Genome-wide association study of type 2 diabetes in Africa

South African Zulu individuals were type 2 diabetes cases and controls from two studies: the Durban Diabetes Study (DDS) and the Durban Diabetes Case Control study (DCC). DDS was a population-based cross-sectional study of non-pregnant urban black African adults of Zulu descent, aged >18 years, residing in Durban, South Africa [15, 16]. Further details are provided in the electronic supplementary material (ESM) Methods. Additional type 2 diabetes cases from the same ethnic group and locality were obtained from the DCC, which included individuals with type 2 diabetes attending a diabetes clinic. Type 2 diabetes was defined using WHO criteria [15, 16]. The combined type 2 diabetes cases and controls from DDS and DCC were aggregated into a single Zulu study.

The Africa America Diabetes Mellitus (AADM) study comprised individuals from sub-Saharan Africa, enrolled from university medical centres in Nigeria, Ghana and Kenya. A person with type 2 diabetes was identified using ADA criteria or if he or she was receiving treatment for type 2 diabetes. Probable cases of type 1 diabetes were excluded and controls had no evidence of diabetes based on fasting/2 h glucose or symptoms of suggestive diabetes [14]. The characteristics of the Zulu and AADM participants are shown in ESM Table 1.

In total, 2707 African individuals of Zulu descent (2003 women and 704 men) were genotyped using the Illumina Multi-Ethnic Genotyping Array (Illumina, Illumina Way, San Diego, CA, USA). Following sample and variant quality control (QC) (ESM Methods), there were 2578 samples with genotype and phenotype information (1602 cases and 976 controls) and 1,434,868 variants (1,395,345 autosomal and 39,523 on the X chromosome).

The AADM samples were genotyped on the Affymetrix Axiom PANAFR SNP array as described previously [14]. After QC (ESM Methods), there were 1031 cases and 738 controls and 2,141,465 variants (2,080,378 autosomal and 61,087 on the X chromosome) in AADM.

All samples were imputed to a merged panel of 1000 Genomes phase 3 [17] and African samples using IMPUTE2 [18] (Zulu) or positional Burrows–Wheeler transform (PBWT) [19] using the Sanger imputation server (AADM) (ESM Methods). We retained all imputed SNPs with MAF > 0.01 and imputation information score > 0.4 that were also in a newer version of the imputation panel.

In Zulu samples, association with type 2 diabetes was performed for each variant based on the imputation dosage using a linear mixed model that accounts for the presence of related individuals and any population structure implemented in genome-wide efficient mixed-model association (GEMMA) [20], adjusting for age, sex and BMI. The kinship matrix was estimated from directly genotyped autosomal variants with MAF > 0.01. In AADM, association with type 2 diabetes was performed for each variant based on the imputation dosage using an additive logistic regression model implemented in SNPTEST v2.5.2 [21] (Oxford University, Oxford, UK www.​well.​ox.​ac.​uk/​~gav/​resources/​snptest_​v2.​5.​2_​linux_​x86_​64_​dynamic.​tgz) adjusting for age, sex, BMI and the first three principal components (PCs) to account for population structure. The number of PCs adjusted for in AADM was determined by testing for the number of PCs using the minimum average partial test [22]. The first three PCs were determined to be significant and thus were adjusted for in the association analyses.

Meta-analysis of the Zulu and AADM summary statistics for shared variants was performed using a fixed-effects meta-analysis (weighted for effective sample size) in METAL [23] and we applied double genomic-control correction (ESM Methods). To identify distinct signals of association, we performed approximate conditional analyses using the joint model implemented in genome-wide complex trait analysis (GCTA) [24, 25] and variants with p < 2.5 × 10⁻⁸ in the joint model were selected as signals with genome-wide significance [26]. To estimate meta-analysis ORs, we also performed an inverse-variance-weighted meta-analysis using an approximation of the allelic log_eOR and variance from the linear model in the Zulu samples [27], and the log_eOR estimates obtained directly from SNPTEST for the AADM samples.

We used FINEMAP [28] (C. Benner, University of Helsinki, Finland www.​christianbenner.​com/​finemap_​v1.​1_​x86_​64.​tgz) to identify likely causal variants within 500 kb either side of the most significant variant at the loci TCF7L2 and AGMO in the African meta-analysis and in Europeans [5] (ESM Methods).

We used ‘direct’ (same lead variant with p < 0.05 and directionally consistent) and ‘local’ (locus-level) detection to explore the extent to which existing GWAS signals (almost all from non-African samples) were detected in the African GWAS (ESM Methods, ESM Table 2). We used two complementary approaches to test for enrichment of signals detected using the ‘direct’ approach: (1) a binomial test taking significance (p < 0.05) and direction of effect into account; and (2) enrichment of directly detected variants, accounting for the properties of the variants in GARFIELD [29] (ESM Methods). For loci demonstrating ‘direct’ and/or ‘local’ detection between our African data and existing GWAS signals (ESM Table 2), we performed co-localisation analyses implemented in the R package ‘coloc’ [30] using summary statistics from the largest available European type 2 diabetes GWAS at the time of analysis [5] (default prior for causal variant sharing set to 0.5) (ESM Methods). Using the weighted allele frequencies and sample sizes from the African meta-analysis and previously reported effect sizes, we estimated the power to detect established variants at the significance thresholds p < 0.05 and p < 2.5 × 10⁻⁸ using R version 3.3.0 [31] (ESM Table 2).

