Introduction
Coffee is consumed widely within most societies around the world (International Coffee Council, 2012). Scandinavian countries rank highly in terms of caffeine intake, with an average daily intake of >400 mg of caffeine (equivalent to approximately four cups of coffee) (Fredholm, Bättig, Holmén, Nehlig, & Zvartau, Reference Fredholm, Bättig, Holmén, Nehlig and Zvartau1999). During pregnancy, coffee consumption remains widespread (Fredholm et al., Reference Fredholm, Bättig, Holmén, Nehlig and Zvartau1999; Lukic, Barnung, Skeie, Olsen, & Braaten, Reference Lukic, Barnung, Skeie, Olsen and Braaten2020). However, a vast array of physiological changes during gestation result in a significant reduction in maternal caffeine metabolism (Aldridge, Bailey, & Neims, Reference Aldridge, Bailey and Neims1981; Horning, Butler, Nowlin, & Hill, Reference Horning, Butler, Nowlin and Hill1975; Soyka, Reference Soyka1981). Caffeine and its primary metabolites (paraxanthine, theophylline, and theobromine) are known to readily cross the placenta (Fernandes et al., Reference Fernandes, Sabharwal, Smiley, Pastuszak, Koren and Einarson1998; Goldstein & Warren, Reference Goldstein and Warren1962), and are not easily cleared due to underdevelopment of fetal caffeine metabolizing enzymes (Aldridge et al., Reference Aldridge, Bailey and Neims1981; Grosso & Bracken, Reference Grosso and Bracken2005). Consequently, it has been proposed that accumulated caffeine metabolites may exert detrimental effects on the developing fetal brain (Brent, Christian, & Diener, Reference Brent, Christian and Diener2011; Gressens, Mesples, Sahir, Marret, & Sola, Reference Gressens, Mesples, Sahir, Marret and Sola2001; Qian, Chen, Ward, Duan, & Zhang, Reference Qian, Chen, Ward, Duan and Zhang2020; Ross, Graham, Money, & Stanwood, Reference Ross, Graham, Money and Stanwood2014; Temple et al., Reference Temple, Bernard, Lipshultz, Czachor, Westphal and Mestre2017).
Several observational epidemiological studies have investigated the relationship between maternal coffee/caffeine consumption during pregnancy and offspring neurodevelopment; however, they have yielded inconsistent results (James, Reference James2021). Many have found that increased maternal caffeine consumption is associated with offspring neurodevelopmental difficulties (NDs) (Hvolgaard Mikkelsen, Obel, Olsen, Niclasen, & Bech, Reference Hvolgaard Mikkelsen, Obel, Olsen, Niclasen and Bech2017; Nishihara et al., Reference Nishihara, Kobayashi, Ikeda-Araki, Miyashita, Itoh, Yamazaki and Kishi2022; Patti et al., Reference Patti, Li, Eliot, Newschaffer, Yolton, Khoury and Braun2021; Zhang, Manza, & Volkow, Reference Zhang, Manza and Volkow2022), and one study reported that the effects differed according to caffeine source (i.e. an effect for soft drink but not tea or coffee) (Bekkhus, Skjøthaug, Nordhagen, & Borge, Reference Bekkhus, Skjøthaug, Nordhagen and Borge2010). However, a number of other observational studies have reported no meaningful relationship between maternal coffee consumption during pregnancy and offspring NDs (Berglundh et al., Reference Berglundh, Vollrath, Brantsæter, Brandlistuen, Solé-Navais, Jacobsson and Sengpiel2021; Klebanoff & Keim, Reference Klebanoff and Keim2015; Linnet et al., Reference Linnet, Wisborg, Secher, Hove Thomsen, Obel, Dalsgaard and Henriksen2009; Loomans et al., Reference Loomans, Hofland, Van Der Stelt, Van Der Wal, Koot, Van Den Bergh and Vrijkotte2012).
Observational epidemiological studies of maternal coffee/caffeine consumption during pregnancy and offspring neurodevelopment are unlikely to sufficiently control for environmental and genetic confounders. Coffee and caffeine consumption are strongly positively associated with potential confounders such as age, smoking status, alcohol consumption, and negatively with maternal educational attainment (Brice & Smith, Reference Brice and Smith2002; Hewlett & Smith, Reference Hewlett and Smith2006; Papadopoulou et al., Reference Papadopoulou, Botton, Brantsæter, Haugen, Alexander, Meltzer and Sengpiel2018; Torvik et al., Reference Torvik, Eilertsen, McAdams, Gustavson, Zachrisson, Brandlistuen and Ystrom2020; Treur et al., Reference Treur, Taylor, Ware, Mcmahon, Hottenga, Baselmans and Vink2016). Even when these confounders are accounted for, reporting biases and measurement error can render attempts at adjustment insufficient. For example, it has been proposed that while coffee consumption may be accurately reported, stigmatized behaviors such as smoking and drinking alcohol, especially during pregnancy, may be underreported and therefore adjustment may only partially remove their confounding effect (Cornelis & Munafo, Reference Cornelis and Munafo2018). Additionally, genetic confounding may also be an issue for observational studies– where for example, maternal coffee consumption, smoking, and/or alcohol consumption could be linked to maternal neurodevelopmental or psychiatric traits (e.g. ADHD, impulsivity, or anxiety), whose genetic predisposition can then be transmitted to offspring and influence their neurodevelopment (Havdahl et al., Reference Havdahl, Wootton, Leppert, Riglin, Ask, Tesli and Stergiakouli2022; Hvolgaard Mikkelsen et al., Reference Hvolgaard Mikkelsen, Obel, Olsen, Niclasen and Bech2017).
