Design

The present study was embedded in the Generation R Study, a population-based prospective cohort study from fetal life onwards in Rotterdam, The Netherlands⁽Reference Jaddoe, Bakker and van Duijn^21, Reference Jaddoe, van Duijn and van der Heijden²²⁾. Enrolment in the study was aimed at early pregnancy, but was allowed until the birth of the child. Information about maternal diet and other lifestyle-related variables during pregnancy was collected at enrolment. At the age of 6 years, all participating children and their mothers were invited to a dedicated research centre, to participate in detailed hands-on measurements. The study has been approved by the Medical Ethics Committee of the Erasmus Medical Center, Rotterdam. Written informed consent was obtained from all parents of the participants. The present analysis was limited to Dutch mothers, since the FFQ was validated for the assessment of dietary intake in a Dutch population. We selected mothers who were enrolled in the study before a gestational age of 25 weeks, because we aimed to assess dietary intakes in the first trimester of pregnancy. In total, 4032 Dutch mothers were enrolled before a gestational age of 25 weeks with a median of 13·6 weeks of gestation (90 % range 11·5–20·2 weeks; see Fig. 1). Data on maternal dietary intake or biomarker concentrations were available in 3960 (98 %) of these mothers. We excluded multiple births (n 104) and stillbirths (n 29) from the analyses, leaving 3827 Dutch mothers. Of the 3827 singleton live-born children, 2949 (77 %) children attended the follow-up visit at the age of 6 years. Blood pressure was successfully measured in 2863 (97 %) of the children who visited the research centre.

Fig. 1 Flow chart of the participants included for analysis.

Maternal daily dietary intake

We assessed maternal dietary intake at enrolment in the study in Dutch mothers using a modified version of the validated semi-quantitative FFQ of Klipstein-Grobusch et al. ⁽Reference Klipstein-Grobusch, den Breeijen and Goldbohm²³⁾. The FFQ considered food intake over the prior 3 months, thereby covering the dietary intake in the first trimester of pregnancy. The FFQ consisted of 293 items structured according to the meal pattern. Questions included consumption frequency, portion size, preparation method and additions. Portion sizes were estimated using Dutch household measures and photographs of foods showing different portion sizes⁽Reference Donders-Engelen, van der Heijden and Hulshof²⁴⁾. We used the Dutch food composition table for calculating daily intake of nutritional values⁽²⁵⁾.

Folic acid supplement intake

Information on folic acid supplement use (0·4–0·5 mg) and the initiation of supplementation was obtained by questionnaires at the enrolment of the study. We categorised folic acid supplement use into three groups: (1) periconceptional use; (2) start when pregnancy was known; (3) no use during pregnancy. Self-reported folic acid use was validated in a subgroup by serum folate levels in the first trimester, i.e. before 12 weeks of gestation. Within the group of mothers who reported using folic acid supplements (n 204), the median of serum folate was 23·5 (range 4·3–45·3) nmol/l, whereas the median serum folate concentration of mothers who did not report folic acid supplement use (n 68) was 11·1 (range 4·7–29·6) nmol/l. The difference in distribution function (Mann–Whitney test) was statistically significant (P< 0·001)⁽Reference Timmermans, Jaddoe and Hofman²⁶⁾. Information about folic acid supplement use was available in 2505 subjects (87·5 %).

Folate, homocysteine and vitamin B₁₂ concentrations

In early pregnancy (median 12·9 weeks of gestation, 90 % range 10·6–16·8), venous samples were drawn and stored at room temperature before being transported to the regional laboratory for processing and storage for future studies. Processing was aimed to be completed within a maximum of 3 h after venous puncture. The samples were centrifuged and thereafter stored at − 80°C⁽Reference Jaddoe, Bakker and van Duijn²¹⁾. To analyse folate, homocysteine and vitamin B₁₂ concentrations, EDTA plasma samples (folate and homocysteine) and serum samples (vitamin B₁₂) were picked and transported to the Department of Clinical Chemistry at the Erasmus University Medical Center, Rotterdam in 2008. Folate, homocysteine and vitamin B₁₂ concentrations were analysed using an immunoelectrochemoluminence assay on the Architect System (Abbott Diagnostics B.V.). The between-run CV for plasma folate were 8·9 % at 5·6 nmol/l, 2·5 % at 16·6 nmol/l and 1·5 % at 33·6 nmol/l, with an analytic range of 1·8–45·3 nmol/l. The same CV for plasma homocysteine were 3·1 % at 7·2 μmol/l, 3·1 % at 12·9 μmol/l and 2·1 % at 26·1 μmol/l, with an analytic range of 1–50 μmol/l. This CV for serum vitamin B₁₂ was 3·6 % at 142 pmol/l, 7·5 % at 308 pmol/l and 3·1 % at 633 pmol/l, with an analytic range of 44–1476 pmol/l. Plasma concentrations of maternal folate, homocysteine and serum concentrations of vitamin B₁₂ in the first trimester of pregnancy were available in 2305 (80·5 %) of the mothers of the children included in the present study. Missing data were mainly due to logistical reasons.

