Recognition of distinct HLA-DQA1 promoter elements by a single nuclear factor containing Jun and Fos or antigenically related proteins

doi:10.1093/nar/21.8.1811

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Nucleic Acids Research, 1993, Vol. 21, No. 8 1811-1818
© 1993

MOLECULAR BIOLOGY

Recognition of distinct HLA-DQA1 promoter elements by a single nuclear factor containing Jun and Fos or antigenically related proteins

Maria Neve Ombra, Monica Autiero, Andrea DeLerma Barbaro⁺, Rosalba Barretta, Giovanna Del Pozzo and John Guardiola^*

International Institute of Genetics and Biophysics via Guglielmo Marconi 10, 1-80125 Naples, Italy

^* To whom correspondence should be addressed

Received January 14, 1993. Revised March 18, 1993. Accepted March 18, 1993.

The activity of MHC class II promoters depends upon conservedregulatory signals one of which, the extended X-box, containsIn its X₂ subregion a sequence related to the cAMP responseelement, CRE and to the TPA response element, TRE. Accordingly,X₂ is recognized by the AP-1 factor and by other c-Jun or c-Foscontaining heterodlmers. We report that the X-box dependentpromoter activity of the HLA-DQA1 gene is down-modulated byan array of DNA elements each of which represented twice eitherin an invertedly or directly repeated orientation. In this frame,we describe a nuclear binding factor, namely DBF, promiscuouslyInteracting with two of these additional signals, ${delta}$ and ${sigma}$ , andwith a portion of the X-box, namely the X-core, devoid of X₂.The presence of a single factor recognizing divergent DNA sequenceswas indicated by the finding that these activities were co-elutedfrom a heparin-Sepharose column and from DNA affinity columnscarrying different DNA binding sites as ligands. Competitionexperiments made with oligonucleotides representing wild typeand mutant DNA elements showed that each DNA element specificallyInhibited the binding of the others, supporting the contentionthat DBF is involved in recognition of different targets. Furthermore,we found that DBF also exhibits CRE/TRE binding activity andthat this activity can be competed out by addition of an excessof ${sigma}$ , ${delta}$ and X-core oligonucleotides. Anti-Jun peptide and anti-Fospeptide antibodies blocked not only the binding activity ofDBF, but also its X-core and ${sigma}$ binding; this blockade was removedby the addition of the Jun or Fos peptides against which theantibodies had been raised. In vitro synthesized Jun/Fos wasable to bind to all these boxes, albeit with seemingly differentaffinities. The cooperativity of DBF interactions may explainthe modulation of the X-box dependent promoter activity mediatedby the accessory DNA elements described here.

⁺ Present address: Istituto di Scienze Immunologiche, Universitàdi Verona, Verona, Italy

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