Study design and participants⁽ Reference Celis-Morales, Livingstone and Marsaux ^{3 )}

The Food4Me intervention study was designed as a pan-European randomised controlled trial (RCT) to determine whether providing personalised dietary advice leads to greater improvements in eating patterns and health outcomes compared with a conventional population-based general guidelines approach. Seven research centres in seven European countries participated with more than 220 participants from each centre. DBS samples were collected and analysed at three time points: at baseline, after 3 and 6 months of intervention, respectively. Details of the study design and baseline characteristics of the participants have been published elsewhere⁽ Reference Celis-Morales, Livingstone and Marsaux ^{3 )}. The seven participating study centres were located in Munich (Germany), Athens (Greece), Dublin (Ireland), Maastricht (The Netherlands), Warsaw (Poland), Navarra (Spain) and Reading (UK), and recruitment was carried out countrywide. A total of 5562 participants (65 % females) were screened online over a 12-month period between August 2012 and August 2013 and consented to participate. Of these, 1607 (28·9 %) were recruited to the RCT. Participants aged 18–79 (mean 39·8 (sd 13·1)) years were included in the study, of whom 60·9 % (n 980) were women and 96·7 % were from white-European background. The mean BMI of all the participants was 25·5 (sd 5·2) kg/m², and 44·8 % (n 721) of the participants were overweight or obese (BMI≥25·0 kg/m²). This study was conducted according to the guidelines laid down in the Declaration of Helsinki, and all the procedures involving human subjects were approved by the ethics committees of the participating centres. Written or online informed consent was obtained from all the participants. Further details on study design and participant characteristics can be found in the study by Celis-Morales et al.⁽ Reference Celis-Morales, Livingstone and Marsaux ^{3 ,} Reference Livingstone, Celis-Morales and Navas-Carretero ^{19 )}.

Samples and sampling protocol

Finger-prick blood samples were collected by participants themselves using a collection pack with two cards, one provided by Vitas Ltd, and one by DSM. Before spotting blood, cards for vitamin D analysis (Whatman Protein Saver 903 Card; GE Healthcare) were pre-treated with 1 % of 2,6-di-tert-butyl-4-methylphenol (BHT) dissolved in methanol (MeOH); 30 µl of 1 % BHT in MeOH were pipetted to each circle on the card and allowed to dry for at least 30 min at RT. These pre-treated cards were packed in an airtight Al bag (Whatman Foil Bags, item no. 10534321; Whatman Inc.) with a drying agent (Sorb-it, item no. 10548234; Süd-Chemie) and stored at RT until use. To help with blood collection, participants had access to an online video demonstration with written instructions and frequently asked questions in the language of recruitment. For the finger pricks, 2·0-mm contact-activated lancets (BD Microtainer; Becton, Dickinson and Company) were used. Each participant was asked to fill the two DBS cards each with five spots at each collection time point. This is the approximate equivalent of five drops of blood or 250 µl of blood/card. When the ten blood spots were filled, participants were instructed to let the cards dry at RT for at least 2 h, but not longer than 4 h, before samples were put back into the Al bags and returned by mail to the corresponding recruiting centre. The centres verified the content of the bags, and shipped one bag containing the DBS card to DSM (DSM Nutritional Products Ltd) for measurements of vitamin D (25(OH)D₂ and 25(OH)D₃). Although the shipments carried out done at ambient temperature, the closed bags were stored at the centres and at DSM at nominal −20°C.

Calibration was carried out using whole-blood samples received from blood donors of the ‘Blutspendezentrum SRK beider Basel’ (Blood Donation Centre at Basel Hospital), including haematocrit values for each sample. The calibration samples (n 15) had a mean haematocrit content of 44·2 % (range 38·7–49·3 %). Donors were twelve females and three males with an average age of 49 years. The calibration samples were prepared as follows: blood aliquots of 50 µl were pipetted onto a card and allowed to dry for 2–4 h at RT, avoiding exposure to direct sunlight; the cards were then transferred into Al foil bags with a desiccant inside and then stored in a freezer at nominal −20°C. Calibration samples were used for 3–6 months. As quality control, DBS samples with independently determined 25(OH)D₃ content were analysed within each analytical run.

Reagents and instruments

25-Hydroxycholecalciferol monohydrate (25-OH-D₃ monohydrate) was obtained from Dr Ehrenstorfer; 25-hydroxyergocalciferol (25(OH)D₂) and SDS (≥99 %) were supplied by Sigma-Aldrich; 26,26,26,27,27,27-hexadeutero-25-hydroxycholecalciferol (25(OH)D₃-d6) was supplied by Medical Isotopes; 2,6-di-tert-butyl-4-methylphenol (≥99 %, BHT), acetonitrile (gradient grade), formic acid (Suprapur), toluene and MeOH were from Merck; and MS-grade water was prepared using a Milli-Q instrument (Merck Millipore). Eppendorf tubes were centrifuged using a 5417 R model centrifuge (Vaudaux-Eppendorf), and evaporation was carried out using a Cyclone (Prolab). Analyte separation was performed using an Agilent 1260 HPLC with auto sampler, two binary pumps and column oven coupled with an AB Sciex Qtrap 5500 MS/MS-System with atmospheric pressure photoionisation (APPI source).