Blood pressure measurements

Blood pressure measurements in children were conducted around the age of 6 years in a dedicated research centre in the Erasmus Medical Center, Rotterdam, The Netherlands. The child was lying quietly, while systolic blood pressure and diastolic blood pressure were measured at the right brachial artery in a supine position, four times with 1 min intervals. A cuff was selected with a cuff width approximately 40 % of the arm circumference and long enough to cover 90 % of the arm circumference. We used the validated automatic sphygmomanometer Datascope Accutorr Plus™ (Mindray DS USA, Inc.)⁽Reference Wong, Tz Sung and Leung²⁷⁾. Of all children visiting the research centre, 91·3 % had four successful blood pressure measurements available.

Covariates

Information on maternal age, pre-pregnancy BMI, parity, alcohol use and smoking habits during pregnancy, and educational level was obtained from questionnaires. Maternal education was defined as highest followed education according to the classification of Statistics Netherlands and categorised into primary, secondary and higher⁽²⁸⁾. Child sex, gestational age at birth and birth weight were obtained from midwife and hospital registries. Breast-feeding (ever/never) was assessed using questionnaires. Current height and weight were measured without shoes and heavy clothing at the visit at 6 years, and BMI (kg/m²) was calculated.

Statistical methods

Differences in child characteristics at the age of 6 years between boys and girls were assessed using the t test and χ² tests for independent samples. Maternal dietary intake variables were categorised into quintiles. This approach was used for all dietary exposures (total energy, carbohydrate, fat, protein intake and protein:carbohydrate ratio; Ca, Fe and Na intake; folate, homocysteine and vitamin B₁₂ concentrations). We used mixed models to assess the associations between predictors and blood pressure⁽Reference Laird and Ware²⁹⁾. The mixed-model method fits each of the as many as four blood pressure measurements of every child as repeated outcome measures. An advantage of this modelling approach over using the average measure of blood pressure for each child as an outcome is that children with more measurements and less variability in their measurements are assigned more weight than those with fewer measurements, more variability or both⁽Reference Bakker, Rifas-Shiman and Kleinman^9, Reference Gillman and Cook³⁰⁾. We used similar mixed models to assess the association of folic acid supplement use with blood pressure at the age of 6 years. All analyses were adjusted for child's sex and age at blood pressure measurement (crude model). Potential covariates were selected based on previous literature⁽Reference Lawlor, Najman and Sterne^31, Reference Lawlor and Smith³²⁾. We assessed crude associations, adjusted for age and sex, of possible covariates with childhood blood pressure. Only the covariates that were significantly associated with systolic or diastolic blood pressure in the present study population were included in our fully adjusted model. The fully adjusted model included maternal age, pre-pregnancy BMI, alcohol use and smoking during pregnancy, educational level, gestational age at birth, birth weight, current BMI and month in which blood pressure measurement was taken. Tests for trends were conducted by using maternal dietary intake variables as the continuous variable in the linear mixed models. We provided the effect per standard deviation increase in the dietary intake variable. In the macronutrient analyses, we used the energy partition method to adjust for energy intake of the other macronutrients, since total energy intake and macronutrient intakes were strongly correlated⁽³³⁾. The actual energy derived from the macronutrients was used in the analyses. In the micronutrient analyses, we used the residual nutrient method, and additionally adjusted for total energy intake⁽³³⁾.

Missing values in covariates (ranging from 0 to 15 %) were multiple-imputed to reduce potential bias associated with missing data⁽Reference Sterne, White and Carlin³⁴⁾. We created five imputed datasets and each dataset was analysed separately to obtain the effect sizes and standard errors. The results of all the five imputed analyses were pooled and are presented in the present study. We investigated maternal macronutrient intake, micronutrient intake and maternal biomarker concentrations in pregnancy. Within these exposure groups, variables are correlated (Table S1, available online). To take into account multiple testing, we applied a Bonferroni correction and considered a P value lower than 0·017 (0·05/3 (three exposure groups)) as statistically significant. The mixed models were fitted using the SAS version 9.2 (SAS Institute, Inc.). All other statistical analyses were performed using SPSS version 17.0 for Windows (SPSS, Inc.).