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P068 The novel recombinant HLA-A*11:271 story: Serology to the rescue of the misnomenclature

HUMAN IMMUNOLOGY(2018)

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摘要
Aim The wide spread use of NGS for HLA typing has resulted in exponential growth of novel alleles reported to the IMGT. However, the majority of these novel alleles have not been serologically characterized which has significant clinical implications in solid organ and HCT, particularly pertaining to assignment of donor specific HLA antibodies. Methods The identified novel allele had been originally and unsuccessfully tested by rSSOP, SSP, Sanger SBT and Real-Time PCR. Subsequently, the sample was tested by NGS using Mia Fora reagents and analysis software (Immucor). The subject was redrawn for serologic typing using Terasaki trays (One Lambda). A family study analysis was conducted to determine the segregation of the novel allele carrying haplotype by descent. Results With the exception of NGS, none of the molecular methods produced a result of the A locus. NGS revealed a novel HLA-A allele that appears to result from a recombination between A*11:01:01:01 (ex 1 and partial ex 2) u0026 A:01:01:01 (starting from ex 2) as depicted in the figure of the nucleotide and amino acid partial sequence alignments and the NGS coverage plot. The Mia Fora software assigned the HLA A locus typing as A*33:03:01 and the second allele as novel with the closest reference allele match as A*01:01:01:01. The haplotype assignment function of Mia Fora identified the 2 haplotypes of the subject carrying the novel allele which was confirmed by a family study. The novel allele was confirmed by NGS using TruSight HLA typing kit (Illumina) and submitted to IMGT and assigned the name A*11:271. Serological typing was performed and showed positive reactions with 2 operationally monospecific A1 antisera and one polyspecific (A1 u0026 A36) sera, but with neither of the 2 operationally monospecific A11 antisera on the typing tray. Download high-res image (465KB) Download full-size image Conclusions This report presents a cautionary note that in the absence of serological characterization of HLA alleles, the current IMGT nomenclature may not reflect the clinically relevant antigen specificity of these alleles.
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