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In vivo metabolic tracking of 14C-radiolabelled isoflavones in kudzu (Pueraria lobata) and red clover (Trifolium pratense) extracts

Published online by Cambridge University Press:  09 July 2009

Jonathan G. Mun
Affiliation:
Division of Nutritional Sciences, University of Illinois, Urbana, IL61801, USA
Michael D. Grannan
Affiliation:
Department of Foods and Nutrition, Purdue University, West Lafayette, IN47907, USA
Pamela J. Lachcik
Affiliation:
Department of Foods and Nutrition, Purdue University, West Lafayette, IN47907, USA
Adam Reppert
Affiliation:
Division of Nutritional Sciences, University of Illinois, Urbana, IL61801, USA
Gad G. Yousef
Affiliation:
Department of Natural Resources and Environmental Sciences, University of Illinois, Urbana, IL61801, USA
Randy B. Rogers
Affiliation:
Department of Natural Resources and Environmental Sciences, University of Illinois, Urbana, IL61801, USA
Elsa M. Janle
Affiliation:
Department of Foods and Nutrition, Purdue University, West Lafayette, IN47907, USA
Connie M. Weaver
Affiliation:
Department of Foods and Nutrition, Purdue University, West Lafayette, IN47907, USA
Mary Ann Lila*
Affiliation:
Division of Nutritional Sciences, University of Illinois, Urbana, IL61801, USA Department of Natural Resources and Environmental Sciences, University of Illinois, Urbana, IL61801, USA
*
*Corresponding author: Dr Mary Ann Lila, fax+1 704 250 5409, email [email protected]
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Abstract

Absorption, distribution and elimination of 14C-labelled isoflavone-containing extracts from kudzu (Pueraria lobata) root culture and red clover (Trifolium pratense) cell culture were investigated in an in vivo rat model. The predominant isoflavones in the kudzu extract were the glycosides puerarin, daidzin and malonyl daidzin, while in the red clover extract, the major isoflavones were formononetin and its derivatives, genistein and biochanin A, with radioactivities of 3·770 and 7·256 MBq/g, respectively. Male Sprague–Dawley rats, implanted with a jugular catheter and a subcutaneous ultrafiltrate probe, were orally administered with 14C-labelled isoflavone extracts from either kudzu or clover cell cultures. Serum, interstitial fluid (ISF), urine and faeces were collected using a Culex® Automated Blood Collection System for 24 h. Analysis of bone tissues revealed that radiolabel accumulated in the femur, tibia and vertebrae at 0·04, 0·03 and 0·01 % of the administered dose, respectively, in both kudzu and red clover treatments. The liver accumulated the greatest concentration of radiolabel among the tissues tested, at 1·99 and 1·54 % of the administered kudzu and red clover extracts, respectively. Serum and ISF analysis showed that both extracts were rapidly absorbed, distributed in various tissues, and largely eliminated in the urine and faeces. Urine and faeces contained 8·53 and 9·06 % of the kudzu dose, respectively, and 3·60 and 5·64 % of the red clover dose, respectively. Serum pharmacokinetics suggest that extracts from kudzu may undergo enterohepatic circulation.

Type
Full Papers
Copyright
Copyright © The Authors 2009

Oestrogens are hormones that are involved in the development and maintenance of female physical traits, sexual reproduction(Reference Jacobs and Lewis1), plasma lipid levels and bone mineral density(Reference Genant, Lucas and Weiss2). Isoflavones are a class of plant-derived compounds that bind to oestrogen receptors to yield oestrogenic activity. Kudzu (Pueraria sp.) and red clover (Trifolium pratense) are leguminous species that are rich sources of isoflavones(Reference Kaufman, Duke and Brielmann3, Reference Swinny and Ryan4) and have demonstrated positive effects on bone health in vitro and in vivo. Kudzu-derived puerarin promoted new bone formation in vitro in treated rat osteoblasts(Reference Zhang, Zeng and Zhang5) and in vivo in repair of rabbit parietal bone defects when grafted with puerarin solution mixed with collagen matrix(Reference Wong and Rabie6). Extracts from both Pueraria mirifica and P. lobata have also prevented bone loss in ovariectomised rats(Reference Urasopon, Hamada and Cherdshewasart7) and mice(Reference Wang, Wu and Chiba8), respectively. Red clover isoflavones at a dosage of 57 mg/d have similarly exhibited potential to improve bone mineral density of the proximal radius and ulna by 4·1 % over 6 months in postmenopausal women(Reference Clifton-Bligh, Baber and Fulcher9). A double-blind, randomised, placebo-controlled study of the effects of red clover isoflavones on postmenopausal women, aged 49–65 years, further supported these data, showing that women taking the isoflavone supplement experienced a reduction in bone mineral content loss and bone mineral density loss in the lumbar region of the spine(Reference Atkinson, Compston and Day10).

