Sample

We employ two samples in our study. Our primary sample is the CHDS, which is an ongoing birth cohort of 1265 children born in the Christchurch (New Zealand) urban region in mid-1977. Participants have been studied on a total of 23 occasions from birth to age 35 years.Reference Fergusson, Horwood, Joyce, Nicholls, Thomas and Wilkinson^13, Reference Fergusson and Horwood¹⁴ The present analysis is based on data collected during assessments on the cohort at ages 21, 25, 30 and 35 years. Sample retention rates have remained high throughout the course of the study and, at age 35, the study was still able to assess 79% of the surviving cohort. Participant consent was obtained for all forms of data collection and all phases of the study have been subject to ethical approval. Ethical approvals relevant to the current research are from the Southern Health and Disability Ethics Committee (ref CTB/04/11/234/AM09, 16/STH/188/AM01).

We also employed the ALSPAC (www.bris.ac.uk/alspac/), which is a birth cohort study based on children born in South West England (Avon) between 1 April 1991 and 31 December 1992.Reference Boyd, Golding, Macleod, Lawlor, Fraser and Henderson⁹ Participants were not randomly selected, but the demographic characteristics of ALSPAC have been shown to be representative of the UK as a whole.Reference Boyd, Golding, Macleod, Lawlor, Fraser and Henderson⁹ The resource comprises a wide range of phenotypic and environmental measures in addition to biological samples, genetic (DNA on 11 343 children, genome-wide data on 8365 children and complete genome sequencing on 2000 children) and epigenetic (methylation sampling on 1000 children) information, and linkage to health and administrative records. The study website contains details of all the data, searchable through the data dictionary (www.bris.ac.uk/alspac/researchers/data-access/data-dictionary/). This study received ethical approval from the ALSPAC Law and Ethics Committee and Local Research Ethics Committees (http://www.bristol.ac.uk/alspac/researchers/research-ethics/).

DNA extraction and genotyping

In the CHDS sample, individuals between the ages of 28–30 years provided a DNA sample for genetic analysis. In 91.4% of cases, DNA was extracted from whole blood; for the remaining participants (8.6%), saliva was collected using Oragene Collection Kits (DNA Genotek, Ottawa, Canada) and DNA was extracted according to the supplier's instructions. DNA extractions were completed at the Gene Structure and Function Laboratory, based at the University of Otago, Christchurch, New Zealand.Reference Fergusson, Horwood, Miller and Kennedy¹⁶ Available samples were genotyped using Illumina Human660W-Quad v1 DNA Analysis BeadChips at the Mayo Clinic.Reference Adkins, Clark, Copeland, Kennedy, Conway and Angold¹⁵

Full details of sample and variant quality control are given in Supplementary Text and Supplementary Table 1 available at https://doi.org/10.1192/bjp.2018.227. Genotypes were imputed using the 1000 Genomes Phase 3 data set as a reference panel (see Supplementary Text). Principal component analysis was performed to produce population principal components for use as covariates in further analyses. The data set from which the risk alleles are derived are overwhelmingly of European ancestry so to maximise power and avoid confounding,Reference Martin, Gignoux, Walters, Wojcik, Neale and Gravel¹⁷ analyses were limited to individuals of European ancestry as defined by genomic similarity to the European reference samples represented in the 1000 Genomes data set.¹⁸

PRS construction

The PRS is a summary score of the number of risk alleles carried by an individual, weighted according to their effect sizes, where risk allele and effect size are determined from an independent genome-wide association study (GWAS) of the disorder (the ‘discovery set’).³ PRSs can predict schizophrenia status in case–control studies and capture sufficient risk to examine genetic relationships between different diagnostic categories.⁵

PRSs were derived using the method employed by the International Schizophrenia Consortium.³ Risk alleles and odds ratios were taken from the discovery data set made available by the Schizophrenia Working Group of the Psychiatric Genomics Consortium (PGC) which contained 35 476 cases of the disorder and 46 839 controls.⁵ To allow for the effects of linkage disequilibrium, variants were restricted to autosomal single-nucleotide polymorphisms (SNPs) in relative linkage equilibrium (using --clump in PLINK version 1.07 on a UNIX systemReference Purcell, Neale, Todd-Brown, Thomas, Ferreira and Bender¹⁹ with the PGC2 schizophrenia meta-analysis P-values, with a maximum r ² of 0.25 and a window size of 500 kb), leaving 87 713 SNPs. PRSs were calculated for each CHDS participant as the mean number of risk alleles surpassing a particular association P-value threshold (P _T) in the PGC study, each weighted by its log-odds ratio, using the program PLINK.Reference Purcell, Neale, Todd-Brown, Thomas, Ferreira and Bender¹⁹ Primary analyses are based on scores constructed using a significance threshold (P _T) of 0.05 in the discovery GWAS as this is the modal threshold that captures the maximal variance to the schizophrenia phenotype in each of the subsamples of that meta-analysis.⁵ The risk scores were divided into quartiles for further analysis. For phenotypes that showed significant relationships with schizophrenia PRSs, secondary analyses were performed across a range of P _T values (P _T = 1, 0.5, 0.3, 0.2, 0.1, 0.01, 0.001, 1 × 10⁻⁴, 1 × 10⁻⁶, 5 × 10⁻⁸) to ensure the pattern of results was not particularly sensitive to the chosen threshold. Secondary analyses were also performed on these phenotypes by using continuous PRS values to ensure that our results were not sensitive to our use of PRS quartiles as a primary measure.

