A genome-wide association study for rheumatoid arthritis replicates previous HLA and non-HLA associations in a cohort from South Africa

Author:

Mathebula Evans M12ORCID,Sengupta Dhriti2ORCID,Govind Nimmisha23,Laufer Vincent A456,Bridges Jr S Louis7ORCID,Tikly Mohammed3,Ramsay Michèle12ORCID,Choudhury Ananyo2ORCID

Affiliation:

1. University of the Witwatersrand Division of Human Genetics, School of Pathology and National Health Laboratory Services, Faculty of Health Sciences, , Johannesburg, 2000 , South Africa

2. University of the Witwatersrand Sydney Brenner Institute for Molecular Bioscience, Faculty of Health Sciences, , Johannesburg, 2193 , South Africa

3. University of the Witwatersrand Division of Rheumatology, , Johannesburg, 1864 , South Africa

4. University of Alabama at Birmingham (UAB) Division of Clinical Immunology and Rheumatology, , Birmingham, AL 35294 , USA

5. University of Alabama at Birmingham Medical Scientist Training Program (UAB MSTP) , Birmingham, AL 35294 , USA

6. University of Alabama at Birmingham Department of Medicine, , Birmingham, AL 35294 , USA

7. Weill Cornell Medicine Department of Medicine, Hospital for Special Surgery, New York, NY, USA and Division of Rheumatology, , New York, NY 10021 , USA

Abstract

Abstract The complex pathogenesis of rheumatoid arthritis (RA) is not fully understood, with few studies exploring the genomic contribution to RA in patients from Africa. We report a genome-wide association study (GWAS) of South-Eastern Bantu-Speaking South Africans (SEBSSAs) with seropositive RA (n = 531) and population controls (n = 2653). Association testing was performed using PLINK (logistic regression assuming an additive model) with sex, age, smoking and the first three principal components as covariates. The strong association with the Human Leukocyte Antigen (HLA) region, indexed by rs602457 (near HLA-DRB1), was replicated. An additional independent signal in the HLA region represented by the lead SNP rs2523593 (near the HLA-B gene; Conditional P-value = 6.4 × 10−10) was detected. Although none of the non-HLA signals reached genome-wide significance (P < 5 × 10−8), 17 genomic regions showed suggestive association (P < 5 × 10−6). The GWAS replicated two known non-HLA associations with MMEL1 (rs2843401) and ANKRD55 (rs7731626) at a threshold of P < 5 × 10−3 providing, for the first time, evidence for replication of non-HLA signals for RA in sub-Saharan African populations. Meta-analysis with summary statistics from an African-American cohort (CLEAR study) replicated three additional non-HLA signals (rs11571302, rs2558210 and rs2422345 around KRT18P39-NPM1P33, CTLA4-ICOS and AL645568.1, respectively). Analysis based on genomic regions (200 kb windows) further replicated previously reported non-HLA signals around PADI4, CD28 and LIMK1. Although allele frequencies were overall strongly correlated between the SEBSSA and the CLEAR cohort, we observed some differences in effect size estimates for associated loci. The study highlights the need for conducting larger association studies across diverse African populations to inform precision medicine-based approaches for RA in Africa.

Funder

National Institutes of Health

University of the Witwatersrand

National Research Foundation

Publisher

Oxford University Press (OUP)

Subject

Genetics (clinical),Genetics,Molecular Biology,General Medicine

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