The Mendelian randomization (MR) method is robust to some of the issues faced by traditional observational epidemiological approaches (Davey Smith & Ebrahim, Reference Davey Smith and Ebrahim2003). Following the identification of several genetic variants associated with coffee consumption (Cornelis et al., Reference Cornelis, Byrne, Esko, Nalls, Ganna, Paynter and Walker2015) and caffeine metabolites (Cornelis et al., Reference Cornelis, Kacprowski, Menni, Gustafsson, Pivin, Adamski and Ingelsson2016) in genome-wide association studies (GWAS), MR has been used to investigate the causal effect of coffee/caffeine exposure, outside of and during pregnancy, on both own and offspring outcomes (Brito Nunes et al., Reference Brito Nunes, Huang, Wang, Lundberg, D'Urso, Wootton and Moen2022; Cornelis & Munafo, Reference Cornelis and Munafo2018). This includes the potential causal relationship between maternal caffeine consumption and offspring NDs (Haan et al., Reference Haan, Sallis, Zuccolo, Labrecque, Ystrom, Reichborn-Kjennerud and Munafò2022; Schellhas et al., Reference Schellhas, Haan, Easey, Wootton, Sallis, Sharp and Zuccolo2021). Schellhas and colleagues used maternal polygenic scores (PGS) to assess the causal relationship between maternal caffeine consumption (and smoking) on offspring neuropsychiatric outcomes (autism diagnosis, behavioral problems, and emotional problems across childhood and adolescence) in ~ 7000 mother-child duos in the Avon Longitudinal Study of Parents and Children (ALSPAC) (Schellhas et al., Reference Schellhas, Haan, Easey, Wootton, Sallis, Sharp and Zuccolo2021). They found little evidence of an intrauterine (or offspring mediated) causal effect of maternal caffeine consumption on offspring outcomes. In addition, Haan and colleagues analyzed both ALSPAC (N ~ 8196 mothers) and the Norwegian Mother, Father and Child Cohort Study (early MoBa genetic data release; N ~ 14 584 mothers) and found no strong evidence for a causal effect of maternal smoking, alcohol or caffeine consumption (proxied by maternal PGS) and childhood ADHD symptoms at age 7–8 years (Haan et al., Reference Haan, Sallis, Zuccolo, Labrecque, Ystrom, Reichborn-Kjennerud and Munafò2022).
In this study, we leveraged the world's largest cohort of genotyped parent-offspring trios, the Norwegian Mother, Father and Child Cohort Study (MoBa) (Magnus et al., Reference Magnus, Birke, Vejrup, Haugan, Alsaker, Daltveit and Stoltenberg2016), to investigate the relationship between maternal coffee consumption and a broad range of offspring childhood NDs (46 245 mother-child duos with genetic and phenotypic data available). Firstly, we assessed the observational relationship between maternal coffee consumption (at three time points; before pregnancy, at week 15 and week 22) and offspring NDs, and implemented a paternal-negative control analysis to evaluate the likelihood of postnatal confounding effects (i.e. paternal coffee consumption should not be independently related to offspring neurodevelopment through prenatal pathways). Next, we used a range of MR approaches to investigate whether the observational relationships were likely to be causal. We leveraged the parent-child relationships within MoBa to control for offspring and paternal mediated pleiotropy (i.e. genetic confounding and postnatal mechanisms respectively). We assessed other potential sources of pleiotropy (smoking, alcohol consumption and education) using a series of MR sensitivity analyses. Finally, we conducted a gene by environment (GxE) MR analysis (Chen, Davey Smith, Harbord, & Lewis, Reference Chen, Davey Smith, Harbord and Lewis2008; Davey Smith, Reference Davey Smith2010), where we do not expect to see an effect of maternal genotype on offspring outcomes in mothers who reported no coffee consumption, if there is a true causal effect.
Methods
Cohort description
MoBa is a population-based pregnancy cohort study conducted by the Norwegian Institute of Public Health (Magnus et al., Reference Magnus, Birke, Vejrup, Haugan, Alsaker, Daltveit and Stoltenberg2016). Participants were recruited from all over Norway from 1999–2008. All pregnant women in Norway during this period were eligible for participation in MoBa, resulting in a total of 277 702 invitations sent (Magnus et al., Reference Magnus, Birke, Vejrup, Haugan, Alsaker, Daltveit and Stoltenberg2016, Reference Magnus, Irgens, Haug, Nystad, Skjærven and Stoltenberg2006). The women consented to participation in 41% of the pregnancies. Blood samples were obtained from both parents during pregnancy and from mothers and children (umbilical cord) at birth (Paltiel et al., Reference Paltiel, Anita, Skjerden, Harbak, Bækken, Kristin and Magnus2014). The cohort includes approximately 114 500 children, 95 200 mothers and 75 200 fathers. The current study is based on version 12 of the quality-assured data files released for research in January 2019. MoBa has been linked to the Medical Birth Registry of Norway (MBRN), a national health registry containing information about all births in Norway. The establishment of MoBa and initial data collection was based on a license from the Norwegian Data Protection Agency and approval from The Regional Committees for Medical and Health Research Ethics. The MoBa cohort is currently regulated by the Norwegian Health Registry Act. The current study was approved by The Regional Committees for Medical and Health Research Ethics (2016/1702). This project used MoBa genetic data that was cleaned and imputed as per the MoBaPsychGen pipeline (N = 207 569 individuals passed quality control) (Corfield et al., Reference Corfield, Frei, Shadrin, Rahman, Lin, Athanasiu and Havdahl2022).
Phenotype derivation
MoBa mothers completed ratings of offspring NDs at age 6, 18 and 36 months, 5 and 8 years. The phenotools R package (Hannigan et al., Reference Hannigan, Corfield, Askelund, Askeland, Hegemann, Jensen and Havdahl2023) (v 0.2.2) was used to extract scale scores from ND measures across the MoBa questionnaires, covering a range of domains: language, motor, social communication, behavioral flexibility, attention and hyperactivity. See online Supplementary Materials 1 for a description of the 20 offspring ND measures that were extracted. Mean imputation was used to impute an individual's missing phenotype, when the number of non-missing items for that individual was greater than or equal to 50%. Items were reverse-coded where necessary so that high scores reflected greater difficulties. NDs were rank-based inverse normal transformed.
Three maternal coffee consumption variables were derived from self-reported dietary intake variables in MoBa Questionnaire 1 (administered at gestational week 15; reports of coffee consumption before pregnancy and at week 15) and Questionnaire 2 (week 22). For each timepoint, maternal coffee consumption (cups/day) was calculated from reported intake of filtered, instant and boiled coffees as well as lattes and espressos. Paternal coffee consumption (cups/day) was also derived from self-reports in the Father's Questionnaire (week 15). Maternal and paternal caffeine intake (mg/day) were also calculated using an approach previously described in a MoBa study (Papadopoulou et al., Reference Papadopoulou, Botton, Brantsæter, Haugen, Alexander, Meltzer and Sengpiel2018). In short, multiple caffeine intake variables (mg/day; before pregnancy, week 15 and week 22) were derived by aggregating caffeine from all sources available in the questionnaires (several types of coffee, black and herbal tea, soft drink, and energy drinks) (Papadopoulou et al., Reference Papadopoulou, Botton, Brantsæter, Haugen, Alexander, Meltzer and Sengpiel2018). Individuals who had consumed greater than 3.5L of coffee per day were excluded from all analyses (Papadopoulou et al., Reference Papadopoulou, Botton, Brantsæter, Haugen, Alexander, Meltzer and Sengpiel2018).
