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Uncoordinated HLA-D Gene Expression in a RFXANK-Defective Patient with MHC Class II Deficiency
Author(s) -
Ana-María Len-Duménil,
MohamedRidha Barbouche,
Jocelyn Vedrenne,
Thomas Prod’homme,
Mohamed Béjaoui,
Salma Ghariani,
Dominique Charron,
Marc Fellous,
Koussay Dellagi,
Catherine AlcaïdeLoridan
Publication year - 2001
Publication title -
the journal of immunology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.737
H-Index - 372
eISSN - 1550-6606
pISSN - 0022-1767
DOI - 10.4049/jimmunol.166.9.5681
Subject(s) - exon , gene , biology , human leukocyte antigen , mutation , genetics , complementation , microbiology and biotechnology , phenotype , mhc class i , major histocompatibility complex , promoter , gene expression , antigen
We describe the analysis of a patient, JER, presenting classical immunological features of MHC class II deficiency. Unexpectedly, some HLA transcripts (HLA-DRA, HLA-DQA, and HLA-DMA) were found to be expressed in the JER cell line at nearly wild-type levels, while HLA-DPA and the HLA-D beta-chain transcripts were not detected. Gene reporter experiments confirmed the differential transcriptional activities driven by the HLA-D promoters in the JER cells. A defect in RFXANK was first suggested by genetic complementation analyses, then assessed with the demonstration of a homozygous mutation affecting a splice donor site downstream exon 4 of RFXANK. Because the severe deletion of the resulting protein cannot account for the expression of certain HLA-D genes, minor alternative transcripts of the RFXANK gene were analyzed. We thereby showed the existence of a transcript lacking exon 4, encoding a 28-aa-deleted protein that retains a transcriptional activity. Altogether, we characterize a new type of mutation in the RFXANK gene in a MHC class II-defective patient leading to an uncoordinated expression of the HLA-D genes, and propose that this phenotype is ensured by severely limited amounts of an active, although truncated RFXANK protein.

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