While our understanding of kudzu and red clover phytochemicals has greatly improved in recent years, little is known about how these dietary constituents are absorbed, distributed, metabolised and excreted in the human body(Reference Grusak11, Reference Grusak, Rogers and Yousef12). This is attributed to the difficulty in examining the phytochemical absorption within a complex diet and discriminating between newly absorbed phytochemicals and previously existing levels in the body(Reference Grusak11, Reference Yousef, Seigler and Grusak13). One approach to studying phytochemical bioavailability, while circumventing these problematic issues, is the use of stable isotope- or radioisotope-labelled compounds(Reference Grusak11), which offers a means of tracking an administered dose of phytochemicals in human subjects or animal models(Reference Grusak, Rogers and Yousef12). A key advantage of using radiolabelled compounds over non-radioactive compounds in such studies is that sensitive detection systems make it possible to administer diet-relevant doses and still be able to track pharmacokinetics and biodistribution(Reference Lila, Yousef and Jiang14).

The present study was conducted to investigate the absorption, distribution and elimination of 14C-labelled isoflavone-containing extracts from kudzu root culture and red clover cell culture in an in vivo rat model.

Materials and methods

Chemicals and reagents

Standards for puerarin, daidzein, genistein, formononetin and biochanin A were purchased from Sigma-Aldrich (St Louis, MO, USA) for isoflavone identification and quantification. Standards for daidzin, genistin and malonyl-genistin were purchased from LC Laboratories (Woburn, MA, USA). Standards for ononin (formononetin 7-O-β-d-glucoside) and sissotrin (biochanin A 7-O-β-d-glucoside) were purchased from Indofine Chemical Company, Inc. (Hillsborough, NJ, USA). Isoflavones that could not be authenticated by standards due to commercial unavailability were instead quantified by a method of molecular-weight adjustment of related standards(Reference Chandra, Rana and Li15).

Plant material

Kudzu (P. lobata) seed was obtained in October 2003 from the Binkley Rd population in Johnston City (Williamson County, IL, USA). This kudzu accession was identified by Terry Esker (Natural Heritage Biologist, Illinois Department of Natural Resources) and a voucher specimen (voucher no. 227615) was deposited in the Illinois Natural History Survey herbarium. Late-flowering red clover (T. pratense ‘Mammoth’) seed was obtained from Johnny's Selected Seeds (Winslow, ME, USA).

Kudzu seeds were surface scarified with a scalpel and agitated in tap water containing two drops of polyoxyethylene sorbitan monolaurate (Tween-20; Sigma-Aldrich, St Louis, MO, USA) per litre for 14 h to overcome seed dormancy and promote germination. Seeds were surface disinfested in 0·9 % sodium hypochlorite for 15–30 min. Seeds were rinsed three times with sterile distilled water and explanted to test-tubes containing 15 ml 1/2 × Murashige and Skoog basal media (2·2 g/l)(Reference Murashige and Skoog16) with rose vitamins(Reference Rogers and Smith17), myoinositol (0·1 g/l; PhytoTechnology Laboratories, Shawnee Mission, KS, USA), sucrose (30 g/l), agar (6 g/l; Sigma-Aldrich, St Louis, MO, USA) and pH adjusted to 5·7.

