Methods

Measurement error model

We assumed protein, Na and K intake assessed by urinary excretion to be unbiased in assessing usual intake⁽ Reference Jenab, Slimani and Bictash ^{3 )}, which we assumed not to vary within the 3 years of study. All our measurement error models assumed a linear relationship between DP, 24hRT, 24hRW, FFQ, biomarker and the true unknown intake T. In our measurement error model i is the person, and j indicates the occasion. Furthermore, α _X expresses the constant bias for reference method X (X being DP for the DP method, 24hRT for the telephone-based 24hR, and 24hRW for the web-based 24hR) and β _X is the proportional scaling bias where α _Q and β _Q are similar respective parameters for the FFQ. The person-specific bias of the reference method is given by w _xi and for the FFQ by v _i . Finally, ε _Xij is the random error with mean zero and constant variance for the reference method, whereas ε _Qij is the random error for the FFQ.

(1) $${\rm Reference}\,{\rm method}\,X\colon\,\,Xij=\alpha _{X} {\plus}\beta _{X} T{\plus}w_{{xi}} {\plus}{\varepsilon}_{{Xij}} {\rm ,}$$

(2) $${\rm FFQ}\colon\,\,Qij=\alpha _{Q} {\plus}\beta _{Q} T{\plus}v_{i} {\plus}{\varepsilon}_{{Qij}} {\rm ,}$$

(3) $${\rm Biomarker}\colon\,\,Mij=T{\plus}{\varepsilon}_{{Mij}} {\rm .}$$

Statistical analysis

Descriptive statistics were presented in percentages and as means with their standard deviation. Presence of bias between the mean of the recovery biomarker and the mean of the available replicates of FFQ, DP, 24hRW and 24hRT was tested by performing a Student’s paired t test. The significance level was set at a two-sided P value of 0·05.

A Bayesian approach⁽ Reference Richardson and Gilks ^{23 )}, Markov Chain Monte Carlo, the PROC MCMC procedure in SAS, was used to estimate the parameters of our measurement error models for which uninformative priors were set to make the model data driven (syntax can be found in Appendix II). The sensitivity of our measurement error model was tested by using different distributions for the parameters and changing the prior estimates. As little variation in model outcomes was observed, we assumed the model to be robust. Sex-specific models for Na did not converge (because of the low variance of the person-specific biases compared with within- and between-person variances) and are therefore not reported. To assess whether the reference method adequately corrects for measurement error it should be unbiased, which is indicated by the absence of proportional scaling bias (a β _x equal to one in equation 1 of the measurement error model indicates that there is no proportional scaling bias present). Furthermore, the reference method should have uncorrelated errors with the errors in the FFQ; that is, the error correlation should be 0. The error correlation (ρ _XQ ) is calculated according to formula 4 specified below from the measurement error model outcomes. From the model outcomes we also calculated the attenuation factor (λ _X ) for each reference method according to formula 5 as specified below. Note that this is not the attenuation factor for the FFQ using the reference method, but the attenuation factor for the reference method using the biomarker as reference.

(4) $$\rho _{{XQ}} ={{{\mathop{\rm cov}} _{{wivi}} } \over {\sqrt {\left( {{\mathop{\rm var}} {\varepsilon}_{{Xij}} {\plus}{\mathop{\rm var}} w_{{xi}} } \right){\times}\left( {{\mathop{\rm var}} {\varepsilon}_{{Qij}} {\plus}{\mathop{\rm var}} v_{i} } \right)} }},$$

(5) $$\lambda _{X} ={{\beta _{X} {\times}{\mathop{\rm var}} \,T} \over {\beta _{X} ^{2} {\times}{\mathop{\rm var}} \,T{\plus}{{{\mathop{\rm var}} \,{\varepsilon}_{{Xij}} } \over k}{\plus}{\mathop{\rm var}} \,w_{{xi}} }},$$

where cov _wivi is the covariance between the error in the FFQ and the error in the reference method X; varε _Xij is the variance of the random error of the reference method X; varw _xi indicates the variance of the person-specific bias of method X; varv _i is the variance of the person-specific bias of the FFQ; varε _Qij is the variance of the random error of the FFQ; and β _X is the proportional scaling bias of method X. To obtain the estimates of the attenuation factor for multiple DP and 24hR, the variance of the random error of the method (varε _Xij ) was divided by the number of measurements (k) of the method. All statistical tests were performed in SAS version 9.3 (SAS Institute Inc., 2012).

