM) induce only cell proliferation in cell lines with a predominance for ER-α, while in cell lines expressing mainly ER-β the cell growth is reduced by isoflavone incubation.27,28 The second aim of the present study was to determine the estrogenic activities of the 11 investigated isoflavone-rich supplements.
For isoflavone analysis, the capsule content (around 300 to 500 mg) was weighed and dissolved in 100 mL of 70% methanol resulting in isoflavone extraction as described by others.7,19 Four capsules of each supplement were analytically examined regarding their isoflavone composition. For the reporter gene assays, 10 capsules of each supplement were diluted in 25 mL of 70% methanol. Solutions were sonicated for 10 min and filtered several times through a filter with a pore size of 450 nm (Carl Roth GmbH, Germany). The filtered solution was used for the isoflavone analysis as well as for the cell culture.
For analysis, a standard solution was prepared by dissolving the isoflavone standards in 70% methanol obtaining a stock solution with concentrations between 0.2 and 1.3 mM. Subsequently, this solution was diluted 1 to 10 times obtaining the standard solution with the following isoflavone concentrations: 89.6 μM genistein, 88.9 μM daidzein, 23.2 μM glycitein, 21.0 μM daidzin, 34.8 μM glycitin, 127.0 μM biochanin A, 92.4 μM formononetin and 72.9 μM prunetin. Due to supply bottleneck of genistin, a separate genistin standard solution (60.1 μM) was used for quantitative determination. Prior to the HPLC application, samples of the isoflavone supplements were further diluted 1:500 in 70% methanol and the standard solution 1:200. All solutions were stored at 7 °C.
Isoflavones | HPLC retention time (min) | Ion mass (Da) | Collision energy (eV) |
---|---|---|---|
a Main ion. | |||
Genistein | 3.19 | 270.99a | |
91.0 | 51 | ||
153.0 | 39 | ||
65.0 | 69 | ||
Genistin | 1.96 | 433.08a | |
271.1 | 25 | ||
91.1 | 83 | ||
153.2 | 69 | ||
Daidzein | 2.7 | 254.96a | |
91.1 | 51 | ||
65.1 | 73 | ||
137.2 | 31 | ||
Daidzin | 1.9 | 417.01a | |
255.0 | 23 | ||
91.1 | 87 | ||
199.1 | 57 | ||
Glycitein | 6.19 | 285.02a | |
270.1 | 35 | ||
242.1 | 43 | ||
118.0 | 57 | ||
Glycitin | 1.84 | 446.99a | |
285.0 | 27 | ||
270.1 | 53 | ||
242.2 | 67 | ||
Biochanin A | 6.17 | 285.01a | |
152.0 | 37 | ||
213.0 | 49 | ||
89.0 | 83 | ||
Formononetin | 4.37 | 269.09a | |
197.2 | 51 | ||
89.0 | 81 | ||
90.0 | 67 | ||
Prunetin | 5.64 | 285.01a | |
91.0 | 53 | ||
167.0 | 39 | ||
242.1 | 43 |
The isoflavones were separated according to their molecular mass with a tandem mass spectrometer. MS separation was carried out with an AB Sciex API 2000 Triple-Quadrupol mass spectrometer (AB Sciex, Germany) using the MRM (Multiple Reaction Monitoring) modus. For the positive ionization, an ion spray voltage of 6000 V was used. Fragmentation was induced by CID (collision induced dissociation) with nitrogen as collision gas. The detection was carried out with a channel electron multiplier. Table 1 shows the masses of the main ions and their fragmentation products and the corresponding collision energies of the fragmentation products. The structural fragmentation and a representative chromatogram of daidzein are shown in Fig. 2. For the quantitative determination of the isoflavone content, calibration curves were plotted with each isoflavone standard. For the calibration curves, standard solutions were diluted from 1:20 to 1:400. The isoflavone quantity was calculated from the peak areas in the chromatogram of the supplements and the corresponding isoflavone calibration curve. The isoflavone content was expressed as the mean.
The accuracy of the system was tested using standard additions. Here, we prepared different solutions with specific concentrations of supplement S1 and the standard solution. The measured concentration was in accordance with 95% of the expected value.