Following germination, roots were excised and transferred to 250 ml flasks containing 40 ml root culture media, which consisted of Murashige and Skoog basal media (4·3 g/l) with rose vitamins, myoinositol (0·1 g/l), sucrose (30 g/l), 1-naphthaleneacetic acid (1·0 mg/l)(Reference Hakamatsuka, Ebizuka, Sankawa and Bajai18) and pH adjusted to 5·7. Cultures were maintained in the dark on a rotary shaker (150 rpm) at 25°C and subcultured at 21 d intervals by replacing all but 5 ml of the spent medium with 35 ml fresh root culture medium. Root cultures were divided approximately every 9 weeks, after they had accumulated about 25 % new growth.

Red clover seeds were surface disinfested by wrapping in filter paper, submerging in 70 % ethanol for 1 min, and then in a 0·9 % sodium hypochlorite solution with two drops of polyoxyethylene sorbitan monolaurate (Tween-20) per litre for 10 min. Seeds were rinsed five times with sterile water and explanted to 1/2 × Murashige and Skoog basal medium with rose vitamins, myoinositol (0·1 g/l), bacteriological-grade agar (6 g/l) and pH adjusted to 5·7. Petiole segments from 21-d-old seedlings were placed onto 15 ml solid red clover callus-inducing medium(Reference Beach and Smith19), consisting of Gamborg B5 salts (3·08 g/l)(Reference Gamborg, Miller and Ojima20), B5 vitamins, myoinositol (0·1 g/l), sucrose (20 g/l), 2,4-dichlorophenoxyacetic acid (2·25 mg/l), 1-naphthaleneacetic acid (2·0 mg/l), and kinetin (2·12 mg/l; Sigma-Aldrich, St Louis, MO, USA) and bacteriological-grade agar (6 g/l) in culture tubes. After callus cultures had developed, the undifferentiated cells were transferred to 125 ml flasks containing 80 ml callus induction medium, without agar added. Cells maintained as suspension cultures in the dark were transferred to fresh callus media (3 ml settled cell volume in 7 ml spent medium) every 14 d.

Radiolabelling

Uniformly labelled, crystalline [14C]sucrose with a specific activity of 374 MBq/mmol (ICN Biomedicals, Inc., Irvine, CA, USA) was utilised as the label source. A stock solution of [14C]sucrose was prepared in sterile, pH 5·7-adjusted, double-distilled water and filter-sterilised. Concentrated media, at 80 and 90 % of the final volume (32 and 72 ml per 250 ml flask for kudzu and red clover, respectively), containing all constituents except [14C]sucrose, were prepared and autoclaved. Following transfer of established cultures to fresh, concentrated medium as described above, 8 ml stock [14C]sucrose solution were added to kudzu root or red clover cell suspension cultures to bring the final media volumes up to 40 and 80 ml, respectively. The final concentration of [14C]sucrose added was 0·248 and 0·126 MBq/ml medium for kudzu root cultures and red clover cell cultures, respectively. Culture flasks were then placed into an enclosed Plexiglas labelling chamber, designed to siphon and capture respired 14CO2(Reference Grusak, Rogers and Yousef12). Kudzu root cultures were grown in this chamber for 21 d, before being harvested. Red clover cultures were permitted to grow for 11 d, before being removed and treated with 40 μl of a 50 μm-CuCl2 solution, as an elicitor for isoflavone synthesis(Reference Engelmann, Rogers and Vattem21). Red clover cultures were returned to the labelling chamber and were exposed to the CuCl2 elicitor for 3 d, then harvested.

Extraction and chemical analysis of isoflavone extracts

At harvest, root and cell suspension cultures were vacuum filtered using a Buchner funnel with Whatman no. 4 filter paper. Cells and roots were rinsed with distilled, deionised water to wash away residual media and [14C]sucrose that was not taken up. Excess moisture was removed by suction and fresh weight was recorded. Fresh roots or cells were then placed into a blender with 80 % methanol in a 1:5 (w/v) ratio and blended for 2 min. The methanolic extract was separated by filtration with Whatman no. 4 filter paper and stored in a flask at − 20°C. The extraction procedure was repeated twice using the same volume of solvent, with the third extraction held overnight at 4°C, before filtration. The three extractions were combined, filtered with Whatman no. 1 filter paper, concentrated by rotoevaporation (Buchi Rotavapor; Büchi Labortechnik, Flawil, Switzerland) and dried down completely by lyophilisation in a freeze dryer (Labconco Freezone 4.5; Labconco Corp., Kansas City, MO, USA).