A sensitivity analysis was performed, comparing the model outcomes from the complete urine data set with the model outcomes after exclusion of the urine samples with <78 % PABA recovery⁽ Reference Jakobsen, Ovesen and Fagt ^{22 )}. Measurement error model outcomes did not differ substantially when no urine samples were excluded compared with excluding urines with PABA <78 %. This points in the same direction as the finding of Subar et al. ⁽ Reference Subar, Midthune and Tasevska ^{24 )}, who observed a modest effect on correction factors when urines were excluded on the basis of PABA recovery compared with not excluding urines in the OPEN study⁽ Reference Subar, Midthune and Tasevska ^{24 )}. We therefore report the results based on the complete urine set in this article.

Results

At baseline, participants were on average 55·7 (sd 10·2) years of age, and women were slightly younger than men (53·8 v. 58·0 years, Table 1). The average BMI was 25·1 (sd 3·7) kg/m², and a higher percentage of women (64 %) had a healthy BMI (18·5–25·0 kg/m²) compared with men (46 %). Furthermore, 58 % of the men and 48 % of the women were classified as highly educated (university or college).

Table 1 Baseline characteristics of the study population (Mean values and standard deviations; percentages)

* Primary or lower education.

† Secondary or higher vocational education.

‡ University or college.

The percentage of the number of 24hRT and 24hRW varied between 18 and 29 % over the seasons (Table 2). The variation in the number of urine collections per season was larger, and varied between 4 % collected in spring and 51 % in summer. Most DP (34 %) were collected in spring (Table 2). For the FFQ, 39 % were collected in autumn and 12 % in winter. The DP, 24hRT, 24hRW and urine collections were evenly distributed between week (range, Monday–Friday 63–76 %) and weekend days (range, Saturday–Sunday 24–37 %).

Table 2 Percentage of the number of collection days distributed over the seasons and weekend v. weekdays

DP, duplicate portion; 24hRT, telephone-based 24 h recall; 24hRW, web-based 24 h recall.

* Weekend days are Saturdays and Sundays.

The DP underestimated protein by 20·9 %, K by 6·8 % and Na by 33·5 % (Table 3). For all nutrients, underestimation was smallest using the 24hRT (protein 12·7 %, K 4·7 % and Na 28·7 %). The FFQ, the method to be validated, underestimated protein (22·6 %) and Na (41·6 %) to the largest extent. A similar pattern was observed for men and women. Overall, women tended to underestimate to a lesser extent than did men for all dietary assessment methods and nutrients.

Table 3 Mean intake and bias for the intake of protein, potassium and sodium, compared with the urinary excretion marker (Mean values and standard deviations)

n, number of participants.

* Values were significantly different from the biomarker (P<0·01).

† For Na, sex-specific models did not converge because of the low variance of the person-specific biases compared with within- and between-person variances and are therefore not reported.

A proportional scaling bias, as indicated with β _x in Table 4, closer to 1 means less bias. In general, the estimates for the DP were closest to 1, 0·58 for protein, 0·72 for K and 0·52 for Na, compared with those for 24hRT and 24hRW (Table 4). For the sex-specific models, the proportional scaling bias was closest to 1 for the DP for K for women (0·77) and for protein for men (0·72). However, the 24hRT performed better for protein for women (0·62) and for K for men (0·93).

Table 4 Proportional scaling bias and correlated error with the FFQ for the intake of protein, potassium and sodium (Mean values and standard deviations)

24hR, 24 h recall.

* Adjusted for BMI and sex.

† Adjusted for BMI.

‡ For Na, sex-specific models did not converge because of the low variance of the person-specific biases compared with within- and between-person variances and are therefore not reported.

