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Antibody-Based Approach to High-Volume Genotyping for MIC-1 Polymorphism

    D.A. Brown

    St. Vincent’s Hospital, Sydney, Australia

    ,
    A.R. Bauskin

    St. Vincent’s Hospital, Sydney, Australia

    ,
    W.D. Fairlie

    St. Vincent’s Hospital, Sydney, Australia

    ,
    M.D. Smith

    St. Vincent’s Hospital, Sydney, Australia

    ,
    T. Liu

    St. Vincent’s Hospital, Sydney, Australia

    ,
    N. Xu

    St. Vincent’s Hospital, Sydney, Australia

    &
    S.N. Breit

    *Address correspondence to: Dr. Samuel N. Breit, Centre for Immunology, St. Vincent’s Hospital, Victoria Street, Sydney NSW 2010, Australia. e-mail:

    E-mail Address: s.breit@cfi.unsw.edu.au

    St. Vincent’s Hospital, Sydney, Australia

    Published Online:https://doi.org/10.2144/02331rr03

    Macrophage inhibitory cytokine-1 (MIC-1) is a divergent member of the TGF-β superfamily. There are at least two known alleles of MIC-1 that are due to a G→C point substitution at position 6 of the mature protein, which alters a histidine to an aspartic acid (MIC-1 H and MIC-1 D). We have determined the phenotype of MIC-1 circulating in serum by exploiting the differences in the affinity of the two monoclonal antibodies to the H and D alleles of MIC-1. A PCR-RFLP-based method for genotyping MIC-1 is also described. We validate these two assays using DNA sequencing of 19 subjects as the standard. We then used the validated assay to determine the frequency of the two MIC-1 alleles in a population of 261 adult blood donors. Inter-assay and sequencing concordance was 100%. The frequency of the three common MIC-1 genotypes was homozygous (HH), 54%; heterozygous (HD), 39%; and homozygous (DD), 7%. This novel antibody-based assay confidently determines the genotype of MIC-1. It offers the advantages of an ELISA—ease of automation, high-volume throughput of samples, and ease of use in a routine, clinical laboratory.