Avon Longitudinal Study of Parents and Children

The ALSPAC recruited 14 541 pregnant women resident in Avon, UK with expected dates of delivery from 1 April 1991 to 31 December 1992.20 21 A detailed description of the cohort can be found in online supplementary methods appendix A1. SHBG and total testosterone (TT) were measured in a subset of 513 males at 9.9, 11.8, 13.8, 15.5 and 17.8 years of age using ELISA in peripheral blood samples as previously described.22 Longitudinal sex hormone measurements were not available for females in ALSPAC. Bioavailable testosterone (BT) was derived from measures of TT and SHBG as previously described.22 Genetic data for the ALSPAC children were generated by Sample Logistics and Genotyping Facilities at the Wellcome Trust Sanger Institute and LabCorp. Data on asthma in the last 12 months were extracted from questionnaires completed by the ALSPAC mothers at 10.7, 13.1 and 13.8 years of age, and by the study participants themselves at 16.5 and 22.9 years. Details of the hormone measurements, genotype preprocessing and derived asthma measures can be found in online supplementary methods appendix A1.

UK Biobank

The UK Biobank project is a large prospective cohort study of approximately 500 000 individuals from across the UK, aged 40–69 years at recruitment. Details of the study recruitment have been previously described.23 24 Genotype imputation and quality control (QC) are described in online supplementary methods appendix A1. Data on ever having had an asthma diagnosis were self-reported by UK Biobank participants by touchscreen questionnaire. Following genotype-related exclusions and QC, a total of 38 337 asthma cases and 296 245 controls remained.

Trans-National Asthma Genetics Consortium genome-wide association study

The TAGC performed a large-scale ancestry-specific GWAS of asthma25 using a total of 23 948 asthma cases and 118 538 controls from 66 studies. The subsample of European ancestry comprised 19 954 asthma cases and 107 715 controls from 56 studies, identifying 673 genome-wide significant SNPs. The study meta-analysed results from cohorts of individuals with both childhood-onset and adult-onset asthma across a range of ages. Full summary statistics from the GWAS meta-analysis for all analysed SNPs are available online via the GWAS catalogue.26 The results of the random effects meta-analysis of European ancestry were used in all analyses.

Observational analyses

Cross-sectional associations of sex hormones and asthma at each of the five time points in ALSPAC were investigated using serial logistic regression in STATA V.14.2. Model 1 was unadjusted for the previous measure of asthma/hormone and model 2 was adjusted for the previous measure, therefore modelling change between time points. Hormone measures were matched with their closest asthma response, ensuring asthma (the outcome) proceeded the hormone measurement. Analyses were carried out in male singletons (n=512). Results of cross-sectional models were compared with the path analysis.

In order to test for potential differences in effects between time points, path analysis (a type of multiple regression analysis) was conducted using STATA V.14.2 and STATA structural equation model (SEM) builder. Separate generalised SEMs were fitted for SHBG, TT and BT and asthma (online supplementary figures S1–S3 appendix A1). All models were adjusted for maternal confounders (maternal smoking, maternal education, parity, gestational age, maternal age) as well as participants’ exact age. Details of covariate adjustments and the rationale of the path analyses can be found in online supplementary methods appendix A1.

In order to increase statistical power and counter possible bias due to missingness, multiple imputation was used to complete missing values in the exposure, outcome and covariates, in both the cross-sectional regressions and the path analysis using ICE27 in STATA V.14.2 (StataCorp, release 14).27 A detailed description of the multiple imputation can be seen in online supplementary appendix A1. Results using the imputed data set were compared with the complete case analysis. Descriptions of the variables are shown in table 1.

Age-dependent effects of SHBG variants

As a preliminary step, we examined whether the effects of the SNPs associated with SHBG in the GWAS by Coviello et al 18 had an age-dependent effect on SHBG and TT using the ALSPAC subsample (males aged 9.9–17.8 years). Generalised linear regression models were implemented in R V.3.4.1 to test cross-sectional associations between each of the SNPs and either z-scored SHBG, TT or BT at each of the five time points, adjusting for the top 20 derived principal components (PC).

