Population

Healthy children between the ages of 3 to 12 years, as well as 17 year olds, and some of their parents were recruited for the present study through cooperation with a local Waldorf school. A total of nineteen adults (sixteen female and three male) and twenty children (twelve female and eight male) completed the study protocol correctly and were included in the analysis (Table 1). Three of the original forty recruited participants were eliminated from the study; two gave an incomplete urine collection and the other had high UIER (>1 nmol/h per kg) at baseline due to soya consumption before starting the study. No participants reported any adverse reactions to soya. Overnight urine (ONU) was collected for 12·13 (sd 0·81) h (Table 1). Subjects were excluded if they had been on antibiotics less than 25 d before participating in the study. Other exclusion criteria were wearing diapers at night, the inability to collect urine for a 12 h overnight period, kidney disease, digestive problems, and an allergy or intolerance to soya. The Waldorf school participants were accustomed to eating soya products, and thus we asked them to avoid, or at least reduce, the consumption of soya on the study day, but only excluded those participants who had a high UIER (>1 nmol/h per kg) at baseline.

Table 1 Participant characteristics

The University of Hawaii Committee on Human Studies approved the study protocol and all consent and assent forms. All parents signed a consent form for themselves when participating and in addition one for their children; participating children 7 years of age and above provided their own additional assent separately.

Study procedures

The participants first learned about the study through word of mouth, then Waldorf school teachers gave them basic information about the study. If the student and/or family were interested, the study staff followed up with details of the study and methods for collecting urine during a visit or phone call to the parents before commencing the study. All participants had to be able to consume soya nuts and to collect an ONU sample. Forty participants received soya nuts in amounts adjusted to their BW (15 g/54·4 kg), supplies for their urine collection, including urine containers with small amounts of boric and ascorbic acid as preservativesReference Franke and Custer²⁹, a worksheet, and a background information questionnaire to complete. Participants were instructed to start the study in the evening by emptying their bladder at approximately 18.00 hours in a container provided to them (baseline urine; BLU) and to consume the soya nuts immediately thereafter. They were asked to collect all following urine voids in large containers until they got up the next morning (ONU). They were also instructed to chill the urine in the coolers provided and to avoid, as much as possible, all other soya products including supplements with soya or IFL from the time they woke up on the study day until the next day. The urine was transported on ice or cool packs to our laboratory where all ONU was mixed and weighed as surrogate for volume determination. Samples of 2 ml BLU and ONU were stored at − 20°C.

On the worksheets, participants recorded their BW and all food consumed the day of the first urine collection, including before and after having eaten the study soya food. They also recorded the time the soya food was consumed (just a few min after providing the spot urine) and the time of the final urine collection in the morning, typically between 05.00 and 07.00 hours. In addition, they reported their current age and ethnicity.

Soya foods used in the study were lightly salted and roasted soya nuts (Revival brand; Physicians Pharmaceuticals, Inc., Kernersville, NC, USA). The IFL composition and content of the nuts was determined by us using HPLC with photodiode array detection without hydrolysis; flavone was used as an internal standard. This method has been validated in a comparison with liquid chromatography-MS-based assaysReference Franke, Hankin, Yu, Maskarinec, Low and Custer³². We checked variations in IFL content caused by crop, manufacturing or other factorsReference Tsukamoto, Shimada, Igita, Kudou, Kokubun, Okubo and Kitamura³³ by measuring IFL in each batch received, which resulted in between-batch CV of less than 6 % for total IFL (DE+GE+GLYE+dihydrodaidzein+dihydrogenistein+equol+DMA; Table 2).

Table 2 Isoflavone dose* per 50 kg body weight (BW) in aglycone equivalents†(Mean values and standard deviations)

ND, not detected.

* 0·615 (sd 0·036) mg total isoflavones/kg BW equivalent to 0·28 g soya nuts/kg BW or 15 g/120 lbs BW.

† All values obtained by HPLC–photodiode array analysis.

The soya nut serving sizes were controlled for BW to provide an IFL dose of 15 g soya nuts/54·4 kg (120 lbs) which led to a consistent total IFL dose of 0·615 (sd 0·036) mg total IFL/kg BW (mg/kg; Table 2). When the first batch of soya nuts was finished, we started a new batch with IFL composition being very similar (Table 2). Every participant from within each respective age group and from within every family received nuts from the same batch. Thirteen children and thirteen adults ate from the first batch of nuts; six children and five adults ate from the second batch of nuts.