Assay

Sample preparation

Before analysis, the samples were assessed to check whether they met the quality criteria (Fig. 1): spot size (circle filled), thoroughly soaked (observed from the back) and one application of blood (not composed of many small spots). Two punches (inner diameter of 3·175 mm) were taken out of the card and placed into a 2-ml Eppendorf tube. After adding 100 µl of 0·1 % SDS solution and 20 µl of internal standard (ISTD, 25,25,25,26,26,26-hexa-deutero-25(OH)D₃, 25 ng/ml in MeOH), the tubes were shaken at 40°C for 30 min. Subsequently, 400 µl of acetonitrile was added and the shaking continued at RT for 5 min (260/min, IKA shaker). Following this, the tubes were centrifuged at 20 000 g for 5 min, and the supernatant was transferred into a new 2-ml Eppendorf tube. The solvent was evaporated to dryness under vacuum (Cyclone), and the residue was reconstituted with 50-µl injection solvent (MeOH–water, 70:30) and transferred into a micro vial for analysis.

Fig. 1 Quality control criteria for dried blood spots from the Food4Me study. (a) Spot suitable for analysis. (b–d): Spots not suitable for analysis due to (b) small spot size not filling the circle, (c) multiple application of too small spots, including spots outside the circle, (d) multiple application of small spots and no thorough soaking of the paper (view from the back).

Determination of nominal 25-hydroxy vitamin D₃ content of calibration samples

An aliquot of each whole-blood sample spotted for calibration was used for preparation of plasma. The 25(OH)D₃ content of this plasma was measured using an established reference method⁽ Reference Lauridsen, Halekoh and Larsen ^{20 )}. The haematocrit content of the whole blood used for calibration was measured at the blood donation centre. As the haematocrit contents of the study samples were unknown, an estimated mean value of 40 % was used for calculation. This value was based on the rounded mean haematocrit content of the samples used for method development and validation. The following equation was used to normalise the calibration samples accordingly:

$${\rm c(25(OH)D}_{{\rm 3}} {\rm )}_{{{\rm normalised}}} = \, {\rm c(25(OH)D}_{{\rm 3}} {\rm )}_{{{\rm measured}}} {\times}{{(100{\minus}{\rm haematocrit})} \over {60}}.$$

$$$$ c(25(OH)D₃)_normalised: concentration of 25(OH)D₃ (ng/ml plasma) in a calibration sample, normalised to 40 % haematocrit content; c(25(OH)D₃)_measured: concentration of 25(OH)D₃ (ng/ml plasma) measured with reference method in plasma samples obtained from whole blood used for calibration; haematocrit: haematocrit value (%) for whole-blood sample obtained from Blutspendezentrum Basel.

For study samples, the resulting 25(OH)D₃ concentration was then corrected for sex-specific mean haematocrit values of 41·5 % for female and 46·5 % for male participants by applying correction factors of 1·026 for females and 1·121 for males. This was based on information from the sex-specific reference ranges and means obtained from the seven clinical centres (U Hoeller et al., personal information).

Performance criteria

The method was validated based on the procedures described in the ‘Guideline on bioanalytical method validation’ of the European Medicines Agency^{( 21 )}, taking into account specific requirements and recommendations for DBS analysis⁽ Reference Timmerman, White and Globig ^{22 )}. Selectivity was tested by comparing chromatograms from five samples of different donors with and without spike of either 25(OH)D₃-d6 or 25(OH)D₃ at 20 ng/ml blood. As the samples contained endogenous 25(OH)D₃, area ratios of qualifier ion m:z (383:257) to quantifier ion m:z (383:211) were calculated and used for the assessment of selectivity of the detection of 25(OH)D₃. Carry over was assessed by measuring blank samples after analysis of high-content samples. No significant carry over was observed. Linearity was determined by analysis of calibration samples according to the method on 3 different d. Linear regression of the analyte peak area ratio (analyte peak area v. ISTD peak area) against the nominal concentration was calculated. Differences between nominal concentrations and calculated concentrations were determined and expressed in percentage. Deviations of the measured values from nominal values should be ≤20 % and at least two-thirds of the calibration levels at each day should meet these criteria. As calibration was performed with endogenous samples, only a limited concentration range could be tested: 32·5–120 nmol/l calculated as plasma concentrations. The lower limit of quantification was set to 25 nmol/l, as this represents the accepted cut-off for vitamin D deficiency⁽ Reference Bendik, Friedel and Roos ^{23 )}. Accurate determination of lower concentrations was not within the scope of this study. For assessing accuracy, samples of five different subjects were analysed. Before spotting the whole-blood samples, plasma was separated from a whole blood aliquot of each sample and analysed using a reference method⁽ Reference Bischoff-Ferrari, Dawson-Hughes and Stocklin ^{24 )}. Nominal DBS concentrations were calculated by correcting the plasma concentrations with the corresponding haematocrit values (nominal concentration=plasma concentration×(100–haematocrit value)/100). DBS samples from each subject were analysed in 5-fold and compared with the nominal DBS concentration. Mean accuracy was calculated and reported as percentage of nominal DBS concentration value. As additional measure for accuracy and of the influence of varying haematocrit values in the calibration samples, we re-analysed calibration samples for which the 25(OH)D₃ concentration values were assigned previously within a new set of calibration samples with independently assigned 25(OH)D₃ concentration values. The mean haematocrit value of these samples was 42·0 (range 39·6–43·8) %. To determine intra-day precision, the results from samples prepared for accuracy were used. To estimate inter-day precision, triplicates of each sample were analysed on 3 different d. Precision was reported as CV of the measured concentrations. For determination of stability in the auto sampler at 10°C, extracts of incurred and spiked DSB samples were re-analysed after 60 h. Long-term stability was tested by storing DBS samples for upto 6 months at nominal −20°C and comparing the content analysed after the storage with initial values. There was good stability under both conditions.

