Dimer-tetramer transition controls RUNX1/ETO leukemogenic activity

Author:

Wichmann Christian1,Becker Yvonne1,Chen-Wichmann Linping1,Vogel Vitali2,Vojtkova Anna1,Herglotz Julia1,Moore Sandra1,Koch Joachim1,Lausen Jörn1,Mäntele Werner2,Gohlke Holger345,Grez Manuel1

Affiliation:

1. Institute for Biomedical Research, Georg-Speyer-Haus, Frankfurt;

2. Institute for Biophysics and

3. Molecular Bioinformatics Group, Goethe-University, Frankfurt;

4. Institute of Pharmaceutical Chemistry, Christian-Albrechts-University, Kiel; and

5. Institute of Pharmaceutical and Medicinal Chemistry, Heinrich-Heine-University, Duesseldorf, Germany

Abstract

Abstract RUNX1/ETO, the fusion protein resulting from the chromosomal translocation t(8;21), is one of the most frequent translocation products in acute myeloid leukemia. Several in vitro and in vivo studies have shown that the homo-tetramerization domain of ETO, the nervy homology region 2 (NHR2), is essential for RUNX1/ETO oncogenic activity. We analyzed the energetic contribution of individual amino acids within the NHR2 to RUNX1/ETO dimer-tetramer transition and found a clustered area of 5 distinct amino acids with strong contribution to the stability of tetramers. Substitution of these amino acids abolishes tetramer formation without affecting dimer formation. Similar to RUNX1/ETO monomers, dimers failed to bind efficiently to DNA and to alter expression of RUNX1-dependent genes. RUNX1/ETO dimers do not block myeloid differentiation, are unable to enhance the self-renewal capacity of hematopoietic progenitors, and fail to induce leukemia in a murine transplantation model. Our data reveal the existence of an essential structural motif (hot spot) at the NHR2 dimer-tetramer interface, suitable for a molecular intervention in t(8;21) leukemias.

Publisher

American Society of Hematology

Subject

Cell Biology,Hematology,Immunology,Biochemistry

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