Abstract
Since the anti-inflammatory, antidiabetic and hypolipidemic effects of soy isoflavones may be mediated by activation of peroxisome proliferator-activated receptors (PPAR), the present study investigated whether the methanolic fractions obtained from soybean seeds (E1) and soybean seed coats with hypocotyls (E2) could influence PPARα, PPARγ and PPARβ/δ transcriptional activity. The isoflavones from E1 and E2 were quantified by HPLC analysis. E1 and E2 were rich in isoflavones (daidzin, glycitin, genistin, malonyldaidzin, malonylglycitin, malonylgenistin, daidzein, glycitein, and genistein). Moreover, E1 and E2 showed no evidence of genetically modified material containing the gene CP4 EPSPS. To investigate PPAR transcriptional activity, human promonocytic U-937 cells were treated with E1 and E2 (200, 400, 800, and 1600 µg/mL), positive controls or vehicle. Data are reported as fold-activation of the luciferase reporter driven by the PPAR-responsive element. Dose-response analysis revealed that E1 and E2 induced the transcriptional activity of PPARα (P < 0.001), with activation comparable to that obtained with 0.1 mM bezafibrate (positive control) at 1600 µg/mL (4-fold) and 800 µg/mL (9-fold), respectively. In addition, dose-response analysis revealed that E1 and E2 activated PPARβ/δ (P < 0.05), and the activation at 800 µg/mL (4- and 9-fold, respectively) was comparable to that of 0.1 mM bezafibrate (positive control). However, no effect on PPARγ was observed. Activation of PPARα is consistent with the lipid-lowering activity of soy isoflavones in vivo, but further studies are needed to determine the physiological significance of PPARβ/δ activation.
Isoflavones; Nuclear receptors; Soybean; PPARα; PPARγ; PPARβ/δ
Braz J Med Biol Res, June 2009, Volume 42(6) 545-550
Effects of a methanolic fraction of soybean seeds on the transcriptional activity of peroxisome proliferator-activated receptors (PPAR)
V.S. Carrara1, A.A. Amato2, F.A.R. Neves2, R.B. Bazotte1, J.M.G. Mandarino3, C.V. Nakamura1, B.P.D. Filho1 and Correspondence and Footnotes D.A.G. Cortez1
1Departamento de Farmácia e Farmacologia, Universidade Estadual de Maringá, Maringá, PR, Brasil
2Departamento de Farmacologia Molecular, Universidade de Brasília, Brasília, DF, Brasil
3Empresa Brasileira de Pesquisa Agropecuária, Londrina, PR, Brasil
References
Correspondence and Footnotes Correspondence and Footnotes Correspondence and Footnotes
Abstract
Since the anti-inflammatory, antidiabetic and hypolipidemic effects of soy isoflavones may be mediated by activation of peroxisome proliferator-activated receptors (PPAR), the present study investigated whether the methanolic fractions obtained from soybean seeds (E1) and soybean seed coats with hypocotyls (E2) could influence PPARα, PPARγ and PPARβ/δ transcriptional activity. The isoflavones from E1 and E2 were quantified by HPLC analysis. E1 and E2 were rich in isoflavones (daidzin, glycitin, genistin, malonyldaidzin, malonylglycitin, malonylgenistin, daidzein, glycitein, and genistein). Moreover, E1 and E2 showed no evidence of genetically modified material containing the gene CP4 EPSPS. To investigate PPAR transcriptional activity, human promonocytic U-937 cells were treated with E1 and E2 (200, 400, 800, and 1600 µg/mL), positive controls or vehicle. Data are reported as fold-activation of the luciferase reporter driven by the PPAR-responsive element. Dose-response analysis revealed that E1 and E2 induced the transcriptional activity of PPARα (P < 0.001), with activation comparable to that obtained with 0.1 mM bezafibrate (positive control) at 1600 µg/mL (4-fold) and 800 µg/mL (9-fold), respectively. In addition, dose-response analysis revealed that E1 and E2 activated PPARβ/δ (P < 0.05), and the activation at 800 µg/mL (4- and 9-fold, respectively) was comparable to that of 0.1 mM bezafibrate (positive control). However, no effect on PPARγ was observed. Activation of PPARα is consistent with the lipid-lowering activity of soy isoflavones in vivo, but further studies are needed to determine the physiological significance of PPARβ/δ activation.