In the total population, the correlated errors between the DP and FFQ were the lowest for the two micronutrients, Na (0·19) and K (0·17) (Table 4). For protein, the error correlations with the FFQ were comparable between the three reference methods (0·28 for the DP and 24hRT, and 0·27 for the 24hRW). The range of correlated errors was comparable for men (0·12–0·28) and women (0·08–0·29).

An attenuation factor close to one indicates an overall better estimation of the nutrient intake. In the total population, looking at estimates for single measurements, attenuation factors for the DP were highest for all three nutrients (0·74 for protein, 0·54 for K and 0·43 for Na), whereas for the 24hRW attenuation factors tended to be the lowest for all nutrients (0·30 for protein, 0·31 for K and 0·18 for Na) (Table 5). The same trend was seen for women and men separately. Attenuation factors increased when the number of replicates was expanded. For protein, the attenuation factor for one measurement of the DP was 0·74, whereas for the 24hRT three measurements gave a similar attenuation factor (0·73). In general, attenuation factors for all dietary assessment methods tended to be higher for men than for women.

Table 5 Attenuation factors for the reference methods for the intake of protein, potassium and sodium (Mean values and standard deviations)

DP, duplicate portion; 24hRT, telephone-based 24 h recall collection; 24hRW, web-based 24 h recall collection.

* Adjusted for BMI and sex.

† Adjusted for BMI.

‡ For Na, sex-specific models did not converge because of the low variance of the person-specific biases compared with within- and between-person variances and are therefore not reported.

Discussion

In this Dutch validation study, we found that all dietary assessment methods underestimated the intake of protein, K and Na compared with the biomarker measurements where the 24hRT showed the smallest underestimation. Furthermore, all dietary assessment methods were biased (affected by proportional scaling bias) and showed correlated errors with the FFQ for protein, K and Na. However, dietary intake measures from the DP were less affected by proportional scaling bias compared with the 24hRT and 24hRW. Furthermore, error correlations between the DP and FFQ were the lowest. Attenuation factors also indicated that the DP had the best performance (attenuation factors were closer to one).

To our knowledge, this is the first study assessing error correlations between the FFQ and DP, proportional scaling bias for DP and estimating attenuation factors for the DP. Research on 24hR has among others been performed in a pooled analysis of five American validation studies comparing protein intakes assessed by the FFQ and 24hR with urinary N excretion⁽ Reference Freedman, Commins and Moler ^{25 )}. Freedman et al. ⁽ Reference Freedman, Commins and Moler ^{25 )} found wide ranges of study-specific attenuation factors (0·14–0·54) for the 24hR. This is comparable to our results, but we found estimates at the higher end of this range. One of the possible explanations is that our study population was highly motivated; they were willing to collect, in addition to filling out multiple 24hR and various food and lifestyle questionnaires, two urine and two DP samples. Above that, a high percentage of our participants were highly educated. Furthermore, cultural differences in dietary patterns and the design of the FFQ and 24hR could also explain our findings to be in the upper part of the range.

Proportional scaling bias for the 24hRT for protein was similar to that found in the OPEN study, a large American study from Montgomery County, Maryland, for women (0·62 for DuPLO v. 0·60 for OPEN), but our estimate was slightly lower for men (0·64 for DuPLO v. 0·70 for OPEN)⁽ Reference Kipnis, Subar and Midthune ^{1 )}. Error correlations between the 24hR and FFQ were slightly higher in our study compared with the EPIC study, a large European multi-centre study, showing 0·21 for K and 0·21 for protein⁽ Reference Ferrari, Roddam and Fahey ^{5 )}, and the OPEN study (showing 0·24 for protein for women and 0·18 for men)⁽ Reference Kipnis, Subar and Midthune ^{1 )}. Prentice & Huang⁽ Reference Prentice and Huang ^{26 )} found slightly higher error correlations between their FFQ and 24hR for protein (0·33)⁽ Reference Prentice and Huang ^{26 )}. Differences between error correlations of the 24hR with the FFQ in studies are expected because of different sets of covariates included – different modes of administration (web based and interviewer administered) and numbers of replicates of a 24hR – varying ways of portion-size estimations and differences between the study populations (ethnic groups, social economic status, age).