Maternal smoking (cigarettes/week) was available at three timepoints (the last 3 months before pregnancy, at week 15 and week 30). Binary smoking (yes/no) variables were also derived for each time point. Maternal alcohol frequency (weekly) was assessed at five timepoints by the question ‘How often did you consume alcohol’ (i.e. times per week; last 3 months before pregnancy; week 0–12 (referred to as week 12), week 15; week 13–24 (referred to as week 24); and week 25 + (referred to as week 30)). Binary alcohol consumption (yes/no) variables were derived for each time point. Socioeconomic variables were extracted from Questionnaire 1. The highest level of education completed by both mothers and fathers was transformed into years of education according to the International Standard Classification of Education (ST1). Maternal and paternal gross yearly incomes in Norwegian Kroner (NOK) were also obtained, and each income bracket was converted to its respective midpoint (ST1). We note that all analyses involving income also included birth year, to account for some of the differing effects of income over time.
Offspring were excluded from analyses if they had congenital birth defects, chromosomal abnormalities, were a part of a multiple birth, as registered in MBRN, or identified as twins found in the KING analysis (Corfield et al., Reference Corfield, Frei, Shadrin, Rahman, Lin, Athanasiu and Havdahl2022; Manichaikul et al., Reference Manichaikul, Mychaleckyj, Rich, Daly, Sale and Chen2010). Individuals who had withdrawn from MoBa at the time of analysis commencement (December 2022) were excluded.
Multiple testing correction threshold
Since the neurodevelopmental trait measures are correlated, we used a principal component analysis (PCA) to estimate the effective number of statistical tests being performed and employed this number in statistical correction for multiple testing. The PCA was performed across 15 719 offspring with complete ND phenotypes available to determine the number of principal components (PCs) that explained >80% of the variance shared between the 20 neurodevelopmental outcomes, consistent with previous research (Havdahl et al., Reference Havdahl, Wootton, Leppert, Riglin, Ask, Tesli and Stergiakouli2022). Ten PCs accounted for 80% of the covariance between traits, suggesting an approximate multiple-testing corrected p-value threshold of p < 0.005 for statistical significance in analyses involving all 20 ND outcomes (i.e. the traditional epidemiological analyses, individual-level MR and two-sample MR analyses). The sensitivity analyses, which were conducted across only one ND, used a less stringent p-value threshold of p < 0.05. Analyses were performed in R using the prcomp function.
Traditional epidemiological analyses
Linear regression analyses were performed to investigate the relationship between the exposure, maternal coffee consumption at three time points (before pregnancy, week 15, week 22), and offspring NDs. The relationship between paternal coffee consumption and offspring NDs was also assessed, as a negative control (i.e. if the negative effects of coffee consumption are mediated by maternal/intrauterine effects then similar associations should not be seen in fathers). Offspring birth year and parental ages at birth were included as covariates in both analyses. All linear regression analyses were conducted using R version 4.1.1.
We ran additional linear regression analyses where we also included additional potential confounders. These were maternal and paternal education, maternal and paternal income, maternal smoking before pregnancy, at week 15 and week 30, maternal alcohol consumption before pregnancy, at week 12, week 15, week 24, and week 30. By including smoking and alcohol related variables, this model attempts to remove any direct confounding effect of those variables as well as the potential confounding effect of maternal impulsivity (i.e. genetic confounding) (Havdahl et al., Reference Havdahl, Wootton, Leppert, Riglin, Ask, Tesli and Stergiakouli2022). We also included binary (yes/no) variables for maternal smoking and alcohol consumption at each time point.
In a separate model, we attempted to isolate the effect of maternal coffee consumption during pregnancy (i.e. the intrauterine effect) by controlling for maternal coffee consumption before pregnancy. This model included the covariates maternal coffee consumption before pregnancy, offspring birth year, maternal age at birth, paternal age at birth, maternal smoking before pregnancy, at week 15, and week 30, maternal alcohol before pregnancy, at week 15, week 24, and week 30, maternal and paternal income, maternal and paternal education, and offspring genotyping batch. We also included binary variables for maternal smoking and alcohol consumption at each timepoint.
Similar analyses were conducted in the genotyped subset of MoBa using a genetic linear mixed model approach that is more robust to the effects of cryptic relatedness and population structure (see online Supplementary Materials 2).
Mendelian randomization analyses
Individual-level and Two-Sample MR analyses were performed to assess the causal nature of the relationship between maternal coffee consumption during pregnancy and offspring NDs. Power calculations for these analyses are presented in online Supplementary Materials 3.
Genetic variant selection
Eight independent genome-wide significant genetic variants that have been previously associated with coffee consumption (Cornelis et al., Reference Cornelis, Byrne, Esko, Nalls, Ganna, Paynter and Walker2015) (log10Bayes-factor>5.64, ST2) were aggregated into weighted and unweighted polygenic scores (PGS) to be used in the MR analyses.
Benchmarking checks
We assessed whether the coffee PGS and individual SNPs were associated with maternal coffee consumption before and during pregnancy in MoBa while adjusting for offspring birth year, parental ages at birth, and maternal genotyping batch using a genetic linear mixed model. A maternal GRM was included in the random effects part of the model.
Individual-Level MR analyses
In the present study, we used genetic association analyses to inform on potential causal relationships, and these analyses are hereafter referred to as ‘individual-level MR analyses’. We assessed whether maternal weighted and unweighted PGS for coffee consumption were associated with offspring NDs using a genetic linear mixed model. This approach was chosen to account for cryptic relatedness and genetic confounding (see Discussion). The model incorporated an offspring GRM from all genotyped and imputed autosomal loci, excluding the eight coffee variants and 1 MB either side of these variants (to avoid modelling the same signal in both the fixed and random effect part of the model). The unweighted PGS analyses included terms for offspring unweighted PGS, offspring birth year, parental ages at birth, and both offspring and maternal genotyping batches. The offspring unweighted PGS was included as a covariate to block potential pleiotropic pathways through the offspring genome (D'Urso et al., Reference D'Urso, Wang, Hwang, Moen, Warrington and Evans2021; Lawlor et al., Reference Lawlor, Richmond, Warrington, McMahon, Davey Smith, Bowden and Evans2017). The weighted PGS analyses conditioned upon offspring genotype (at all loci) rather than the PGS, to fully block potential pleiotropic pathways through the offspring genome.