Key words: Isoflavones; Nuclear receptors; Soybean; PPARα; PPARγ; PPARβ/δ
Introduction
Dietary soy has been shown to improve serum lipid levels, glycemic control and atherosclerosis in many animal models of obesity and insulin resistance (1). Clinical studies have also suggested the lipid-lowering effects of soy protein consumption in humans (2). However, the specific components of soy and the mechanisms underlying these beneficial effects are still a matter of controversy and remain to be identified (1).
Dietary soy components include protein, lipids, fiber, and phytochemicals, such as isoflavones, which have been identified as bioactive agents and widely recognized as estrogen receptor agonists or phytoestrogens (3,4). Although this activity has been implicated in the atheroprotective effects of isoflavones, it has been increasingly accepted that these phytochemicals might activate other nuclear receptors regulating lipid metabolism, such as liver x receptor, farsenoid x receptor and peroxisome proliferator-activated receptors (PPARs) (1).
PPARs are members of the nuclear hormone receptor superfamily of ligand-activated transcription factors and regulate the expression of target genes involved in several physiological processes (5). Three receptor subtypes have been identified in mammals, namely PPARα, PPARβ/δ and PPARγ, with overlapping tissue distribution and functions. PPARα is expressed in high levels in the liver, kidney and heart, PPARγ is largely expressed in adipose tissue and PPARβ/δ is ubiquitously expressed (6).
PPARα controls the transcription of many genes involved in the catabolism of lipids, and this explains its hypolipidemic effects (7). Activation of PPARγ increases insulin sensitivity and appears to be a favorable factor in the treatment of insulin resistance associated with type 2 diabetes (8). In contrast to PPARα and PPARγ, the physiological role of PPARβ/δ is not fully known (9). It has been suggested that the anti-inflammatory, antidiabetic and hypolipidemic effects of soy isoflavones may be mediated by activation of PPARα and PPARγ (10-12). However, little is known about the possibility of activation of PPARβ/δ with soy isoflavones. Therefore, in the present study, we investigated whether the methanolic fractions of soybean rich in isoflavones could activate PPARβ/δ.
Material and Methods
Material
Soybean seeds and soybean seed coats with hypocotyl fragments were obtained from the COAMO Company (Brazil). The seed coats were obtained as an industrial residue resulting from oil extraction from the seed. Isoflavone standards were purchased from Sigma (USA) and Fuji Co. (Japan). Human promonocyte U937 cells were obtained from Cells Culture Facility (University of California, USA). RPMI-1640 medium was obtained from Gibco (USA). Lysis buffer and the kit for testing luciferase activity were purchased from Promega (USA). Bezafibrate and troglitazone were purchased from Sigma, and rosiglitazone was purchased from Cayman Chemicals (USA). The expression vectors for PPARα, PPARαβ/δ and PPARαγ and the plasmid containing the luciferase reporter driven by a PPAR-responsive element were kindly provided by J. Magae (Japan). The plasmid construction has been described (13).
Analysis of transgenic soy
Genetically modified herbicide-tolerant soy varieties contain the CP4 EPSPS gene that encodes 5-enol-pyruvylshikimate-3-phosphate synthase from Agrobacterium spp strain CP4. This gene confers resistance to herbicides containing glyphosate. The presence of transgenic soybean was investigated using the Trait Crop and Grain Testing kit from Strategic Diagnostics Inc. (USA), as recommended by the manufacturer. Conventional non-genetically modified soybean seeds and soybean seeds containing the EPSPS gene were used as negative and positive controls, respectively. Transgenic grains were provided by the Monsanto Company (USA). These tests were authorized by the National Technical Commission for Biosafety (Certificate of Quality on Biosafety, CQB #0002/96) and carried out at Embrapa Soybean (Brazil).