Mendelian randomisation

Two-sample MR was used to investigate the hypothesised causal effect of SHBG on asthma. The two-sample approach requires only summary-level data from GWAS, enabling SNP-outcome and SNP-exposure effects to be derived from different data sets. The assumptions of two-sample MR are similar to those of one-sample MR, while additionally requiring that the summary statistics for both the exposure and the outcome are derived from studies of comparable populations. Analyses were performed using the TwoSampleMR R package, part of MR-Base.17 The inverse-variance weighted (IVW) approach was used as a primary analysis, with two complementary estimation methods as sensitivity analyses to assess horizontal pleiotropy (where the genetic variant associates with the outcome via an independent pathway to the exposure): a weighted-median estimator28 and MR Egger regression.29 Evidence for effect size dilution was assessed using the unweighted I² statistic,30 also called the I² _GX statistic.

IV combinations

Two combinations of independent SHBG IVs were used, based on associations reported in the previous GWAS (online supplementary table S5)18. IV combination A comprised entirely SNPs located in the SHBG gene, determined as independent variants in the conditional analysis by Coviello et al.18 Variants in the SHBG gene region are less likely to be subject to horizontal pleiotropy. This resulted in three variants comprising IV combination A. For IV combination B, all SNPs identified in the previous GWAS of SHBG were used (nine variants), including those in combination A. We excluded only SNPs located on the X-chromosome (rs1573036), SNPs with a minor allele frequency <0.01 in UK Biobank (rs6258), or SNPs unavailable in the Haplotype Reference Consortium-imputed UK Biobank data set (rs2411984). This approach using two complementary IV combinations has been used previously for assessing the effects of SHBG on metabolites31 in an MR framework. The diagram in figure 1 presents an overview of the analyses performed.

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Figure 1

Flow diagram of the Mendelian randomisation (MR) analyses performed. GWAS, genome-wide association studies; SHBG, sex hormone-binding globulin; SNP, single nucleotide polymorphism; TAGC, Trans-National Asthma Genetic Consortium. 

Age-dependent effects of SHBG variants

Serial cross-sectional analysis of the effect of the SHBG SNPs in ALSPAC revealed that only the rs12150660 variant had a consistent effect on SHBG levels and an age-dependent effect on TT and BT (figure 2 and online supplementary appendix A2). For SHBG there was an estimated 0.41 (95% CI 0.24 to 0.59), 0.39 (95% CI 0.23 to 0.55), 0.24 (95% CI 0.06 to 0.42), 0.38 (95% CI 0.21 to 0.55) and 0.38 (95% CI 0.20 to 0.55) SD increase in circulating SHBG (nmol/L) per copy of the rs12150660 variant allele (GT or TT genotype) at the ages of 9.9, 11.8, 13.8, 15.5 and 17.8 years, respectively. For TT, there was no evidence of an association at the earlier ages, however an effect was observed at the later time points. There was an estimated −0.03 (95% CI −0.21 to 0.15), −0.07 (95% CI −0.24 to 0.10), 0.27 (95% CI 0.09 to 0.45), 0.30 (95% CI 0.13 to 0.47) and 0.30 (95% CI 0.13 to 0.48) SD increase in testosterone per copy of the rs12150660 variant allele at the ages of 9.9, 11.8, 13.8, 15.5 and 17.8 years, respectively. For BT, there was an inverse pattern of association to that of SHBG, consistent with its derivation from the assayed SHBG and TT measures. There was a −0.37 (95% CI −0.54 to −0.19), −0.15 (95% CI −0.32 to 0.02), 0.10 (95% CI −0.09 to 0.28), −0.10 (95% CI −0.27 to 0.07) and −0.23 (95% CI −0.40 to −0.05) SD change in BT per copy of the rs12150660 variant allele at the five respective time points. There was also some evidence for an effect of rs1641537 and rs8023580 on SHBG and BT levels in childhood (figure 2 and online supplementary appendix A2). However, the remaining SNPs indicated inconsistent patterns of effect on SHBG, TT and BT across the five time points.

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Figure 2

Serial cross-sectional associations of estimated SD change in SHBG, bioavailable testosterone (BT) or total testosterone (TT), per copy of SHBG-raising allele for nine genetic variants used as SHBG instrumental variables (IV) in the Mendelian randomisation (MR) analyses. Associations assessed in a subset of Avon Longitudinal Study of Parents and Children (ALSPAC) males across five available time points. SHBG, sex hormone-binding globulin. 