We ran MR sensitivity analyses in the smaller subset of parent-offspring trios. These analyses were conducted to investigate the potential collider pathway introduced in the mother-child duo analyses when conditioning on offspring genome, but not the paternal genome, if a postnatal (paternal) pathway from paternal genotype to offspring NDs were present. Here, we assessed whether maternal weighted (or unweighted) PGS for coffee consumption were associated with offspring NDs using a genetic linear mixed model, while adjusting for offspring genotype (or unweighted PGS), paternal genotype (or unweighted PGS), offspring birth year, parental ages at birth, and all genotyping batches. We also estimated the effect of the paternal PGS conditional on offspring genome, maternal genome, offspring birth year, parental ages at birth, and all genotyping batches. This analysis served as a negative control, allowing us to evaluate the presence of a postnatal (confounding) effect of coffee consumption on offspring NDs.
Two-sample MR analyses
The Inverse Variance Weighted (IVW) Two-Sample MR approach was applied to investigate the relationship between maternal coffee consumption and offspring NDs (Burgess, Butterworth, & Thompson, Reference Burgess, Butterworth and Thompson2013). SNP-exposure data were extracted from the external GWAS of coffee consumption (Cornelis et al., Reference Cornelis, Byrne, Esko, Nalls, Ganna, Paynter and Walker2015) (ST2).
SNP-outcome data for the Two-Sample MR analyses (as well as the multivariable MR analyses; see below) came from our own analyses within the MoBa cohort. For analyses of maternal exposures on offspring outcomes, we require estimates of the effect of the maternal genotype on offspring outcome, with the effect of the offspring genotype removed. Therefore, maternal and offspring GWAS of the ND outcomes were conducted and the genetic effects were then partitioned to provide estimates of the maternal-SNP-outcome effect. The GWAS were implemented using the fastGWA linear mixed model approach (Jiang et al., Reference Jiang, Zheng, Qi, Kemper, Wray, Visscher and Yang2019). A GRM of all mothers and offspring was generated and converted into a sparse GRM before being included in the maternal and offspring GWAS. We included offspring birth year, parental age at birth, and ten offspring and maternal genetic PCs as covariates. The maternal GWAS of NDs were limited to one pregnancy per mother (first-born child in MoBa). The maternal and offspring genetic effects on each ND were partitioned using the Direct and INdirect effects analysis of Genetic lOci (DINGO) approach (Hwang et al., Reference Hwang, Cuellar-Partida, Yengo, Zeng, Beaumont, Freathy and Evans2023). The effective sample overlap between the offspring and maternal GWAS for DINGO was estimated using bivariate linkage disequilibrium (LD) score regression and the 1000 Genomes Project European reference panel (Bulik-Sullivan et al., Reference Bulik-Sullivan, Finucane, Anttila, Gusev, Day, Loh and Neale2015a, Reference Bulik-Sullivan, Loh, Finucane, Ripke, Yang and Neale2015b) (see ST3 for GWAS sample sizes and bivariate LD score regression estimates used for partitioning the genetic effects).
Two Sample MR analyses were performed using the TwoSampleMR package (Hemani et al., Reference Hemani, Zheng, Elsworth, Wade, Haberland, Baird and Haycock2018) (https://github.com/MRCIEU/TwoSampleMR) in R version 4.1.1 (https://cran.r-project.org/). Sensitivity analyses were performed using the MR-Egger (Bowden, Davey Smith, & Burgess, Reference Bowden, Davey Smith and Burgess2015), Weighted Median (Bowden, Davey Smith, Haycock, & Burgess, Reference Bowden, Davey Smith, Haycock and Burgess2016), Simple Mode and Weighted Mode (Hartwig, Davey Smith, & Bowden, Reference Hartwig, Davey Smith and Bowden2017) methodologies. Heterogeneity tests of the causal effect estimates were conducted using Cochran's Q. Directional pleiotropy was assessed through the MR–Egger intercept. I2GX was calculated to evaluate the risk for weak instrument bias in the MR-Egger analyses. Exposure and outcome GWAS summary statistics are provided in ST4.
Investigations into pleiotropy
Several additional sensitivity analyses were performed to investigate potential pleiotropic effects of the SNPs and PGS used in the MR analyses (i.e. violations of MR assumptions). Firstly, we examined whether coffee SNPs and PGS were associated with maternal alcohol consumption (amongst consumers), smoking (amongst smokers), education and income, as well as binary (yes/no) variables for smoking and alcohol consumption. These analyses were performed using GCTA and adjusted for offspring birth year, parental ages at birth and maternal genotyping batch. If associations were identified, we performed additional MR analyses to control for the potential confounders. Firstly, additional individual-level MR analyses were repeated in mother-child duos using weighted PGS, this time adjusting for variables that the coffee PGS were associated with (as well as offspring genome, offspring birth year, parental ages at birth and genotyping batches). Secondly, multivariable IVW MR (MVMR) was employed to estimate the direct causal effect of maternal coffee exposure on offspring NDs, conditional on smoking heaviness and alcohol frequency. Educational attainment was not included in the MVMR (see Discussion). Genetic instrumental variables for smoking heaviness (cigarettes/day) and alcohol frequency (weekly) were identified in the ancestry-stratified GWAS meta-analyses of Europeans (excluding 23&Me) (Saunders et al., Reference Saunders, Wang, Chen, Jang, Liu, Wang and Project2022). Summary statistics were clumped (p < 5 × 10−8, r2 = 0.001), and palindromic SNPs were removed, resulting in 17 and 48 SNPs for smoking and alcohol frequency (that were available across all exposure and outcome GWAS data) respectively. Coffee consumption was proxied by the aforementioned genetic variants. The maternal genetic effects on offspring ND outcomes were used for the outcome data. MVMR analyses were performed using the TwoSampleMR package and the input summary statistics are provided in ST5.