Characterisation of isoflavones in extracts

An LCQ Deca XP mass spectrometer (150–1000 mass:charge ratio (m/z)) attached to a photodiode array detector (UV: 262 mm) (Thermo Finnigan Corp., San Jose, CA, USA) was utilised in HPLC–electrospray ionisation–MS analysis on a C18-reversed-phase column (2·1 × 150 mm, VYDAC, catalogue no. 201 SPS215). The mobile phase was composed of 95 % double-distilled water with 5 % acetonitrile and 0·1 % trifluoroacetic acid (solvent A) and 5 % double-distilled water with 95 % acetonitrile and 0·1 % trifluoroacetic acid (solvent B). A step gradient of 0, 70, 100 and 0 % of solvent B was used at 0, 30, 35 and 40 min, respectively. Samples were prepared by dissolving approximately 20 mg dry extract in 4 ml 80 % methanol (5 mg/ml), sonicating and filtering through a 0·45 μm nylon syringe filter (Fisher Scientific, Pittsburgh, PA, USA). A quantity of 5 μl of each sample was injected for analysis at a flow rate of 200 μl/min. Commercial standards were also used in this analysis to verify UV absorption, retention time and molecular weights of isoflavones present in extract.

Surgical protocol

Male Sprague–Dawley rats (body weight 275–350 g), acclimatised to a 12 h photoperiod, were anaesthetised with 3–5 % isofluorane and delivered with O2 at 2–4 litres/min. A jugular catheter was inserted into the right jugular vein and an ultrafiltrate probe (Bioanalytical Systems, Inc., West Lafayette, IN, USA) was implanted subcutaneously down the dorsal midline. Following surgery, the rats were administered 0·3 ml of 10 % buprenex in 0·9 % NaCl (w/v) and connected to a Culex® Automated Blood Sampling System (Bioanalytical Systems, Inc.) for blood, interstitial fluid (ISF), urine and faeces collection. Rats were given 48 h for recovery. Food (AIN93M; Dyets, Inc., Bethlehem, PA, USA) and water were provided ad libitum and the catheter was flushed with 10 units heparin/ml saline (0·9 % NaCl, w/v) every 15 min. All experimental procedures involving animals were approved by the Purdue Animal Care and Use Committee, which adheres to policies set forth by the US Department of Agriculture and the US Public Health Service.

Oral administration protocol

Preliminary experiments demonstrated that a dose of 0·148 MBq of 14C-labelled extract could be traced effectively in vivo using a scintillation counter and were used as a basis for choosing dose sizes for radiolabelled kudzu and red clover extracts. Rats were food-deprived for 8 h before oral administration and 200 μl blood were drawn as the baseline. Approximately 100 mg/kg body weight of 14C-labelled kudzu extract (3·770 MBq/g) or 75 mg/kg body weight of red clover extract (7·256 MBq/g) in 1 ml distilled water were administered to the rats (six rats for kudzu treatment and four rats for the red clover treatments) by oral administration, followed by an immediate rinse of the oral administration needle with 0·5 ml distilled water. The Culex® system (Bioanalytical Systems, Inc.) automatically extracted approximately 200 μl blood at 5, 15, 30, 45, 60, 90, 120, 180, 240, 300, 360, 480, 600, 720 and 1440 min after oral administration and collected ISF at 60 min intervals for a total of 24 h. Urine and faeces were collected for 24 h. Food was returned 240 min after oral administration.