Cells were cultured in Dulbecco's Modified Eagle Medium (DMEM) with 4 mM L-glutamine, 1% penicillin/streptomycin solution, 1% non-essential amino acids and 10% foetal calf serum in a humidified incubator at 37 °C and 5% CO2. For the cell viability/luciferase reporter gene assay, cells were seeded in 96-well plates (Greiner bio-one, Germany) at a density of 20000 cells per well and allowed to attach for 48 h. For dilutions of the test substances and the performance of the luciferase reporter gene assay, foetal calf serum was replaced in the medium with charcoal-stripped foetal calf serum (7.5%). After medium replacement, the application of the test substances to the cells was carried out for 48 h. The final solvent concentration (70% methanol) in the culture medium was lower than 0.01%. Subsequently, cell viability was determined using the CTB test (cell titer-blue, PAA Laboratories). Twenty μL CTB reagents were added to each well. After 2 h, fluorescence was measured at 590 nm with a Mithras LD 940 microplate reader (Berthold, Germany).
After medium removal, cells were lysed with 75 μL lyses buffer containing 0.1 M TrisAcetate, 2 mM ethylene diamine tetraacetic acid, 1% Triton X-100 (pH 7.5), frozen overnight at −20 °C and thawed at room temperature on a plate shaker. Fifty μl lysate were transferred in a white 96-well plate (Greiner bio-one). The samples were mixed automatically with 50 μL luciferin-containing buffer (20 mM) and 150 μl assay buffer (25 mM glycylglycine, 15 mM MgSO4, 4 mM ethylene glycol tetraacetic acid, 1 mM dithiothreitol, 1 mM ATP, pH 7.8). Luminescence (luciferase activity) was measured with a Mithras LB 940 microplate luminometer (Berthold). Results were calculated in relation to the maximum ER activation induced by E2 at concentrations of 10−10 to 2 × 10−9 M which were set as 100%. Sigmoidal dose–response curves were fitted with SigmaPlot software. All tests were performed as fourfold determination. Estrogenic activity was expressed as mean ± SE.
Supplement | Genistein | Daidzein | Glycitein | Genistin | Daidzin | Glycitin | Formononetin | Biochanin A | Prunetin | Sum (SD) | Expecteda |
---|---|---|---|---|---|---|---|---|---|---|---|
a According to manufacturer's information. | |||||||||||
S1 | 2.50 | 2.40 | 0 | 9.83 | 16.27 | 0.86 | 0.01 | 0 | 0 | 31.9 (2.0) | 50 |
S2 | 0.11 | 0.94 | 0 | 4.04 | 25.44 | 5.70 | 0.05 | 0 | 0 | 36.3 (2.6) | 35 |
S3 | 3.45 | 2.51 | 0.07 | 17.86 | 29.99 | 1.88 | 0.04 | 0 | 0 | 55.8 (6.9) | 60 |
S4 | 3.79 | 4.41 | 0 | 18.03 | 17.91 | 1.49 | 0.50 | 0 | 0 | 46.1 (4.2) | 50 |
S5 | 1.74 | 1.70 | 0 | 21.79 | 26.35 | 1.38 | 0.17 | 0 | 0 | 53.1 (1.5) | 50 |
S6 | 2.26 | 2.89 | 0 | 28.10 | 19.08 | 1.22 | 0.05 | 0 | 0 | 53.6 (4.0) | 50 |
S7 | 0.76 | 0.20 | 2.91 | 0 | 0.03 | 0 | 21.12 | 9.65 | 0.20 | 34.9 (0.7) | 40 |
S8 | 1.78 | 2.02 | 0.70 | 0.81 | 0.35 | 1.67 | 36.64 | 4.22 | 0 | 48.2 (5.7) | 50 |
S9 | 0.49 | 0.58 | 2.61 | 0.57 | 0.26 | 1.46 | 31.85 | 9.24 | 0 | 47.1 (3.0) | 50 |
S10 | 0.93 | 0.66 | 3.74 | 0.42 | 0.45 | 1.42 | 27.94 | 13.61 | 0.86 | 50.2 (3.9) | 50 |
S11 | 0.84 | 0.28 | 10.68 | 0 | 0.13 | 1.37 | 29.19 | 35.64 | 1.15 | 79.3 (17.2) | 80 |
The isoflavone composition of the dietary supplements is shown in Table 2. Capsules had a real isoflavone content of around 32 to 80 mg per capsule. The total isoflavone contents varied up to 22% between the 4 examined capsules per product. Soy-based supplements (S1–S6) contained primarily the glycosides genistin and daidzin as well as at lower amounts glycitin and the aglycones genistein and daidzein. Glycitein was only found in small amounts in S3 (0.07 mg per capsule). The soy-based products also contained the red clover isoflavone formononetin, but only in small amounts (≤0.5 mg per capsule). The typical red clover isoflavones, biochanin A and prunetin, were not found in the dietary supplements derived from soy.