Gene by environment interaction MR
The GxE MR framework (Chen et al., Reference Chen, Davey Smith, Harbord and Lewis2008; Davey Smith, Reference Davey Smith2010) was also utilized as a sensitivity analysis, where two additional individual-level MR analyses were performed in subgroups stratified by coffee consumption status during pregnancy. Consumers were defined as women who had reported consuming coffee in the week 15 or week 22 Questionnaire (N = 35 250 mothers), while never consumers were defined as those who reported no coffee consumption across both timepoints (N = 8544 mothers). In order to investigate the possibility of introducing collider bias to these analyses when conditioning on coffee consumption (see Discussion), genetic variants were tested for association with ever/never consuming coffee during pregnancy using a genetic linear mixed model in GCTA (N = 43 794). This model adjusted for offspring birth year, maternal age at birth, and maternal genotyping batch, and included a GRM. Any variants significantly associated with ever/never consuming coffee were excluded from the weighted PGS used in the GxE MR. The GxE MR analyses assessed whether maternal weighted PGS for coffee consumption were associated with offspring NDs (amongst ever consumers and never consumers) using the previously described genetic linear mixed model (i.e. while adjusting for offspring genotype, offspring birth year, parental ages at birth, and maternal and offspring genotyping batches) and included a GRM. A heterogeneity test was conducted to compare results from the consumer and non-consumer stratified analyses.
Results
Descriptive characteristics of the MoBa cohort after QC are presented in Table 1. Statistical power to detect causal effect estimates in the present study is shown in online Supplementary Materials 3.
N, Sample size; s.d., Standard deviation; NOK, Norwegian Kroner; SCQ-full, Social Communication Questionnaire; SCQ-RRB, Social Communication Questionnaire restricted and repetitive behavior subscale; SCQ-SCI, Social Communication Questionnaire social communication impairment subscale; CBCL-ADHD, Child Behavior Checklist ADHD subscale; RS-DBD-ADHD: Rating Scale for Disruptive Behavior Disorders ADHD subscale; RS-DBD-INA, Rating Scale for Disruptive Behavior Disorders inattention subscale; RS-DBD-HYP, Rating Scale for Disruptive Behavior Disorders hyperactivity subscale; CPRS: Conners Parent Rating Scale-Revised short form; ASQ-LANG, Ages and Stages Questionnaire language subscale; CCC-S, The Children's Communication Checklist-2 Short Scale; ASQ-MOTOR, Ages and Stages Questionnaire motor items; CDI-MOTOR, Child Development Inventory motor subscale.
*non-whole number due to converting weekly consumption to daily.
**non-whole number due to converting monthly consumption to weekly.
Traditional epidemiological analyses
The unadjusted traditional observational analyses (i.e. not adjusting for smoking/alcohol/education/income) found strong evidence for positive associations between maternal coffee consumption and several measures related to offspring difficulties with social communication and behavioral flexibility (Fig. 1; p < 0.005). Likewise, there was strong evidence of positive associations between maternal coffee consumption and all offspring difficulties with attention and hyperactive-impulsive behavior (Fig. 1; p < 0.005). There was also some evidence for positive associations between maternal coffee consumption and language difficulties at ages 18 months, 3 years, and 8 years (Fig. 1; p < 0.005). Interestingly, negative associations were observed between maternal coffee consumption and language difficulties at age 5 and motor difficulties at age 3 (Fig. 1; p < 0.005). There was little evidence that paternal coffee consumption was associated with the NDs, apart from social communication difficulties at age 3 years (p < 0.005; negative association).
The results from the observational analyses that adjusted for education, income, smoking and alcohol related variables can be found in online Supplementary Materials 4. Many of the previously significant effects attenuated towards zero and some associations switched from being positive to negative. Significant effects only remained for social communication and behavioral flexibility difficulties at age 3, difficulties with attention and hyperactive-impulsive behavior at age 5, and motor difficulties at age 3 (p < 0.005).
When adjusting for maternal coffee consumption before pregnancy, we observed significant negative associations between maternal coffee consumption during pregnancy and offspring difficulties with social communication and behavioral flexibility at age 3, difficulties with attention and hyperactive-impulsive behavior at age 5, and motor difficulties at age 3 (online Supplementary Materials 5; p < 0.005).
Online Supplementary Materials 2 shows similar results for the observational analyses conducted in the genotyped MoBa sample.
Mendelian randomization analyses
Benchmarking checks
Benchmarking analyses found that both the weighted and unweighted maternal PGS for coffee consumption were positively associated with self-reported maternal coffee consumption in MoBa across all timepoints (ST6; p < 0.05). As for the individual SNPs, all except for rs1481012 (ABCG2), showed evidence for positive association with coffee consumption for at least one time point in MoBa (ST7; p < 0.05). Likewise, the I2GX and F statistics for individual SNPs and PGS are given in ST8 and ST9, respectively (all F > 10 and I2GX > 0.9). Together, this suggests that the GRS are appropriate genetic instrumental variables for maternal coffee consumption during pregnancy and that weak instrument bias is unlikely to be an issue.
Individual-Level MR analyses
The mother-child duo individual-level MR analyses found some evidence for association between PGS for increased coffee intake and offspring NDs (Table 2). The weighted PGS was positively associated with social communication difficulties at age 8 years (beta = 0.128; se = 0.043, p = 0.003), although there was little evidence for association between the unweighted PGS and any of the outcomes (Table 2).
p < 0.05 = bold, p < 0.005 = *
PGS, polygenic score; SE, standard error; p, P-value; SCQ-full, Social Communication Questionnaire; SCQ-RRB, Social Communication Questionnaire restricted and repetitive behavior subscale; SCQ-SCI, Social Communication Questionnaire social communication impairment subscale; CBCL-ADHD, Child Behavior Checklist ADHD subscale; RS-DBD-ADHD, Rating Scale for Disruptive Behavior Disorders ADHD subscale; RS-DBD-INA, Rating Scale for Disruptive Behavior Disorders inattention subscale; RS-DBD-HYP, Rating Scale for Disruptive Behavior Disorders hyperactivity subscale; CPRS, Conners Parent Rating Scale-Revised short form; ASQ-LANG, Ages and Stages Questionnaire language subscale; CCC-S, The Children's Communication Checklist-2 Short Scale; ASQ-MOTOR, Ages and Stages Questionnaire motor items; CDI-MOTOR, Child Development Inventory motor subscale.
The parent-child trio analyses (ST10) found some evidence that maternal PGS were associated with difficulties with attention and hyperactive-impulsive behavior (beta = −0.131, se = 0.044, p = 0.003) and language difficulties at 18 months (beta = −0.009, se = 0.003, p = 0.004). In contrast, there was little evidence for association between paternal PGS and offspring NDs in the negative control analyses in parent-child trios (ST11; all p > 0.005).
