Titolo | The nucleoside diphosphate kinase activity of DRnm23 is not required for inhibition of differentiation and induction of apoptosis in 32Dcl3 myeloid precursor cells |
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Tipo di pubblicazione | Articolo su Rivista peer-reviewed |
Anno di Pubblicazione | 2000 |
Autori | Venturelli, D., Cesi Vincenzo, Ransac S., Engelhard A., Perrotti D., and Calabretta B. |
Rivista | Experimental Cell Research |
Volume | 257 |
Paginazione | 265-271 |
ISSN | 00144827 |
Parole chiave | amino acid substitution, animal cell, Animalia, Apoptosis, article, cell differentiation, Cell Survival, cellular distribution, controlled study, enzyme activity, gene deletion, gene overexpression, nonhuman, nucleoside diphosphate kinase, priority journal, promyelocyte, protein protein interaction, stem cell |
Abstract | DRnm23 belongs to a multigene family which includes nm23-H1, the first bona fide metastasis suppressor gene, nm23-H2, nm23-H4, and nm23-H5. Like nm23H1, nm23-H2, and nm23-H4, DRnm23 possesses nucleoside diphosphate kinase (NDPK) activity. Upon overexpression in myeloid precursor 32Dc13 cells, DRnm23 inhibits granulocytic differentiation and promotes apoptosis. Two specific mutants of DRnm23 (H134Q and S136P), at residues required for the NDPK activity, inhibit differentiation and promote apoptosis of 32Dc13 cells. By contrast, substitution of serine 61 with proline (S61P) or deletion of the RGD domain (δRGD) abrogates the effects of wild-type DRnm23. Like wild-type DRnm23, all four mutants show a predominantly mitochondrial subcellular localization. These studies indicate that the enzymatic activity of DRnm23 is not required for the effects observed in 32Dcl3 cells. Moreover, the inability of the S61P and ARGD DRnm23 mutants to inhibit differentiation and promote apoptosis may be due to defective protein-protein interactions at the mitochondria, the predominant site of DRnm23 subcellular localization. (C) 2000 Academic Press. |
Note | cited By 16 |
URL | https://www.scopus.com/inward/record.uri?eid=2-s2.0-0034660253&doi=10.1006%2fexcr.2000.4899&partnerID=40&md5=3bd3a693fe9dede925ca192ceeb75596 |
DOI | 10.1006/excr.2000.4899 |
Citation Key | Venturelli2000265 |