Alternative splicing due to an intronic SNP in HMSD generates a novel minor histocompatibility antigen

Abstract: Here we report the identification of a novel human leukocyte antigen (HLA)-B44-restricted minor histocompatibility antigen (mHA) with expression limited to hematopoietic cells. cDNA expression cloning studies demonstrated that the cytotoxic T lymphocyte (CTL) epitope of interest was encoded by a novel allelic splice variant of HMSD, hereafter designated as HMSD-v. The immunogenicity of the epitope was generated by differential protein expression due to alternative splicing, which was completely controlled by 1… Show more

“…Each clone demonstrated specific lysis against the B-LCLs of the recipient but not against donor B-LCLs, indicating recognition of minor H antigen ( Figure 1A and Kawase et al 9 ). The minor H antigen for CTL-2A12 had been previously identified by expression cloning 9 ; on the other hand, the target minor H antigen for the HLA-A24-restricted CTL-1B9 clone, which was apparently hematopoietic lineage-specific (Figure 1A) and present in approximately 80% of the Japanese population (data not shown), had not yet been determined. Using these CTL clones, a panel of B-LCLs expressing the restriction HLA (HLA-B44 for CTL-2A12 and HLA-A24 for CTL-1B9) endogenously or retrovirally transduced, were subjected to "immunophenotyping" for the presence or absence of the minor H antigen by ELISA and, if necessary, by standard chromium release assay (CRA).…”

“…9 According to the above criteria, no false-positive SNPs were reported in any array types (Table 1). Confirmation genotyping of individual B-LCLs from both panels revealed none of the 44 that had been immunophenotyped as CTX Ϫ were misjudged, while 8 of the 44 CTX ϩ B-LCLs were found to actually carry no minor H-positive allele for ACC-6, which was likely due to the inclusion of individual B-LCLs showing borderline cytotoxicity (data not shown).…”

“…We eventually focused on rs1879894, as it showed a much more significant genome-wide P value than SNP rs1842353 ( Table 1). In contrast to the CTL-2A12 case, where many mutually correlated SNPs around the most significant one created a broad peak in the statistic plots ( In all SNP array types, a common association peak is observed at 18q21, to which the minor H antigen for CTL-2A12, encoded by the HMSD gene, had been mapped based on expression cloning 9 (arrows).…”

“…Based on this method, termed WGA/CTL, we were able to map the previously characterized ACC-6 minor H locus to a 115-kb block containing only 4 genes, including HMSD. 9 Moreover, using the same approach, a novel minor H antigen encoded by the BCL2A1 gene was identified within a 26-kb block containing only BCL2A1 on chromosome 15q25. Surprisingly, the pool size required to identify these regions was no more than 100 individuals.…”

“…7 CTL-1B9 was isolated from PBMCs harvested on day 30 after transplantation from a patient receiving a marrow graft from his HLA-identical sibling (HLA A11, A24, B39, B51, Cw7, Cw14), and CTL-2A12 has been described recently. 9 …”

Identification of human minor histocompatibility antigens based on genetic association with highly parallel genotyping of pooled DNA

“…Each clone demonstrated specific lysis against the B-LCLs of the recipient but not against donor B-LCLs, indicating recognition of minor H antigen ( Figure 1A and Kawase et al 9 ). The minor H antigen for CTL-2A12 had been previously identified by expression cloning 9 ; on the other hand, the target minor H antigen for the HLA-A24-restricted CTL-1B9 clone, which was apparently hematopoietic lineage-specific (Figure 1A) and present in approximately 80% of the Japanese population (data not shown), had not yet been determined. Using these CTL clones, a panel of B-LCLs expressing the restriction HLA (HLA-B44 for CTL-2A12 and HLA-A24 for CTL-1B9) endogenously or retrovirally transduced, were subjected to "immunophenotyping" for the presence or absence of the minor H antigen by ELISA and, if necessary, by standard chromium release assay (CRA).…”

“…9 According to the above criteria, no false-positive SNPs were reported in any array types (Table 1). Confirmation genotyping of individual B-LCLs from both panels revealed none of the 44 that had been immunophenotyped as CTX Ϫ were misjudged, while 8 of the 44 CTX ϩ B-LCLs were found to actually carry no minor H-positive allele for ACC-6, which was likely due to the inclusion of individual B-LCLs showing borderline cytotoxicity (data not shown).…”

“…We eventually focused on rs1879894, as it showed a much more significant genome-wide P value than SNP rs1842353 ( Table 1). In contrast to the CTL-2A12 case, where many mutually correlated SNPs around the most significant one created a broad peak in the statistic plots ( In all SNP array types, a common association peak is observed at 18q21, to which the minor H antigen for CTL-2A12, encoded by the HMSD gene, had been mapped based on expression cloning 9 (arrows).…”

“…Based on this method, termed WGA/CTL, we were able to map the previously characterized ACC-6 minor H locus to a 115-kb block containing only 4 genes, including HMSD. 9 Moreover, using the same approach, a novel minor H antigen encoded by the BCL2A1 gene was identified within a 26-kb block containing only BCL2A1 on chromosome 15q25. Surprisingly, the pool size required to identify these regions was no more than 100 individuals.…”

“…7 CTL-1B9 was isolated from PBMCs harvested on day 30 after transplantation from a patient receiving a marrow graft from his HLA-identical sibling (HLA A11, A24, B39, B51, Cw7, Cw14), and CTL-2A12 has been described recently. 9 …”

Identification of human minor histocompatibility antigens based on genetic association with highly parallel genotyping of pooled DNA

Biology of the Human Graft‐versus‐Tumor Response and How to Exploit It

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