Two-sample MR analyses
The IVW MR analyses found a suggestive positive association (Table 3; p < 0.05) between coffee consumption and social communication difficulties at age 8 (beta = 0.348, se = 0.141; p = 0.014).
p < 0.05 bolded
SE, standard error; p, P-value; SCQ-full, Social Communication Questionnaire; SCQ-RRB, Social Communication Questionnaire restricted and repetitive behavior subscale; SCQ-SCI, Social Communication Questionnaire social communication impairment subscale; CBCL-ADHD, Child Behavior Checklist ADHD subscale; RS-DBD-ADHD, Rating Scale for Disruptive Behavior Disorders ADHD subscale; RS-DBD-INA, Rating Scale for Disruptive Behavior Disorders inattention subscale; RS-DBD-HYP, Rating Scale for Disruptive Behavior Disorders hyperactivity subscale; CPRS, Conners Parent Rating Scale-Revised short form; ASQ-LANG, Ages and Stages Questionnaire language subscale; CCC-S, The Children's Communication Checklist-2 Short Scale; ASQ-MOTOR, Ages and Stages Questionnaire motor items; CDI-MOTOR, Child Development Inventory motor subscale.
Sensitivity analyses
To avoid over-interpretation of results, sensitivity analyses were focused upon NDs where there was some evidence (p < 0.005) of association in the main individual-level MR and two-sample MR analyses (i.e. social communication difficulties at age 8 years; SCI-SCI-8 yr).
Two-sample MR sensitivity analyses
The Weighted Median and Weighted Mode MR analyses all showed evidence for a positive causal effect between maternal coffee consumption and offspring social communication difficulties at age 8 years (weighted median: beta 0.366, se = 0.152, p = 0.016; weighted mode: beta = 0.386, se = 0.153, p = 0.040), while the MR-Egger and Simple Mode did not (ST12; Egger: beta = 0. 510, se = 0.300 p = 0.140; simple mode: beta = 0.386, se = 0.238, p = 0.149). There was no evidence of significant directional pleiotropy or heterogeneity for MR analyses of social communication difficulties at age 8 years (p > 0.05; ST13).
Investigation into pleiotropy
The coffee consumption increaser allele of rs9902453 (G; EFCAB5), was found to be nominally associated with maternal smoking intensity (ST14; Week 15: beta = 1.543, se = 0.608, p = 0.011; Week 30: beta = 1.763, se = 0.689, p = 0.010) and rs1481012 (G; ABCG2), rs4410790 (C; AHR) and rs6265 (C; BDNF) were associated with binary smoking (respectively; OR = 0.994, se = , 9, p = 0.017; OR = 0.997, se = 0.002, p = 0.029; OR = 1.007, se = 0.004, p = 0.046). The increaser allele of rs4410790 (C; AHR) and rs2472297 (T; CYP1A2) were positively associated with maternal alcohol consumption (ST15; Week 30: beta = 0.020, se = 0.007, p = 0.007 and week 30: OR = 1.005, se = 0.002, p = 0.037), while interestingly the increaser allele of a number of SNPs showed a decreased odds of initiation (rs4410790, rs1260326 and rs9902453; p < 0.05 at multiple time points). We found the increaser allele of one SNP rs1260326 (C; GCKR) was negatively associated with education (ST16; beta = −0.029, se = 0.014, p = 0.035) and income (ST16; beta = −1462.350, se = 675.261, p = 0.030).
Nominally significant positive associations were observed between the weighted PGS and maternal alcohol consumption at week 30 (ST17; beta = 0.067, se = 0.032, p = 0.039). The unweighted PGS was positively associated with smoking at week 15 (ST18; beta = 0.563, se = 0.244, p = 0.021) and education (ST19; beta = 0.017, se = 0.009, p = 0.043), and a decreased risk of smoking (yes v. no) at week 30 (ST18; beta = −0.002, se = 0.001, p = 0.023) and alcohol consumption (yes v. no) (ST17; week 12: beta = −0.003, se = 0.001, p = 0.004; week 24: beta = −0.002, se = 0.001, p = 0.007; week 30: beta = −0.002, se = 0.001, p = 0.043). No PGS were associated with income (ST19).
The individual-level MR analyses that adjusted for potential confounding variables showing association with the PGS (smoking, alcohol and education), found the weighted coffee PGS no longer showed significant evidence for association with social communication difficulties at age 8 years (ST20; beta = 0.088, se = 0.049, p = 0.071). The MVMR analysis including coffee consumption, smoking and alcohol consumption, found coffee consumption was independently and positively associated with social communication difficulties at age 8 years (ST21; beta = 0.37, se = 0.13, p = 0.004).
Gene by environment interaction MR
One genetic variant (rs78000944; MLXIPL) was significantly associated with ever/never consuming coffee during pregnancy (ST22; OR = 1.009, se = 0.003, p = 0.002), and was therefore excluded from the PGS used in the GxE MR. The GxE MR analyses found weak evidence for a positive association between coffee consumption and social communication difficulties at age 8 years amongst mothers who consumed coffee during pregnancy (beta = 0.153, se = 0.071, p = 0.032, N = 16 471). Although not statistically significant, we also detected a positive effect of similar magnitude amongst mothers who did not consume coffee during pregnancy (beta = 0.107, se = 0.134, p = 0.424, N = 4304). There was no evidence of heterogeneity in the consumer and non-consumer GxE MR effect estimates (p = 0.619).
Discussion
This study utilized data from a large cohort of genotyped parent-offspring trios to investigate the relationship between maternal coffee consumption and offspring childhood NDs. Our observational analyses, which did not adjust for potential confounders, found that increased maternal coffee consumption was associated with many offspring NDs. However, after adjusting for potential confounders (maternal smoking, maternal alcohol consumption, parental education, and parental income), the previously significant effects of maternal coffee consumption on offspring ND outcomes attenuated towards zero. Our findings agree with previous observational work conducted within an earlier, but much smaller version of MoBa (version 8 released in 2015; Berglundh et al., Reference Berglundh, Vollrath, Brantsæter, Brandlistuen, Solé-Navais, Jacobsson and Sengpiel2021), which included similar outcomes (excluding the Social Communication Questionnaire and the Conners Parent Rating Scale) and covariates.