Red clover-based products (S7–S11) contained, as expected, high amounts of formononetin and biochanin A, but also lower amounts of the other seven analysed isoflavone aglycones and glycosides. However, these seven isoflavones were not always present in the red clover-based supplements. For instance, supplement S7 did not contain genistin and glycitin, while the products S8 and S9 did not contain prunetin (Table 2).
The measured isoflavone content of all dietary supplements (with the exception of S1) was in good accordance with the isoflavone amount that was claimed by the manufacturer. The determined total isoflavone contents of the supplements correspond to 87 to 107% of the isoflavone contents that were given in the package inserts. The supplement S1 contained more than one third less isoflavones than the given manufacturer information (Fig. 3). According to the manufacturer information, the soy based supplements S1 as well as S4 to S6 should have a genistein/genistin content of 30 mg per capsule. The greatest deviation from the real genistein/genistin content was in S1 with an almost 20 mg lower amount per capsule (Table 2).
However, sugar residues of isoflavone glycosides account for about 40% of the molecular weight. Because of this it is more advisable to convert the isoflavone content to isoflavone aglycone equivalents (IAE).30 The calculated IAE values of the isoflavone-rich supplements are depicted in Fig. 3. Due to the high amount of isoflavone glycosides in the soy-based supplements, the IAE values were clearly lower than the total isoflavone amount and comprised only around 61 to 70% of the labelled isoflavone content (exception S1 with only around 43%). Only the manufacturer of S2 gave the IAE value of 21.5 mg with 10.85 mg daidzein per capsule, while we calculated an IAE value of around 22.8 mg with 16.5 mg daidzein per capsule. The IAE values of red clover-based supplements were only marginally lower than the whole isoflavone amount due to their low content of isoflavone glycosides (Fig. 3).
The transactivation potential for both ERs of soy-based supplements was similar in spite of the different isoflavone compositions. For ERα, the dietary supplements based on soy showed a likewise or higher transactivational efficiency compared to E2 (98–177% S1–S6 vs. 100% E2), while for ERβ all supplements exceeded clearly the maximal E2-induced receptor activation (142–211% S1–S6 vs. 100% E2). The soy-based supplements showed either an equal transactivational efficiency to both receptors or a higher efficiency to ERβ (Fig. 4 and Table 3).
Supplement | Efficiencya (%) | EC50b,c (M) | n (μmol isoflavones per capsule) | EEQd (nmol E2 per capsule) | EEQ (μg E2 per capsule) | ||||
---|---|---|---|---|---|---|---|---|---|
ERα | ERβ | ERα | ERβ | ERα | ERβ | ERα | ERβ | ||
a Transcriptional efficiency of S1 to S11 at 10−6 M compared to E2 (= 100%). b Soy (S1–S6): E2: ERα EC50 = 1.5 × 10−11 M; ERβ EC50 = 5.0 × 10−11 M. c Red clover (S7–S11): E2: ERα EC50 = 1.3 × 10−11 M; ERβ EC50 = 2.5 × 10−11 M. d . e n.d. = not determinable. | |||||||||
S1 | 108 | 211 | 2.5 × 10−7 | n.d.e | 82.5 | 5.2 | 1.4 | ||
S2 | 140 | 142 | n.d. | 1.3 × 10−7 | 87.5 | 34.8 | 9.5 | ||
S3 | 154 | 166 | 7.9 × 10−8 | 7.9 × 10−8 | 140.6 | 28.5 | 88.7 | 7.6 | 24.2 |
S4 | 177 | 181 | 1.0 × 10−7 | n.d. | 121.3 | 19.2 | 5.2 | ||
S5 | 129 | 163 | n.d. | 7.9 × 10−8 | 130.5 | 82.4 | 22.4 | ||
S6 | 98 | 177 | n.d. | 5.0 × 10−8 | 133.5 | 133.5 | 36.4 | ||
S7 | 26 | 148 | n.d. | 6.3 × 10−8 | 127.3 | 50.7 | 13.8 | ||
S8 | 33 | 131 | n.d. | n.d. | 174.9 | ||||
S9 | 73 | 51 | 5.0 × 10−8 | n.d. | 169.7 | 42.6 | 11.6 | ||