Urinary isoflavonoid analysis

DE, GE, GLYE, equol, dihydrodaidzein, dihydrogenistein and DMA were analysed from urine by HPLC with detection by electrospray ionisation (negative mode) tandem mass spectrometry (ESI-MS)Reference Blair, Appt, Franke and Clarkson^34, Reference Franke, Custer, Wilkens, Le Marchand, Nomura, Goodman and Kolonel³⁵. In brief, triply ¹³C-labelled internal standards of DE, GE, equol and DMA (University of St Andrews, Fife, UK) were added to each specimen hydrolysed with glucuronidase and sulfatase (Roche Applied Sciences, Indianapolis, IN, USA) followed by repeated phase separation with diethyl etherReference Franke, Custer, Wang and Shi¹⁵. The combined ether fractions were dried under N₂ and redissolved in a 1:1 mixture of acetonitrile–sodium acetate buffer (0·2 m; pH 5). A sample (5–20 μl) of this extract was analysed by LC/ES-MS with a Surveyor TSQ Quantum Ultra triple quadrupole system (ThermoElectron Corp., San Jose, CA, USA) equipped with a Gemini C18 reversed phase column (150 × 2·0 mm; 5 μm) coupled to a Gemini C18 (4·0 × 2.0 mm; 5 μm) direct-connect guard column (Phenomenex, Torrance, CA, USA). The elution, absorbance detection and mass spectrometric measurements were performed as applied previouslyReference Franke, Custer, Wilkens, Le Marchand, Nomura, Goodman and Kolonel^35–Reference Adams, Golden, Franke, Potter, Smith and Anthony³⁷. Limits of quantification for all analytes using 1·8 ml urine were 2·5 nm except for dihydrodaidzein and dihydrogenistein (1·5nm) and DMA (5·0 nm). Between-day CV ranged 4–12 % (DE), 5–18 % (GE) and 3–14 % (GLYE).

Urinary creatinine was determined from BLU and ONU with a Roche-Cobas MiraPlus clinical autoanalyser using a kit from Randox Laboratories (Crumlin, Co. Antrim, UK) that is based on a kinetic modification of the Jaffé reaction.

Calculation of hourly urinary isoflavone excretion rate

As previously reported by the present authorsReference Franke, Halm, Custer, Tatsumura and Hebshi³⁸, UIER expressed relative to time (h) is more accurate than expressed relative to creatinine, because in healthy individuals the latter depends mostly on muscle mass, and consequently, largely on BW, sex and ageReference Fomon^39, Reference Remer, Neubert and Maser-Gluth⁴⁰. This is particularly relevant in growing children, not only due to marked changes of muscle mass in absolute terms but also after adjustment for BWReference Remer, Neubert and Maser-Gluth^40–Reference Kampmann, Siersbaek-Nielsen, Kristensen and Hansen⁴³. The amount of IFL at baseline present in the ONU collection, although small in all samples, was subtracted from the IFL amount in the ONU sample in order to adjust for background IFL in the ONU sample. Since the time of previous void of BLU was unknown its expression in hourly units was not readily available. Hourly units could, however, be calculated by multiplying the creatinine/h value as available from ONU with the known nmol/creatinine value of BLU separately for each subject. This seemed adequate due to the relatively constant creatinine excretion of healthy individualsReference Remer, Neubert and Maser-Gluth^40, Reference Kampmann, Siersbaek-Nielsen, Kristensen and Hansen⁴³. The ONU concentration determined by liquid chromatography–MS (nmol/ml) was multiplied by the weight of the ONU (g) to arrive at absolute amounts (nmol) in the collected urine specimen. This assumed that 1 ml urine weighs approximately 1 g. Although the density of urine is known to be slightly higher than 1, this inaccuracy seems acceptable considering the relatively larger measurement errors connected with urinary volume determinations, and also considering that urine collections per se bear inherent inaccuracies. The absolute amount calculated (nmol) was divided by 12 (for the 12 h of collection) to obtain the hourly excretion rate (nmol/h). This was adjusted if ONU collections deviated from the 12 h urinary collection period (see later). The amount of IFL at baseline contributing to the amount measured in the ONU samples was calculated by applying the known elimination half time of IFL (average T_1/2 8 hReference Setchell, Brown, Desai, Zimmer-Nechimias, Wolfe, Jakate, Creutzinger and Heubi¹⁷, and using the trapezoid method to calculate area under the curve values in order to arrive at absolute amounts (i.e. mg present in the 12 h period)Reference Franke, Custer and Hundahl¹⁶. This value was then subtracted from the measured amount of IFL in the 12 h sample of the ONU collection. If the collection time of the ONU sample deviated from 12 h, adjustment was performed by the known exponential elimination pattern of IFLReference Franke, Custer and Hundahl^16, Reference Zubik and Meydani¹⁸. For this purpose, we weighted area under the curve of the elimination pattern of each IFL and thereby determined factors by which ONU values would be different for every full hour before and after a 12 h period. The following factors were determined and used to multiply the ONU value for collections of 16, 15, 14, 13, 12, 11, 10, 9 and 8 h: DE (0·825, 0·861, 0·898, 0·945, 1·000, 1·074, 1·16, 1·275 and 1·435); GE (0·871, 0·893, 0·922, 0·955, 1·000, 1·059, 1·132, 1·234 and 1·369); GLYE (0·865, 0·889, 0·915, 0·952, 1·000, 1·072, 1·159, 1·276 and 1·464). Due to the similarity of the factors for the individual IFL, we used averages of these factors of each respective urine collection period for the IFL metabolites. If fractions of hours were collected, then the factors above were considered linearly to the next full hour (closest to 12 h) by interpolation and adjusted as described above. Finally, the 12 h excretion adjusted for differential times of collection and for residual IFL present at baseline was divided by 12 to arrive at the adjusted UIER (nmol/h). This was finally divided by the participant's BW (kg) to give BW-adjusted hourly excretion (nmol/h per kg).

Statistical analysis

Unpaired and paired Student's t tests as well as ANOVA calculations were performed with Excel 2004 for the Macintosh (Microsoft Inc., Redmond, WA, USA). These tests were performed on the original UIER values, as well as on logged values to consider non-normality. Because these tests lead to similar results we present most data on a non-logged basis.