Extraction of isoflavones from soybean
One kilogram of frozen soybean seeds (E1) and soybean seed coats with hypocotyl fragments (E2) were triturated and macerated with 12 L hexane for 20 days and filtered. The residues E1 (702 g) and E2 (969 g) were macerated with ethanol:water (3:2 v/v) for seven days and filtered. The solvent from the extracts was evaporated under reduced pressure and the lyophilized extract yielded 160.6 and 194.0 g ethanol extracts E1 and E2, respectively. The ethanol extracts were mixed with 90 mL methanol and centrifuged. The methanol fractions were evaporated to provide 48.0 and 26.7 g of the methanol fraction of E1 and E2, respectively.
High-performance liquid chromatography
Isoflavones from both methanolic fractions (100 mg) were extracted using a 70% water-ethanol solution (w/w) containing 0.1% acetic acid at room temperature. Tubes containing the samples were shaken every 15 min and after 1 h the extracts (1.5 mL) were centrifuged at 14,000 rpm for 15 min at 5°C. The supernatant was then filtered (0.45 µm) and 20 µL of each sample was used for high-performance liquid chromatography (HPLC) analysis.
HPLC analysis of isoflavones was performed on an ODS C18 column (YMC Pack ODS-AM 250 x 0.4 mm ID, 5.0 µm particle size, Japan) in a Waters 2690 HPLC system with an auto sampler and a photodiode array detector (Waters 996, USA). The wavelength was adjusted to 260 nm. A binary gradient solvent system was employed. The mobile phases were: a) acidified methanol (0.025% trifluoroacetic acid, TFA) and b) acidified Milli-Q water (0.025% TFA). The initial composition of the gradient was 20% solvent A system, reaching 100% A after 40 min, and then returning to 20% A at 45 min and maintaining this condition up to 60 min. The flow rate was 1 mL/min, with a column temperature of 25°C. Isoflavones were adequately separated within 60 min. Separated compounds were identified by comparison of retention times and UV spectra with isoflavone standards (glycoside and aglycon forms). Isoflavones were quantified using external standardization method (peak areas), and molar extinction coefficient for malonyl and acetyl forms (14).
Cell culture and transient transfection assays
Human promonocytic U-937 cells were maintained and subcultured in RPMI-1640 medium (Invitrogen®, USA) supplemented with 10% fetal bovine serum, penicillin (50 IU/mL) and streptomycin (50 µg/mL), at 37°C and 5% CO2. For transient transfection assays, cells were collected by centrifugation and resuspended in phosphate-buffered saline (PBS) containing calcium and dextrose (1.5 mL x 107 cells/0.5 mL PBS).
The cells were cotransfected with the expression vectors for PPARα, -β/δ or -γ (1.5 µg) and a PPAR-responsive luciferase reporter vector (DR1-TK-Luc) by electroporation using a gene pulser (Bio-Rad®, USA) at 300 mV and 950 µF. Electroporated cells were then transferred to fresh RPMI-1640 medium and plated onto 12-well dishes (1 mL/well) and treated in triplicate with the methanolic fraction of soybeans containing isoflavones (200, 400, 800, and 1600 µg/mL), bezafibrate (positive control for PPARα and -β/δ transcriptional activity), troglitazone or rosiglitazone (positive control for PPARγ transcriptional activity) or vehicle (ethanol/DMSO, 1:1). After 24 h, cells were collected by centrifugation, lysed by the addition of 150 µL 1X lyses buffer (Promega®, USA) and assayed for luciferase activity using a Luciferase Assay Kit from Promega® and a luminometer (Perkin Elmer®, USA).
Data are reported as fold-activation of the luciferase reporter driven by the PPAR-responsive element calculated as the ratio of luciferase activity obtained in cell samples treated with the different compounds divided by luciferase activity obtained with vehicle. All experiments were performed at least three times in triplicate.
Statistical analysis
The results of the transient transfection assays are reported as means ± SEM. Statistical significance was determined by analysis of variance (ANOVA) followed by the Newman-Keuls multiple comparison test, using the GraphPad Prism software for Windows, version 3.0 (USA). A P value <0.05 was considered to be statistically significant.
Results
Analysis of transgenic soy
Genetically modified soy containing the CP4 EPSPS gene was not detected in any of the samples (data not shown).