S10 | 245 | 186 | n.d. | 7.9 × 10−8 | 179.5 | 56.8 | 15.5 | ||
S11 | 298 | 298 | n.d. | n.d. | 283.4 |
In contrast to the supplements derived from soy, the red clover-based products differed considerably in their transactivational potential to ERα and ERβ. Only the preparations S10 and S11 clearly exceeded the maximum E2-induced ERα activation by a factor of about 2.5 and 3, respectively, while the other red clover supplements also transactivated ERα but to a minor or moderate extent (efficiencies 26–73% S7–S9 vs. 100% E2). For ERβ with the exception of S9 (efficiency 51%), all red clover supplements exceeded the maximal E2-mediated ERβ activation (efficiencies 131–298% S7/8/10/11 vs. 100% E2). Some red clover-based supplements showed a better activation of ERα, others showed activation of ERβ and again some others showed a similar activation of both ERs (Fig. 5 and Table 3).
For the determination of the potency for ER activation, we calculated the half maximal effective concentration (EC50). However, we could not calculate EC50 values for all dietary supplements, because the maximum activation was not achieved in each case. Comparing the EC50 values of E2 (shown in Table 3) with those of the supplements, we could evaluate that the potency of the isoflavone-rich supplements was around 4000 to 16000-fold less for ERα and 1 000 to 3000-fold less for ERβ.
The calculated estradiol equivalents (EEQ, calculation shown in Table 3) of the isoflavone-rich preparations, based on EC50 values of E2 and the supplements, ranged from 1.4 to 11.6 μg E2 per capsule for ERα and 9.5 to 36.4 μg E2 per capsule for ERβ. However only for the supplement S3, we could calculate EEQ values for both ER receptors with 7.6 μg E2 per capsule for ERα and 24.2 μg E2 for ERβ (Table 3).
In our study, the investigated isoflavone-rich supplements should contain 35 to 80 mg isoflavones per capsule. In contrast to numerous studies, the overall isoflavone contents from 9 of 11 of our test supplements were comparable to the manufacturer information (more than 90% total isoflavones of the claimed isoflavone content). Similar results were obtained by Romani et al.33 In a red clover-based supplement (S7) and a soy-based supplement (S1), we found an isoflavone content of 87% and 66%, respectively, compared to the manufacturer information. The isoflavone content between different capsules of one product deviated up to 22%. The supplements S1 and S4 to S6 have additional manufacturer information regarding the genistein/genistin content of 30 mg per capsule. The greatest deviation from the mentioned genistein/genistin content was in S1 with only 11 mg.
These specifications refer to the total isoflavone content. It is well known that soy-based supplements contain primarily isoflavone glycosides.17 The sugar moiety of the isoflavone glycosides accounts for almost 40% of the molecular weight. Manufacturers should state the isoflavone content as IAE values reflecting the biological potency of their products for better consumer awareness and also for regulatory purposes.30 IAE values of the analysed soy-based supplements were only around 40 to 70% of the labelled isoflavone content. Only the manufacturer of S2 specified the IAE value of 21.5 mg with 10.85 mg daidzein per capsule. This correlated quite well with our calculated IAE value of around 22.8 mg (16.5 mg daidzein) per capsule. As already described previously, the majority of red clover isoflavones are aglycones,7 because of that the IAE values of red clover-based supplements differed only marginally from the total isoflavone content.