We also performed genetic risk score (GRS) analyses to harvest association information from multiple variants. GRSs were calculated as the total number of risk alleles in subsets of the 102 variants at established loci from existing GWAS studies of type 2 diabetes (published before May 2018), primarily in populations of European and Asian ancestry (ESM Table 2).

We used the haplotypic information for INS-variable number tandem repeat (VNTR) generated in African-descent individuals by Stead et al (2003) [32] to impute INS-VNTR lineages in the Zulu and AADM samples and perform a meta-analysis (ESM Methods). Conditional analysis was performed to detect distinct association signals by inclusion of dosages of the lead type 2 diabetes variants as covariates in the regression model.

Ethical approval was obtained for each participating cohort: the Institutional Review Board for each AADM participating institution and the Biomedical Research Ethics Committee of the University of KwaZulu-Natal for DCC (BF078/08) and DDS (BF030/12). DDS also had UK National Research Ethics Service approval (reference: 14/WM/1061). Written informed consent was obtained from all participants and the study was conducted in accordance with the principles of the Declaration of Helsinki.

Fine-mapping of TCF7L2 and AGMO identified the most significant variants from the meta-analysis, rs7903146 and rs73284431, as the most likely causal variants with posterior probabilities of association of 0.996 and 0.828, respectively (ESM Table 9). These were the only SNPs in the top configuration of causal variants from FINEMAP (ESM Figs. 1 and 2). At TCF7L2, a second plausible causal variant, rs17746147 (r² = 0.009 with rs7903146 estimated from the African samples in the merged panel), with posterior probability of association of 0.295, was contained in the second most likely configuration of causal variants (ESM Table 9, ESM Fig. 1). The 99% credible intervals and corresponding results in Europeans are presented in ESM Table 9. Fine-mapping results were comparable when using the stepwise approximate Bayes factor approach [42] (data not shown).

We explored the extent to which previously reported type 2 diabetes association signals could be detected in African-descent individuals. Based on the previously reported effect sizes and the effect allele frequency and sample size from our African meta-analysis, we had sufficient power (80%) to detect three signals (TCF7L2, DNER and SRR) at genome-wide significance (p < 2.5 × 10⁻⁸) (ESM Table 2). Only the TCF7L2 variant reached genome-wide significance in our study, whereas both variants in DNER (rs1861612) and SRR (rs391300), originally discovered in Pima Indians and East Asians, respectively, had p > 0.1 (ESM Table 2).

So far, five African-American type 2 diabetes-associated signals have been reported, three of which (two in KCNQ1 and one in HMGA2) were first reported in Europeans and two (INS-IGF2 and HLA-B) were first reported in African-Americans (ESM Table 2) [13]. In our meta-analysis, we detected only a nominal association for the African-American INS-IGF2 signal (rs3842770, p = 0.0020, ESM Table 2). However, we identified another signal at this locus (rs12277475, p = 2.0 × 10⁻⁷, ESM Table 3) that is independent of the African-American signal (rs3842770), and this signal co-localises with association in Europeans (posterior probability H4 = 1, ESM Table 10).

In ‘direct’ analyses (same lead variant with p < 0.05 and directionally consistent in the African meta-analysis), we detected 12 of 100 lead variants (ESM Table 2) at established type 2 diabetes loci first reported in non-African ancestry individuals, significantly more than expected by chance (binomial test of enrichment p = 8.14 × 10⁻⁶, GARFIELD enrichment OR [95% CI] 3.07 (1.50, 6.28), p = 0.002) (ESM Methods). In addition, detection of ‘local’ signals (at least one variant within the 200 kb region flanking the previously reported index variant [100 kb either side] reaching nominal significance [p < 0.05] after correcting for the effective number of independent tests) identified 11 type 2 diabetes loci, two of them overlapping signals also detected with the direct approach (ESM Table 2). Genetic co-localisation analyses suggested that African and non-African populations share the same causal variants at all 21 loci showing direct or local detection in our data (posterior probability H4 > 0.8, ESM Table 10).

We constructed GRSs by combining subsets of 102 previously established loci (including those first reported in African-ancestry individuals) and tested for association with type 2 diabetes (ESM Table 2). A GRS constructed from these variants showed significant association with type 2 diabetes in the Zulu (OR 1.05 per risk allele, p = 1.3 × 10⁻⁵, Fig. 2a) and AADM samples (OR 1.02 per risk allele, p = 0.020, Fig. 2b), an association driven primarily by the 13 directly detected variants (Zulu, OR 1.17, p = 1.7 × 10⁻⁹; AADM, OR 1.05, p = 0.029). GRSs based on the variants detected by only the local approach or the variants not detected by either approach were not significantly associated with type 2 diabetes in African samples (p = 0.19 and 0.084, respectively in the Zulu; p = 0.11 and 0.32, respectively in AADM) (Fig. 2). These results show there is a shared genetic contribution to type 2 diabetes at established loci directly detected in Africans.