Analysis of the methanolic fractions of soybean seeds and soybean seed coats with hypocotyls (HPLC-UV analysis)
The methanolic fractions of soybean seeds (Figure 1A) and soybean seed coats and hypocotyls (Figure 1B) were analyzed for isoflavone composition by HPLC using standard compounds for comparison. The isoflavone composition of both types of soy are given in Table 1. Most of the isoflavones found in the soybean seeds were malonyldaidzin, malonylglycitin and malonylgenistin (Table 1). On the other hand, most of the isoflavones found in the soybean seed coats with hypocotyls were daidzin, glycitin and genistin (Table 1).
Effect of increasing concentrations of a methanolic extract rich in conjugated and non-conjugated soybean isoflavones on PPARα transcriptional activity
Dose-response analysis revealed that the methanolic fraction from soybean seeds and soybean seed coats with hypocotyls induced the transcriptional activity of PPARα, with activation comparable to that obtained with 0.1 mM bezafibrate at 1600 µg/mL (Figure 2A) and 800 µg/mL (Figure 2B), respectively.
Effect of increasing concentrations of a methanolic extract rich in conjugated and non-conjugated soybean isoflavones on PPAR γ transcriptional activity
No activation of PPARγ was detected with any of the concentrations tested of the methanolic fraction from soybean seeds (Figure 3A) or with the methanolic fraction from soybean seed coats with hypocotyls (Figure 3B). The positive controls 10 µM troglitazone and 10 µM rosiglitazone behaved as expected.
Effect of increasing concentrations of a methanolic extract rich in conjugated and non-conjugated soybean isoflavones on PPAR β/δ transcriptional activity
Dose-response analysis revealed that the methanolic fraction from soybean seeds activated PPARβ/δ, and the activation at 800 µg/mL was comparable to that of 0.1 mM bezafibrate (Figure 4A). Similar results were obtained with 800 µg/mL of the methanolic fraction from soybean seed coats with hypocotyls (Figure 4B).
High-performance liquid chromatography (HPLC) profile of the methanolic fractions of soybean seeds (A) and soybean seed coats with hypocotyls (B). Compounds are: 1, daidzin; 2, glycitin; 3, genistin; 4, malonyldaidzin; 5, malonylglycitin; 6, malonylgenistin; 7, daidzein; 8, glycitein; 9, genistein. Chromatographic conditions: column Metasil ODS C18 (250 x 0.4 mm ID, 5.0 µm); linear gradient of methanol [0.025% TFA (solvent A)], water [0.025% TFA (solvent B)], 0-40 min: 20-100% A, at a flow rate of 1.0 mL/min; room temperature; injection 20 µL; detection: 260 nm. The concentration injected for methanolic fractions (A and B) was about 66.6 mg/mL.
Activation of peroxisome proliferator-activated receptor alpha (PPARα) by the methanolic fraction of soybean seeds (Panel A) or soybean seed coats with hypocotyls (Panel B). U-937 cells were cotransfected with the expression vector for PPARα receptor and a luciferase reporter and then treated with vehicle (DMSO/ethanol, 1:1), bezafibrate or increasing amounts of the methanolic fraction of soybean seeds or soybean seed coats for 24 h and assayed for luciferase activity. Data are reported as means ± SEM of fold-activation of PPARα. *P < 0.01 vs vehicle (one-way ANOVA followed by the Newman-Keuls multiple comparison test).
Activation of peroxisome proliferator-activated receptor gamma (PPARγ) by the methanolic fraction of soybean seeds (Panel A) or soybean seed coats with hypocotyls (Panel B). U-937 cells were cotransfected with the expression vector for the PPARγ receptor and a luciferase reporter and then treated with vehicle (DMSO/ethanol, 1:1), glitazone or increasing amounts of the methanolic fraction of soybean seeds or soybean seed coats for 24 h and assayed for luciferase activity. Data are reported as means ± SEM of the fold-activation of PPARγ. *P < 0.01 vs vehicle (one-way ANOVA followed by the Newman-Keuls multiple comparison test).