Our MR analyses found little evidence for a causal effect between maternal coffee consumption and most offspring NDs. Although we observed a significant positive association with social communication difficulties at age 8 years, we were unable to confidently rule out the possibility of pleiotropic pathways driving this association. Importantly, the proposed mechanisms of action for SNPs associated with coffee consumption is highly heterogeneous, with possible roles spanning caffeine metabolism, reward response, taste perception, and additional unknown processes, and may therefore invalidate one of the core MR assumptions (i.e. exclusion restriction assumption) (Brito Nunes et al., Reference Brito Nunes, Huang, Wang, Lundberg, D'Urso, Wootton and Moen2022; Cornelis & Munafo, Reference Cornelis and Munafo2018). Although we did not detect pleiotropy in our MR sensitivity analyses, we took precautions to address this potential issue. Since many of the SNPs/PGS showed evidence for association with potential confounders (smoking/alcohol/education) in MoBa, we conducted additional individual-level MR analyses, that adjusted for these variables. Here, we found that the effect between coffee consumption and social communication difficulties at age 8 years weakened and was no longer significant.
We also attempted to genetically proxy potential confounders. The MVMR analyses found that coffee consumption was significantly associated with social communication difficulties at age 8 years, independent of smoking and alcohol consumption. However, we omitted educational attainment from the MVMR analyses, to avoid potential bias in the MR results stemming from using variants known to be subject to population stratification (Haworth et al., Reference Haworth, Mitchell, Corbin, Wade, Dudding, Budu-Aggrey and Timpson2019), assortative mating (Domingue, Fletcher, Conley, & Boardman, Reference Domingue, Fletcher, Conley and Boardman2014; Howe, Nivard, et al., Reference Howe, Nivard, Morris, Hansen, Rasheed, Cho and Consortium2022; Robinson et al., Reference Robinson, Kleinman, Graff, Vinkhuyzen, Couper and Miller2017; Yengo et al., Reference Yengo, Robinson, Keller, Kemper, Yang, Trzaskowski and Visscher2018), and involve indirect genetic effects (Howe, Evans, Hemani, Davey Smith, & Davies, Reference Howe, Evans, Hemani, Davey Smith and Davies2022; Howe, Nivard, et al., Reference Howe, Nivard, Morris, Hansen, Rasheed, Cho and Consortium2022; Kong et al., Reference Kong, Thorleifsson, Frigge, Vilhjalmsson, Young, Thorgeirsson and Stefansson2018; Lee et al., Reference Lee, Wedow, Okbay, Kong, Maghzian, Zacher and Consortium2018; Wang et al., Reference Wang, Baldwin, Schoeler, Cheesman, Barkhuizen, Dudbridge and Pingault2021), rather than direct genetic effects (Howe et al., Reference Howe, Rasheed, Jones, Boomsma, Evans, Giannelis and Davies2023). While these findings provide some evidence for a causal effect of coffee consumption, it is possible that education (whose association with child ADHD symptoms persists after controlling for shared genetic and family environmental factors (Torvik et al., Reference Torvik, Eilertsen, McAdams, Gustavson, Zachrisson, Brandlistuen and Ystrom2020)) or some other non-modelled confounding variable, could be driving the association.
In presence of a true causal effect of maternal coffee consumption on offspring NDs, we expected our GxE MR analyses to detect an effect only amongst coffee consumers, and not in the non-consumers. Our analyses found a causal effect of similar magnitude in both the consumers and non-consumers, suggesting that pleiotropy may be driving the association between maternal coffee consumption and social communication difficulties at age 8 years. It is worth noting that the proportion of mothers abstaining from coffee within the MoBa dataset is small, consistent with Norway's high coffee consumption rates (International Coffee Council, 2012; Lukic et al., Reference Lukic, Barnung, Skeie, Olsen and Braaten2020), leading to larger standard errors and reduced statistical power in the ‘never consuming’ analysis, possibly explaining why the effect (of similar magnitude) was non-significant in this group. Furthermore, coffee consumption may be a collider (Cornelis & Munafo, Reference Cornelis and Munafo2018) and conditioning upon consumption in the GxE MR analyses may have introduced a path between the genetic instrumental variables and confounders of the exposure outcome relationship (online Supplementary Materials 6). We attempted to minimize this effect by excluding SNPs associated with ever/never consuming coffee during pregnancy in MoBa, however it is possible that the remaining variants could also be associated with ever/never consuming coffee. In addition, it is possible that mothers who drink coffee may be systematically different from mothers who don't in terms of how they report symptoms in their children, and the GxE MR framework is not robust to this.
Unlike traditional observational approaches, our within-family MR is robust to some forms of genetic confounding. For example, if a SNP relates to maternal coffee consumption, maternal ADHD and offspring NDs, the effect of an offspring inheriting that SNP is accounted for through inclusion of offspring genotype in the same model (i.e. essentially blocking the path from maternal to offspring genome). Indeed, a study has shown that pregnant individuals with high ADHD genetic liability are at increased risk of adverse pregnancy-related exposures (such as smoking during pregnancy), which have been linked to offspring neurodevelopmental outcomes (Havdahl et al., Reference Havdahl, Wootton, Leppert, Riglin, Ask, Tesli and Stergiakouli2022), necessitating genetically informative methods to disentangle the complicated relationships between variables.
Importantly, we note that the weightings used in the MR analyses were derived from a GWAS of non-pregnant individuals, and consequently may not accurately reflect effect sizes in pregnant women. Our benchmarking analyses found that the SNPs and PGS were generally positively associated with coffee consumption during pregnancy in MoBa. This mirrors results from a previous study that found the same PGS were positively associated with coffee consumption at week 32 of gestation in the ALSPAC cohort (Brito Nunes et al., Reference Brito Nunes, Huang, Wang, Lundberg, D'Urso, Wootton and Moen2022). While this shows our instruments can proxy coffee consumption during pregnancy, the weightings may not be accurate. Therefore, rather than focusing on the magnitude of the causal effect estimates, we suggest that the presence/absence and direction of the effect may be more informative.
Notably, our MR analyses had limited statistical power, due to the PGS explaining minimal variance in coffee consumption. We attempted to increase statistical power by including six additional SNPs previously associated with coffee consumption in a large US/UK GWAS (Zhong et al., Reference Zhong, Kuang, Danning, Kraft, van Dam, Chasman and Cornelis2019) (N = 672 357), however these SNPs were not strongly or consistently associated with coffee consumption in MoBa (ST23). This difference may be due to differences in study populations (UK v. Norwegian), who may differ in their coffee consumption behavior (i.e. Norwegian preference to coffee, and a UK preference for tea). Therefore, these SNPs may not accurately capture the effect of coffee consumption in MoBa, rendering them unsuitable for this study.