Mendelian randomisation

In contrast to the observational findings, there was evidence of a protective effect of increased SHBG on asthma when using MR (figure 3 and online supplementary tables S6-S7 and supplementary table S8 appendix A1). In IVW analyses, there was an estimated 0.86 (95% CI 0.74 to 1.00) OR per unit increase in log SHBG for IV combination A and 0.94 (95% CI 0.82 to 1.09) OR for asthma when using IV combination B. Meta-analysed weighted-median estimates were similar, with a 0.83 (95% CI 0.72 to 0.96) OR for asthma per unit increase in log SHBG for IV combination A and an estimated 0.85 (95% CI 0.74 to 0.97) OR for asthma for IV combination B. Wider CIs and smaller effect sizes in the IVW estimated effects of combination B may indicate the presence of directional pleiotropy, which the IVW method is not robust to. This conclusion is supported by the results of the more conservative combination A, which is less likely to introduce pleiotropic effects. Estimates from MR Egger regression for combination B (MR Egger regression was not applied to combination A as there were not enough SNPs) were in the same direction as estimates from the other two methods with a 0.81 (95% CI 0.60 to 1.09) OR for asthma per unit increase in log SHBG, but with wider CIs that spanned the null (online supplementary figure S4 appendix A1), possibly reflecting the lower statistical power of MR Egger regression. There was no indication of dilution in the MR Egger regression estimates (I² for dilution=0.99). Heterogeneity tests for combination B in UK Biobank indicated some evidence for heterogeneity between SNPs for the IVW method (Cochran’s Q=15.4, Q p=0.051), with an I² for heterogeneity between SNPs of 48.1%. There was weak evidence for directional pleiotropy in combination B in UK Biobank, estimated using the MR Egger intercept (Egger intercept=1.01, p=0.173). Scatterplots of the SNP-asthma and SNP-SHBG effects can be seen in online supplementary figures S5 and S6 appendix A1.

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Figure 3

Meta-analysis forest plots of the estimated effects of the two SHBG instrumental variable (IV) combinations on asthma, in the TAGC genome-wide association studies (GWAS) and UK Biobank. Fixed effects  (FE)  meta-analysis of (A) the IVW estimated effect of IV combination A on asthma, (B) the IVW estimated effect of IV combination B on asthma, (C) the weighted-median (WM) estimated effect of IV combination A on asthma, (D) the WM estimated effect of IV combination B on asthma. IVW, inverse-variance weighted; SHBG, sex hormone-binding globulin; TAGC, Trans-National Asthma Genetic Consortium.

Sex-stratified MR analysis

The sex-stratified analysis in UK Biobank indicated differences in MR estimated effects between females and males (figure 4 and figure 5). For females, there was an IVW estimated 0.80 (95% CI 0.63 to 1.01) OR for asthma per unit increase in log SHBG when using IV combination A, whereas in males there was an IVW estimated 0.95 (95% CI 0.77 to 1.18) OR for asthma. For the weighted-median estimated effect there was an OR of 0.80 (95% CI 0.64 to 0.98) for females and an OR of 0.93 (95% CI 0.73 to 1.17) for males. When using IV combination B, similar evidence for a protective effect of SHBG on asthma was obtained in females, whereas these estimates largely agreed with estimates based on IV combination A in males. Larger effects were observed in females when using the weighted-median estimator and MR Egger regression sensitivity analyses than the IVW estimate, indicating horizontal pleiotropy in IV combination B (complete description of results in online supplementary tables S9-S10 and supplementary result appendix A1).

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Figure 4

Forest plots of the individual instrumental variable (IV) effects in the female subsample of UK Biobank using the two combinations of IVs to assess the genetic effect of sex hormone-binding globulin (SHBG) on asthma. MR effect sizes are presented as log odds for asthma per unit increase in log SHBG. Methods used include the weighted-median (All-WM), MR Egger regression (All-MR Egger) and inverse-variance weighted (All-IVW). (A) IV combination A includes nine single nucleotide polymorphisms (SNP) and (B) IV combination B includes three SNPs located in the SHBG gene. MR, Mendelian randomisation.

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Figure 5

Forest plots of the individual instrumental variable (IV) effects in the male subsample of UK Biobank using the two combinations of IVs to assess the genetic effect of sex hormone-binding globulin (SHBG) on asthma. Mendelian randomisation (MR) effect sizes are presented as log odds for asthma per unit increase in log SHBG. Methods used include the weighted-median (All-WM), MR Egger regression (All-MR Egger) and inverse-variance weighted (All-IVW). (A) IV combination A includes nine single nucleotide polymorphisms (SNP) and (B) IV combination B includes three SNPs located in the SHBG gene.