Rat sample collection

Rats were anaesthetised 24 h after oral administration with approximately 0·3 ml ketamine (100 mg/ml) and xylazine (100 mg/ml). Blood was drawn from the jugular catheter until no more blood could be collected. This blood was transferred to heparinised microcentrifuge tubes, centrifuged at 5000 g for 10 min, and plasma was collected for analysis. An incision was made through the left jugular vein and the rat was perfused through the right jugular catheter with 240 ml chilled saline, which was sufficient to produce clear perfusate that exited the incision in the left jugular vein. The stomach, small intestines, large intestines, brain, heart, lungs, liver, kidneys and testes were placed into scintillation vials. The contents of the stomach, small intestines and large intestines were collected by flushing the respective organs through with 10 ml saline (0·9 % NaCl, w/v). Femurs, tibias and vertebrae were carefully removed, wrapped in saline-saturated gauze and placed into scintillation vials. All samples were stored at − 80°C until ready for analysis.

Rat sample analysis

Tissue samples were prepared by macerating with a homogeniser (Bio-homogenizer model M133/1281-0; Biospec Products, Inc., Bautlesville, OK, USA). Tissue homogenates were weighed and transferred to scintillation vials in duplicate. Bones were cleaned, dried at 50°C and ground to a fine powder with a mortar and pestle. Weighed samples of ground bone were placed into scintillation vials in duplicate and dissolved in concentrated nitric acid overnight to achieve uniformity. Faeces were dried in an oven at 50°C, 20 ml of 50 % methanol were added to extract 14C-labelled compounds overnight and the methanolic extract was transferred to scintillation vials. Gastrointestinal contents were prepared by adding 10 ml methanol to each sample and the methanolic extract was transferred to scintillation vials. Serum, plasma, ISF and urine required no additional preparation for analysis.

After all homogenised tissues, dissolved bones, bodily fluids and methanolic extracts of faeces and gastrointestinal contents were placed into scintillation vials in duplicate, 20 ml Ecolite scintillation cocktail (MP Biomedicals, Solon, OH, USA) were added. Samples were allowed to sit overnight in the dark, before analysis with a Beckman LS 6500 scintillation counter (Beckman Coulter, Inc., Fullerton, CA, USA).

ISF was collected at an average rate of 60 μl/h. The ultrafiltrate probe tubing was 48 inches (about 122 cm) in length, with a total internal volume of approximately 12 μl. This internal volume presents a delay between the time ISF is collected and the time ISF reaches the sample collection vial. To account for this delay and to more accurately reflect the amount of 14C label present in the ISF at any given time, the ISF collection time points illustrated in Figs. 1 and 2 were shifted 12 min earlier than actually collected. Total serum and ISF volumes were approximated based on the body weight of each rat(Reference Fernandez, Rettori and Mejia22) and were used to estimate the percentage of 14C-labelled compounds remaining in each respective fluid 24 h after oral administration.

Fig. 1 Representative LC–MS spectra showing total ion current (a), LC–UV chromatogram (UV 262 nm) (b) and MS spectrum (c) of isoflavone extract from kudzu (Pueraria lobata) root cultures. m/z, Mass:charge ratio.

Fig. 2 Representative LC–MS spectra showing total ion current (a), LC–UV chromatogram (UV 262 nm) (b) and MS spectrum (c) of isoflavone extract from red clover (Trifolium pratense) cell cultures. m/z, Mass:charge ratio.

Results and discussion

The predominant isoflavones in the kudzu and red clover extracts were unambiguously identified by HPLC–electrospray ionisation–MS and HPLC photodiode array detector using retention time, molecular weight and comparison with known commercial isoflavone standards. Kudzu isoflavones were confirmed as the glycosides puerarin, daidzin and malonyl daidzin (Fig. 1 and Table 1)(Reference Reppert, Yousef and Rogers23, Reference Prasain, Reppert and Jones24). In the red clover extract, the major isoflavones were formononetin and its derivatives, genistein and biochanin A (Fig. 2 and Table 2)(Reference Engelmann, Reppert and Yousef25). Since [14C]sucrose was used as the radiolabel source, 14C was incorporated into all biosynthesised phytochemicals. The kudzu and red clover extracts had average radioactivities of 3·770 and 7·256 MBq/g, respectively, with standardised isoflavones composing 19·7 and 20·3 % of the total extracts, respectively.

Table 1 Isoflavones in radiolabelled kudzu (Pueraria lobata) root culture extracts detected by LC–MS analysis*

tR, retention time; m/z, mass:charge ratio.