There are several future study directions. This study focused on the effect of maternal coffee consumption on offspring difficulties with language, motor skills, social communication, behavioral flexibility, attention, and hyperactivity. The NDs were reported by the mothers and therefore may be subject to certain reporting biases. Consequently, it would be beneficial if future studies investigated clinical assessments, cognitive tests, and teacher ratings of offspring neurodevelopmental traits. Likewise, the effects of maternal coffee consumption on offspring neurodevelopmental disorder diagnoses should also be examined. Many other aspects of coffee consumption are also worth exploring. Our study did not explore whether the effects of maternal coffee consumption act during critical-periods, and we did not directly investigate caffeine, a likely mediator of a potential relationship between maternal coffee consumption and offspring outcomes. However, we observed strong positive associations between maternal (coffee) PGS/SNPs and caffeine intake (ST6 and ST7), suggesting that caffeine may also be proxied by the instruments used in the present study. Investigating the impact of various caffeine sources, such as soft drink and tea, on offspring outcomes is also relevant, as past observational studies have linked maternal soft drink consumption, rather than tea or coffee/caffeine, to childhood NDs (Bekkhus et al., Reference Bekkhus, Skjøthaug, Nordhagen and Borge2010; Berglundh et al., Reference Berglundh, Vollrath, Brantsæter, Brandlistuen, Solé-Navais, Jacobsson and Sengpiel2021). We did not investigate dose-dependent effects or the influence of particular caffeine metabolites (i.e. theobromine, theophylline, paraxanthine). This may be relevant, as a previous observational study examining maternal serum paraxanthine concentrations and childhood cognitive and behavioral outcomes (at ages 4 and 7 years) found little evidence of an adverse association for the majority of pregnant women consuming moderate amounts of caffeine (Klebanoff & Keim, Reference Klebanoff and Keim2015). Importantly, coffee contains many bioactive compounds other than caffeine (e.g. chlorogenic acid, trigonelline, cafestol, kahweol) (Socała, Szopa, Serefko, Poleszak, & Wlaź, Reference Socała, Szopa, Serefko, Poleszak and Wlaź2020; Spiller, Reference Spiller and Spiller2019), which may impact neurodevelopment. As more genetic variants associated with caffeine consumption/metabolism become available, it may be possible to investigate these questions using MR. Lastly, our work was conducted in the MoBa cohort, which may not be representative of other populations, and similar analyses should be conducted in cohorts of different ancestries and ethnicities.
In conclusion, this study applied several conventional and genetic epidemiological approaches to investigate the potential relationship between maternal coffee consumption during pregnancy and offspring NDs. When considering the results of the conventional and genetic epidemiological analyses, and also the broader literature, we conclude that there is little evidence that maternal coffee consumption during pregnancy is strongly causally related to offspring NDs.
Supplementary material
The supplementary material for this article can be found at https://doi.org/10.1017/S0033291724002216.
Data
Data from the Norwegian Mother, Father and Child Cohort Study and the Medical Birth Registry of Norway used in this study are managed by the national health register holders in Norway (Norwegian Institute of Public Health) and can be made available to researchers, provided approval from the Regional Committees for Medical and Health Research Ethics (REC), compliance with the EU General Data Protection Regulation (GDPR) and approval from the data owners. The consent given by the participants does not open for storage of data on an individual level in repositories or journals. Researchers who want access to data sets for replication should apply through helsedata.no. Access to data sets requires approval from The Regional Committee for Medical and Health Research Ethics in Norway and an agreement with MoBa.
Acknowledgements
The Norwegian Mother, Father and Child Cohort Study is supported by the Norwegian Ministry of Health and Care Services and the Ministry of Education and Research. We are grateful to all the participating families in Norway who take part in this on-going cohort study. We thank the Norwegian Institute of Public Health (NIPH) for generating high-quality genomic data. This research is part of the HARVEST collaboration, supported by the Research Council of Norway (#229624). We also thank the NORMENT Centre for providing genotype data, funded by the Research Council of Norway (#223273), South East Norway Health Authorities and Stiftelsen Kristian Gerhard Jebsen, in collaboration with deCODE Genetics. We further thank the Center for Diabetes Research, the University of Bergen for providing genotype data funded by the ERC AdG project SELECTionPREDISPOSED, Stiftelsen Kristian Gerhard Jebsen, Trond Mohn Foundation, the Research Council of Norway, the Novo Nordisk Foundation, the University of Bergen, and the Western Norway Health Authorities.
This work was performed on the TSD (Tjeneste for Sensitive Data) facilities, owned by the University of Oslo, operated and developed by the TSD service group at the University of Oslo, IT Department (USIT). (tsd-drift@usit.uio.no). The analyses were performed on resources provided by Sigma2 - the National Infrastructure for High-Performance Computing and Data Storage in Norway.
SD is supported by an Australian Government Research Training Program (RTP) Scholarship.
LDH is the recipient of an Australian Research Council Discovery Early Career Award (Project number: DE240100014).
GHM is the recipient of an Australian Research Council Discovery Early Career Award (Project number: DE220101226) funded by the Australian Government and supported by the Research Council of Norway (Project grant: 325640). This work was supported by the Nils Normanns mindefond.
AH was supported by the South East Norway Regional Health Authority (grant #2020022, #2021045), the Research Council of Norway (#274611, #336085) and the European Union's Horizon Europe Research and Innovation Programme (FAMILY, grant agreement No 101057529).
REW was supported by the South East Norway Regional Health Authority (grant # 2020024).
DME is supported by an NHMRC Investigator Grant (APP2017942). This work was supported by Australian National Health and Medical Research Council (NHMRC) grants (GNT1183074, GNT1157714).
Author contributions
SD, LDH, GHM, DME, and AH conceived and designed the study. SD and REW curated the data. SD analyzed the data and wrote the original draft. SD, LDH, GHM, DME and AH interpreted the results. GHM, LDH, DME and AH supervised the work. All authors critically reviewed the manuscript and approved the final version of the manuscript. SD, GHM, and AH had access to the data and verified the analyses. All authors could access the data on request.
Disclosures
The authors declare no competing interests. The funding sources had no involvement in study design, data collection, data analysis, interpretation, or writing of the report. Views and opinions expressed are those of the author(s) and do not necessarily reflect those of the European Union or the European Research Executive Agency (REA). Neither the European Union nor the granting authority can be held responsible for them.