Activation of peroxisome proliferator-activated receptor b/d (PPARb/d) by the methanolic fraction from soybean seeds (Panel A) or soybean seed coats with hypocotyls (Panel B). U-937 cells were cotransfected with the expression vector for the PPARb/d receptor and a luciferase reporter and then treated with vehicle (DMSO/ethanol, 1:1), bezafibrate or increasing amounts of the methanolic fraction of soybean seeds or soybean seed coats for 24 h and assayed for luciferase activity. Data are reported as means ± SEM of the fold-activation of PPARb/d. *P < 0.05 vs vehicle (one-way ANOVA followed by the Newman-Keuls multiple comparison test).
Isoflavone composition of the methanolic fractions of soybean seeds and seed coats with hypocotyls.
Discussion
The well-established beneficial effects of dietary soy on lipid metabolism and insulin sensitivity have been recently attributed to the activation of PPARα and PPARγ, respectively, by soy isoflavones (1,8,10). However, little is known about the possibility that isoflavones activate PPARβ/δ, which plays a critical role in the regulation of metabolic homeostasis, and also in cardiac lipid metabolism (15,16), fetal development (17), inhibition of human cancer cell line growth (18), protection against liver toxicity (19), modulation of inflammation (6,20), and improved skeletal muscle oxidative enzyme activity in obese patients with type 2 diabetes mellitus (21).
In the present study, a methanolic fraction from soybean seeds and soybean seed coats with hypocotyls rich in conjugated soybean isoflavones was used to address the question of whether these soy fractions can activate PPARβ/δ. For comparative purposes their effect on PPARα and PPARγ was also investigated.
Our results indicated that the methanolic fractions rich in conjugated soybean isoflavones induced PPARα and b/d transcriptional activity. Activation of PPARα has been previously demonstrated in several other studies (10,11,12, 22). Unexpectedly, however, these fractions in the present study did not induce PPARγ transcriptional activity. A possible explanation for this result certainly depends of future studies with isolated isoflavones.
An important result is that the methanolic fractions rich in conjugated and non-conjugated soybean isoflavones used in this study activated PPARβ/δ. To the authors' knowledge, this is the first demonstration that isoflavones activate PPARβ/δ.
The effects of the methanolic fraction of soybean seeds and soybean seed coats with hypocotyls on PPARα and PPARαβ/δ transcriptional activity were similar although their composition in general terms were different. It is possible that the similar effects on both PPAR isoforms could be due to comparable concentrations of the isoflavones genistein and daidzein in the methanolic fractions of seeds and seed coats with hypocotyls. Further studies will indicate which soy isoflavone or mixtures of isoflavones activate PPARα and PPARβ/δ.
Taken together, our results are consistent with animal and clinical studies addressing the potential of isoflavones as lipid-lowering (8,10,11) and anti-inflammatory agents (12), and it can be expected that the methanolic extract from soybean seeds or seed coats with hypocotyls should promote lipid-lowering and anti-inflammatory effects.
Moreover, the observation that the methanolic extract from soybean seeds and from seed coats with hypocotyls activated PPARα and PPARβ/δ but did not induce PPARγ transcriptional activity is important in view of the potential hepatotoxicity of PPARγ agonists. Furthermore, the possibility that the anti-inflammatory effects of soy isoflavones (12) could be mediated by PPARβ/δ receptors (6) must be considered. However, future in vivo studies will be necessary to determine the physiological significance of activation of both PPARα and PPARβ/δ.
Acknowledgments
The authors are grateful to C.E. Oliveira and S.C. Oliveira from State University of Maringá, Maringá, PR, Brazil, for their technical assistance during the experiments.
Address for correspondence: D.A.G. Cortez, Departamento de Farmácia e Farmacologia, Universidade Estadual de Maringá, 87020-900 Maringá, PR, Brasil. Fax: +55-44-3261-4999. E-mail: dagcortez@uem.br
Research supported by CNPq. Received July 19, 2008. Accepted March 25, 2009.
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Publication Dates
-
Publication in this collection
11 May 2009 -
Date of issue
June 2009
History
-
Accepted
25 Mar 2009 -
Received
19 July 2008