Mental health outcomes (18–35 years)

At ages 21, 25, 30 and 35 years, participants were administered a comprehensive mental health interview that assessed aspects of the individual's mental health and psychosocial adjustment over the period since the previous assessment. As part of this interview, the symptoms obtained were used to assign DSM-IV (1994)²⁰ mood disorders (major depression, manic/hypomanic episode); anxiety disorders (GAD, panic disorders, agoraphobia, social phobia, specific phobia) and alcohol dependence. Questioning was based on the relevant sections of the Composite International Diagnostic Interview (CIDI),²¹ which is a structured interview for mental/psychiatric disorders. The CIDI has been used extensively in community and epidemiological surveys of disorder.²⁰ From age 30 years, interviews were extended to include symptoms required to make DSM-IV diagnoses of schizophrenia/schizophreniform disorder. Interviews were administered by trained lay interviewers, as per the design of the CIDI. In the majority of cases (approximately 80%), interviews were conducted face to face or, if this was not possible (e.g. the participant was resident overseas), via telephone or Skype. Using these data, participants were first classified as to whether they met criteria for each of the above diagnoses in each of the interview periods from age 18–21, 21–25, 25–30 and 30–35 years. This information was then combined over interview periods to classify participants as to whether they had ever met criteria for the DSM-IV diagnoses over the whole period of age 18–35 years. The diagnoses included in the present analysis and associated adult lifetime (18–35 years) prevalence estimates were as follows: major depression (47.6%), manic or hypomanic episode (7.6%), GAD (9.1%), panic disorder with or without agoraphobia (14.2%), social phobia (15.4%), specific phobia (20.7%), alcohol dependence (12.9%) and schizophrenia/schizophreniform disorder (2.0%). The total number of anxiety disorders (defined as specific phobia, social phobia, panic disorder and GAD) was also calculated and used as a phenotypic variable. In this longitudinal study of lifetime adult disorder (up to age 30), consistent with aetiological pleiotropy, there was substantial comorbidity between domains of mood disorder (e.g., major depressive disorder, manic/hypomanic episode), anxiety, alcohol dependence and schizophrenia (odds ratios up to 30 depending on disorder; see Supplementary Table 2).

Sample size and statistical analysis

The present analysis was based on a sample of 590 participants (286 male and 304 female) from CHDS who were observed on mental health outcomes from age 18 to 35 years, who were successfully genotyped on the Illumina chip and therefore for whom schizophrenia PRSs could be constructed. As above, analyses were limited to participants who were of European ancestry. Comparison of those included in the analysis with those not included showed no statistically significant differences in the observed rates of disorder (see Supplementary Text and Supplementary Table 3).

We performed regression of the phenotype variables on quartiles of schizophrenia PRSs (logistic regression for dichotomous outcomes, linear regression for the number of anxiety disorders). Gender and the first two population principal components were included in the regression as covariates. Analyses were conducted using the glm() function in R.²² As phenotype measures were correlated, Bonferroni multiple testing correction would be overly conservative and so we used false discovery rate (FDR) multiple testing correction (in R) instead.Reference Benjamini and Hochberg²³ Where significant associations were found between schizophrenia PRS and anxiety disorders, conditional analysis was conducted to determine whether these associations were independent of each other.

To examine the effect of comorbidity among anxiety disorders, we also performed a secondary association analysis comparing individuals with any one anxiety disorder with those with no anxiety disorders, and another comparing individuals with two or more anxiety disorders with those with no anxiety disorders (see Supplementary Table 2).

Replication sample and analysis

To replicate our novel finding from the CHDS study, we tested the relationship between schizophrenia PRS and mania/hypomania episode in the ALSPAC sample. The initial cohort contained 15 445 participants with extensive baseline information from the first trimester of pregnancy onwards. Data were collected regularly at defined time intervals and is ongoing.

Hypomanic features in ALSPAC was assessed using the Hypomania Checklist (HCL-32) at age 22–23 years. The HCL-32 is a self-rating questionnaire designed to capture a lifetime history of hypomanic symptoms.Reference Angst, Azorin, Bowden, Perugi, Vieta and Gamma^24–Reference Carta, Hardoy, Cadeddu, Murru, Campus and Morosini²⁷ It has been used extensively in clinical and non-clinical settings and is validated as a screening tool for bipolar disorder type II. Following a Rasch analysis for unidimensionality of the HCL-32, four items were identified as redundant and could be excluded.Reference Court, Forty, Jones, Gordon-Smith, Jones and Craddock²⁸ Our primary analysis in ALSPAC was based on the preferred definition of hypomanic episode in ALSPAC, which is defined as meeting a threshold score on the HCL-32 of 14 or more (out of 28), having symptoms for at least 2 days and a response of either a negative or both negative and positive impact of periods of elevated mood on family, social, or work life or on leisure. However, we tested a more stringent definition requiring a 4 day duration, as in CHDS.

Genetic data from 9912 participants were obtained using a genome-wide SNP genotyping platform (HumanHap550-Quad; Illumina). Following quality control, imputation and restriction to 1 young person per family, genetic data were available on 8230 individuals, of whom 2655 individuals were of European ancestry and had HCL-32 data. Based on the 2-day duration criterion, the number of individuals classed as having a hypomanic episode (n = 239) was comparable to that in CHDS (~7%), but this fell to 50 (1.88%) when the 4-day criterion was applied.

The schizophrenia PRS was constructed in the same way as for the CHDS sample (see above), using the PGC2 schizophrenia study as the discovery data set⁵ and a P _T threshold of 0.05. The relationship between schizophrenia PRS and hypomanic episode was examined using logistic regression in STATA (v14.1 SE, Macintosh platform), including gender as a covariate. In both the CHDS and ALSPAC samples, schizophrenia PRSs were calculated blind to phenotype classification.