* See Fig. 1 for LC–MS spectra of kudzu root culture extract. The data in Table 1 correspond with Fig. 1.

Table 2 Isoflavones in radiolabelled red clover (Trifolium pratense) cell culture extracts detected by LC–MS analysis*

tR, retention time; m/z, mass:charge ratio.

* See Fig. 2 for LC–MS spectra of red clover cell culture extract. The data in Table 2 correspond with Fig. 2.

Analysis of baseline serum, ISF, urine and faeces by scintillation counter established a naturally occurring, background level of 14C in each animal, which was subtracted from levels measured after oral administration. Serum analysis showed that kudzu and red clover isoflavone extracts were rapidly absorbed, with peak serum concentrations of 14C attained 15–30 min after oral administration, at an average of 0·30 and 0·33 % of the total administered 14C dose per ml serum in kudzu and red clover treatments, respectively (Figs. 3 and 4). Labelled compounds from both extracts were also rapidly distributed, as seen in the extracellular fluid, collected by the ultrafiltrate probe. A second peak in serum concentration approximately 1 h after oral administration of kudzu extract may be attributed to the varied rates of absorption and distribution of different phytochemicals in vivo, such that one compound may already be undergoing distribution into tissues or elimination from the body, while another is still being absorbed. A plateau in serum concentration approximately 4 h (Fig. 3) after oral administration of the kudzu extract is consistent with the kudzu isoflavones puerarin(Reference Prasain, Peng and Moore26), daidzein(Reference Janning, Schuhmacher and Upmeier27) and genistein(Reference Sfakianos, Coward and Kirk28) undergoing enterohepatic circulation, while also being eliminated from the body. Plasma collected 24 h after oral administration showed no difference in 14C activity compared with serum collected 24 h after oral administration. Peak ISF concentrations of 0·15 and 0·23 % of the administered dose per ml were attained 1–2 h after oral administration of kudzu and red clover extracts, respectively (Figs. 3 and 4). Analysis of serum and ISF over the course of 24 h showed that kudzu and red clover phytochemicals were rapidly metabolised and eliminated. Excrement contained the greatest amount of the administered dose at 9·06 and 8·53 % in the urine and faeces, respectively, in the kudzu treatment (Table 3). While this was also true in the red clover treatment, only 4·44 and 3·59 % of the administered red clover dose were accounted for in the urine and faeces (Table 3). Total 14C in all analysed bones, tissues, excrement and bodily fluids did not fully account for the total administered dose and this indicated that 14C label was incorporated into other tissues such as muscle and adipose, and/or metabolism and elimination of labelled compounds in the form of exhaled 14CO2.

Fig. 3 Distribution of 14C label for kudzu (Pueraria lobata) isoflavone extract in serum () and interstitial fluid () of rats during 24 h after administration. Values are means, with standard errors represented by vertical bars.

Fig. 4 Distribution of 14C label for red clover (Trifolium pratense) isoflavone extract in serum () and interstitial fluid () of rats during 24 h after administration. Values are means, with standard errors represented by vertical bars.

Table 3 Analysis of 14C-labelled extract distribution in rats 24 h after oral administration by scintillation counter (percentage of the orally administered dose)

For isoflavones to have an effect on bone health, they must reach the target tissues. 14C-labelled compounds were detected in the bones and tissues 24 h after oral administration. In animals orally administered with either kudzu or red clover extracts, radiolabel accumulated in femurs, tibias and vertebrae, at 0·04, 0·03 and 0·01 % of the administered dose, respectively (Table 3). Successful delivery of 14C-labelled kudzu and red clover extract to the bones supports the in vitro and in vivo studies that have demonstrated increased bone formation(Reference Zhang, Zeng and Zhang5, Reference Wong and Rabie6) and reduced bone loss(Reference Urasopon, Hamada and Cherdshewasart7, Reference Occhiuto, De Pasquale and Guglielmo29) upon treatment with isoflavones.