The attenuation factor for Na intake for the DP (0·43) was remarkably higher than for both 24hR administrations (0·19 for the 24hRT and 0·18 for the 24hRW), and taking a second replicate for the DP increased the attenuation factor to 0·65. The DP for Na was also less affected by proportional scaling bias (β _DP=0·52) and demonstrated a lower error correlation with the FFQ (0·19) compared with the 24hRT and 24hRW. Accurately assessing Na intake is challenging because of the high variability of Na content of foods⁽ Reference Champagne and Cash ^{27 )}, which is not always accurately reflected in FCD. In addition, it is difficult to accurately report the amount of salt added during cooking or at the table. In the 24hR and FFQ in this study, there is no question included about added salt during cooking or at the table. The accuracy of dietary intake estimates of Na from 24hR and FFQ is therefore expected to be limited. This is supported by other research about Na estimation from 24hR, FFQ and dietary records⁽ Reference Champagne and Cash ^{27 )}. The higher attenuation factor and proportional scaling bias for the DP could be explained by the fact that salt added during cooking was included as a sample of the cooked meal was collected and the DP were chemically analysed and estimates did not depend on information in FCD. However, attenuation factors for Na for the DP were still notably lower than those for protein and K intake.

Correlated errors between the FFQ and reference methods for protein intake tended to have the same order of magnitude for all methods, whereas for K and Na intake the DP showed lower error correlations than the 24hRT and 24hRW. Thus, there must be a source of error equally influencing the estimation of protein in all four methods apart from the correlated errors that are expected between the FFQ and 24hR (use of the same FCD to calculate nutrients, estimation of portion sizes and memory based). A similar error source for all four methods (FFQ, DP, 24hRT and 24hRW) could be response errors, meaning that people tended to forget (for FFQ and 24hR) or not collect (for DP), either on purpose or not, protein-rich products.

A weakness of this study is the unequal spread of biomarker measurements over the seasons (summer was over-represented and spring under-represented), while they were assumed unbiased in our measurement error model. This assumption was based on evidence from the literature that does not indicate seasonal variation of nutrient intake in western populations⁽ Reference Ma, Olendzki and Li ^{28 ,} Reference van Staveren, Deurenberg and Bureman ^{29 )}. Furthermore, the different methods did not exactly cover the same time period. However, we were interested in a person’s usual intake and not in the dietary intake on a specific day. We assumed that energy and nutrient intake of a person would be fairly stable over a longer time period. Thus, although intake data measured by the different dietary assessment methods did not cover the same time period, they could be all considered to represent a person’s usual energy and nutrient intake. Therefore, comparisons between methods can be made.

We reported the results based on all urine samples collected, independent of the PABA results. This was based on a sensitivity analysis to exclude urine samples based on PABA, focussing on the main outcomes: attenuation factor and correlated error. These main outcomes did not differ substantially between inclusion of all urine samples and inclusion of only the complete urine samples (based on PABA recovery). Furthermore, not excluding urine samples provided a larger sample size. However, results for bias (i.e. difference between levels of intake) must be regarded rather carefully as they differed significantly for protein and K when incomplete urine samples were excluded.

Taking into account that in general the DP showed lesser proportional scaling bias, the highest attenuation factors and the lowest error correlations with the FFQ, this method appeared more promising as a reference method than did the 24hR. Important considerations in the collection of DP are that it is burdensome for participants, requires a lot of time from the researcher, is expensive to perform and reactivity bias – mostly causing underestimation of habitual intake – is expected. We carefully instructed our participants not to deviate from their habitual intake and provided them with written instructions, including tips to remind the participant to include everything in the collection baskets. Nevertheless, the DP showed substantial underestimation for protein, K and Na.

Attenuation factors calculated for FFQ using the 24hR as a reference method are affected by correlated errors between the two methods⁽ Reference Wong, Day and Bashir ^{30 )}. Better estimates of attenuation factors will be obtained if these correlated errors between the FFQ and 24hR are taken into account. The error correlations between the 24hR and FFQ found in this study could be considered in the calculation of attenuation factors; however, generalising results from one study population to another should always be done conservatively, taking into account the characteristics of both study populations and the study setup.