Statistical analysis

Longitudinal linear mixed models were used to model 25(OH)D₃ levels. Limit of detection (LOD) values in the 25(OH)D₃ measurements were replaced by 12·5 nmol/l (four measurements, 0·1 %) and lower limit of quantitation (LOQ) values were replaced by 16·25 nmol/l 25(OH)D₃ (134 measurements, 3·5 %). Sensitivity analyses were carried out assuming 0 nmol/l for LOD and LOQ values, and 25 nmol/l for LOD and LOQ values, respectively. For the centre with by far the most LOQ values (Dublin), the model fits differed by −4·0 nmol/l in winter, assuming 0 nmol/l for LOD and LOQ, and +0·2 nmol/l in summer. Assuming 25 nmol/l for LOQ and LOD values, the difference was +2·2 nmol/l in winter and −0·1 nmol/l in summer. The absolute deviations for all other centres were ≤2·4 nmol/l in winter and ≤0·2 nmol/l in summer.

To model the seasonal variation at the study sites, the study centre and the interaction of study centre with the functions sin(sample year×2×π) and cos(sample year×2×π) were included as fixed effects, and the participants as a random effect. The 20 January was found to be the consensus date across all study centres when the 25(OH)D₃ concentrations reached their nadir. To simplify the subsequent modelling and interpretation, a single normalised sine function was derived, which oscillated between −1·0 when the 25(OH)D₃ concentration was at its lowest on the 20 January and +1·0 when the 25(OH)D₃ concentration was at its highest on the 21 July. It assumes synchronised timing of seasons across all study centres, but it differentiates mean levels and seasonal amplitudes by study centre. The function was coded as follows: standardised seasonal amplitude=SSA=sin((sample year−20/365·25−0·25)×2×π). On the 20th of each month, this function had the following values: −1·0 in January, −0·9 in February, −0·5 in March, 0·0 in April, 0·5 in May, 0·9 in June, 1·0 in July, 0·9 in August, 0·5 in September, 0·0 in October, −0·5 in November and −0·9 in December. For a sample taken on the 30 June, the sample year would equal 2013·5, and the resulting SSA would be 0·94. For each measurement, the corresponding SSA was thus calculated. The final model was then fitted using centre and the centre-SSA interaction as fixed effects and participant ID as random effect (presented in Table 2 and Fig. 2). Owing to the absence of a gold standard method, the biological and the analytical variability could not be separated in the present data set. The overall variation should thus be considered as a highly conservative estimate of the variation of the analytical method. R statistics software version 3.02 was used for all statistical analyses^{( 25 )}, and within the R statistics software the function lme() in the package nlme⁽ Reference Pinheiro, Bates and DebRoy ^{26 )} was used for the mixed model regressions.

Fig. 2 Individual measurements for 25-hydroxy vitamin D₃ (25(OH)D₃) by research centre and sampling date, as well as seasonal regression by centre. The model included 3711 measurements from 1412 participants. The predictors were the centre and the interaction of each centre with the standardised seasonal amplitude (SSA). The SSA for this data set is a sine function reaching its minimum −1·0 on 20 January and its maximum +1·0 on 21 July, as explained in the statistical methods section. The participant ID was included as random effect. The fixed effect regression fits are visualised within each plot. The largest seasonal oscillations were observed in Germany (92·1 nmol/l in summer v. 41·9 nmol/l in winter) and the smallest in Poland (67·1 nmol/l in summer v. 50·4 nmol/l in winter). Example calculation: on 20 May, the SSA reaches 0·5, therefore the estimate for a participant in Germany would be 67·0+0·5×25·1=79·6 nmol/l. Horizontal lines indicate vitamin D status intervals: <25 nm deficient, 25–50 nm insufficient, 50–75 nm sufficient, >75 nm optimal range.