The liver accumulated the greatest quantity of radiolabel among tissues analysed, at 1·99 and 1·54 % of the total dose for kudzu and red clover treatments, respectively (Table 1). These data are consistent with the fact that compounds which are absorbed by the digestive system are first transported to the liver before reaching the rest of the body, a phenomenon also known as the first-pass effect(Reference Sfakianos, Coward and Kirk28). These observations further support the notion that isoflavones are absorbed from the intestine, travel to the liver via the portal vein, are enzymically conjugated and secreted in the bile, and may be hydrolysed by gut microflora and reabsorbed(Reference Prasain, Jones and Brissie30).

Analysis of gastrointestinal tract contents indicated that only about 0·12 % of the orally administered dose remained in the stomach, 24 h after oral administration. Larger quantities of extract remained in the small and large intestines at 1·33 and 2·66 % of the administered kudzu dose and at 0·51 and 0·99 % of the administered red clover dose, respectively. While radioactivities of the intestinal contents were lower in the small intestines than the large, the small-intestinal tissues contained a greater quantity of radiolabel than the large intestines in both treatments. The other major tissues examined include the lungs, kidneys, heart and testes, which accumulated 0·07, 0·21, 0·04 and 0·19 % of the dose, respectively, in the kudzu treatment and 0·07, 0·16, 0·04 and 0·22 %, respectively, in the red clover treatment (Table 3).

A comparison of the areas under the serum concentration time curves shows that on average, a dose of 100 mg kudzu extract/kg body weight yielded an exposure of 6·69 % of dose × h per ml, while a dose of 75 mg red clover extract/kg body weight yielded an exposure of 4·22 % of dose × h per ml. These values will be used to establish suitable kudzu and red clover extract doses in future pharmacokinetic studies. Future studies will also include analysis for 14C-labelled metabolites to better understand the biochemical mechanisms by which these phytochemicals exert an effect.

Conclusions

Biosynthesised 14C-labelled isoflavones were administered to rats to determine the absorption and distribution in an in vivo model. These radiolabelled compounds were detected in various rat organ tissues. The results of the present metabolic tracking study support the hypothesis that isoflavones may play a role in bone health by demonstrating that radiolabelled kudzu- and red clover-derived extracts were capable of reaching and accumulating in bone tissues.

Acknowledgements

The present study was supported by the National Center for Complementary and Alternative Medicine-sponsored Purdue University – University of Alabama at Birmingham (Purdue-UAB) Botanicals Center for Dietary Supplement Research (National Institutes of Health (NIH) 2 P50 AT000477-06).

J. G. M., M. D. G. and A. R. were students who conducted these experiments; G. G. Y., R. B. R. and P. J. L. were senior research associates who aided in the analysis; E. M. J., C. M. W. and M. A. L. were faculty members who supervised the research and took charge of the outcomes.

There are no conflicts of interest associated with this paper.

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Figure 0

Fig. 1 Representative LC–MS spectra showing total ion current (a), LC–UV chromatogram (UV 262 nm) (b) and MS spectrum (c) of isoflavone extract from kudzu (Pueraria lobata) root cultures. m/z, Mass:charge ratio.

Figure 1

Fig. 2 Representative LC–MS spectra showing total ion current (a), LC–UV chromatogram (UV 262 nm) (b) and MS spectrum (c) of isoflavone extract from red clover (Trifolium pratense) cell cultures. m/z, Mass:charge ratio.

Figure 2

Table 1 Isoflavones in radiolabelled kudzu (Pueraria lobata) root culture extracts detected by LC–MS analysis*

Figure 3

Table 2 Isoflavones in radiolabelled red clover (Trifolium pratense) cell culture extracts detected by LC–MS analysis*

Figure 4

Fig. 3 Distribution of 14C label for kudzu (Pueraria lobata) isoflavone extract in serum () and interstitial fluid () of rats during 24 h after administration. Values are means, with standard errors represented by vertical bars.

Figure 5

Fig. 4 Distribution of 14C label for red clover (Trifolium pratense) isoflavone extract in serum () and interstitial fluid () of rats during 24 h after administration. Values are means, with standard errors represented by vertical bars.

Figure 6

Table 3 Analysis of 14C-labelled extract distribution in rats 24 h after oral administration by scintillation counter (percentage of the orally administered dose)