Observational analyses

In the observational analysis of the ALSPAC subsample, testosterone distribution at 13.8 years was severely non-normal which may lead to imprecision of the SEs of the estimated effects. It was hypothesised that this was due to some but not all males having transitioned through puberty. However, since the non-normality is observed only at the one time point, estimates from this single measure do not alter the conclusions.

All male hormone measurements were carried out using immunoassays, with evidence suggesting that immunoassays lack precision, particularly in children, where testosterone levels are low.38 At the earliest time point, a large number of measurements had to be set to the lowest detectable assay value. Sample sizes were also small due to the non-overlap of individuals with reports of asthma and those with measured sex hormones, with a large fraction of missing measurements, particularly at the final time point (table 1). We used multiple imputation to attempt to increase power for the analysis and additionally included reports of wheezing in the last 12 months as auxiliary variables that may predict asthma in order to aid the multiple imputation. Assuming an adequate number of imputations and valid imputation, that is, all data are missing at random and the imputation and analysis models are correct, the results from multiple imputation should be unbiased. However, multiple imputation will lead to large SEs and wide CIs if there is little overall information in the data sets. After multiple imputation, we observed large SEs and wide CIs in our estimated effects, indicating that statistical power to detect an association may have remained low in the sample size of 512 individuals despite imputation. All observational analyses were conducted in a subsample of males, and the observational effects of SHBG and testosterone on asthma in females have not been assessed, with the effects likely to differ substantially from males given the differences in effects between the two sexes observed in the genetic analyses.

Genetic analyses

A major limitation of the genetic analyses is that a two-sample MR-based approach estimates average lifetime effects of an exposure on a disease outcome and does not distinguish between changes in the magnitude of that effect during different critical periods of the life course. This means that overall effect estimates may not be representative of true effects at all ages if the exposure only affects the outcome at certain critical periods of the life course. This is particularly true for diseases such as asthma which are known to wax and wane. It was therefore not possible to determine if SHBG is causal to the ‘adolescent switch’ observed in asthma prevalence or if the decreased risk is an unrelated early-life or later-life effect of SHBG on asthma. Future studies could attempt to develop methods to investigate time-varying exposures (eg, SHBG) on time-varying outcomes (eg, asthma) in an MR framework.

We did not attempt to stratify the MR analysis by age of asthma onset due to measurement error being a potential major problem in the UK Biobank, as the adult participants aged 40–69 at recruitment were asked to recall age of asthma onset, likely leading to substantial imprecision in reports. Additionally, as SNPs used as SHBG IVs in the MR were derived from adult population GWAS, we considered them unlikely to proxy SHBG levels as robustly in childhood, given the results of the SNP validation step in the ALSPAC subsample (shown in figure 2), which would further reduce statistical power to detect an association. Similarly, although the TAGC GWAS consortium performed a sensitivity analysis where participants were stratified into childhood-onset asthma and adult-onset asthma, the cut-off age for childhood-onset asthma was 16 years of age, by which time any changes linked to sex hormones will have already occurred. Therefore, we did not conduct an age-of-onset stratified MR to compare the effects of sex hormones prepuberty versus postpuberty. In the sex-stratified analysis in UK Biobank, the lower number of asthma cases in the male subsample compared with the female subsample may have led to lower statistical power and wider CIs, which may explain the differences in results. Given that the CIs overlap substantially, we cannot determine with certainty whether effects are specific to females.

The genetic correlation between SHBG and testosterone (as well as other hormones such as oestrogens) presents a problem in MR and it was not possible to identify SNPs associated with testosterone that were not also associated with SHBG. A previous GWAS of testosterone19 identified several polymorphisms associated with testosterone, including the rs12150660 variant; however, all reported variants were also identified as associated with SHBG. It may be possible to investigate such situations in the future using multivariate MR.39 Winner’s curse is a likely issue in two-sample MR studies that derive SNP-exposure estimates from the same GWAS used to select IVs, and although we used effect estimates from the combined discovery and replication samples of the published GWAS of SHBG, which may mitigate effects due to winner’s curse, some residual bias may remain.

Overall, we have performed multiple analyses at several different time points in order to disentangle the complex relationship between the various sex hormones and asthma. The possibility of spurious results arising due to chance cannot therefore be ruled out. Future work should attempt to replicate these findings in independent data sets in order to confirm the current conclusions.