Most soy-derived products contain a higher amount of genistein/genistin than daidzein/daidzin,4,17,33 but 4 of 6 investigated soy-based supplements contained higher amounts of daidzin than genistin. Interestingly, all the analysed soy-based products showed also small amounts of the typical red clover isoflavone, formononetin (≤0.5 mg per capsule). As described previously, red clover-based supplements contained predominantly formononetin and biochanin A but also more or less the other seven scrutinised isoflavones.6–8
Isoflavones are able to bind weakly to and transactivate ERα or ERβ receptors showing a higher affinity to ER-β.1 However, the binding and transactivation capacities differ between the various isoflavones. Genistein revealed the highest relative binding affinity followed by daidzein. Both isoflavones show good transactivational efficiencies to ERα and ERβ (72–85%) compared to E2 (100%).31 The data about red clover isoflavones and their binding capacity to ER are not conclusive. Pfitscher et al. revealed low binding capacities of formononetin and biochanin A,34 while Kuiper et al. found no binding affinity of biochanin A and formononetin.2 However, genistein, daidzein, biochanin A and formononetin transactivated ERα and ERβ in a yeast transactivation system with great variations of the potency and efficiency in ER activation. The transactivational efficiency varied for ERα between only 14% for daidzein and 107% for genistein (E2 = 100%) and for ERβ between 77% for formononetin and 129% for daidzein (E2 = 100%).5 Morito et al. revealed that the isoflavone glycosides genistin, daidzin and glycitin bind to and transactivate only poorly both ERs compared to their corresponding aglycones.35 However, human kidney tissues express β-glycosidases, which are able to cleave the sugar residues of isoflavone glycosides.36,37 Therefore, the human kidney HEK293 cell line, used in this study, may cleave the isoflavone glycosides to the probably more biologically active isoflavone aglycones.
The calculated potencies of our investigated isoflavone-rich supplements (several 1000-fold lower compared to E2) are in a similar range of the potencies of the single isoflavones genistein, daidzein, formononetin and biochanin as described previously.5 We found similar to earlier studies that the investigated isoflavone-rich supplements have a higher potency for ERβ than for ERα.1,5 However, the transactivational efficiencies of some of our soy- or red clover-based products exceeded clearly the maximum E2-mediated ERα or ERβ activation (e.g. up to a factor of 3 for S11), while previous studies found only a maximum transcriptional efficiency of around 130% with isolated isoflavones (E2 = 100%).5 Although there are differences in the isoflavone composition of the analysed soy-based supplements, the estrogenic activities of both receptors were surprisingly similar, especially for ERβ. In contrast, red clover-based supplements showed considerable differences in their ER activations. Supplement S11 revealed the highest ER activation for both receptors, while other supplements derived from red clover showed only minor or moderate activation potential. Besides formononetin and biochanin A, the supplement S11 contained also a relatively high amount of glycitein compared to the other red clover-based supplements. However, whether glycitein caused the high activation potential could not be clarified in our study. It is known that isoflavone-rich supplements can also contain other unknown compounds or impurities,17,19 which may also have an impact on ER activation.
Based on the EC50 values for ERα and ERβ activation, we calculated EEQ values ranging from 1.4 to 11.6 μg E2 per capsule for ERα and from 9.5 to 36.4 μg E2 per capsule for ERβ. Similarly, Dornstauder et al. specified the transactivation capacity of a red clover extract corresponding to around 18 μg E2 per g red clover extract for ERα and 78 μg for ERβ.5 Behr et al. analysed the estrogenic activity in foodstuff and found the highest activities with up to 1.5 μg EEQ per kg in the traditional soy food tofu.38 For a better comparison, depending on the route of application an estradiol dose of 0.025 to 3 mg per day can be applied during hormone therapy.39
Besides the assumption of numerous beneficial effects on health, concerns have arisen regarding possible adverse effects e.g. on tumour promotion of estrogen-sensitive tissues like the breast. Clear estrogenic potential of such dietary supplements could be verified in this study. The safety of a long-term intake of isolated isoflavones especially in high doses has still to be elucidated.12,24 For risk evaluation, the variance of the isoflavone composition and of the estrogenic potential between different isoflavone-rich supplements should be considered.
CTB | Cell titer-blue |
E2 | 17β-Estradiol |
EC50 | Half maximal effective concentration |
EEQ | Estradiol equivalent concentration |
ER | Estrogen receptor |
HEK293 | Human embryonic kidney 293 cells |
HPLC | High performance liquid chromatography |
IAE | Isoflavone aglycone equivalents |
MS/MS | Tandem mass spectrometry |
Footnote |
† These authors contributed equally to this work. |
This journal is © The Royal Society of Chemistry 2015 |