A bipartite nuclear localization signal in the retinoblastoma gene product and its importance for biological activity.

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Mol Cell Biol. 1993 August; 13(8): 4588-4599

A bipartite nuclear localization signal in the retinoblastoma gene product and its importance for biological activity.

E Zacksenhaus, R Bremner, R A Phillips and B L Gallie

Division of Immunology and Cancer Research, Hospital for Sick Children, Toronto, Ontario, Canada.

ABSTRACT

The retinoblastoma gene product, p110RB1, appears to regulatecell growth by modulating the activities of nuclear transcriptionfactors. The elements that specify the transport of p110RB1into the nucleus have not yet been explored. We now report theidentification of a basic region, KRSAEGGNPPKPLKKLR, in theC terminus of p110RB1, which has sequence similarity to knownbipartite nuclear localization signals (NLSs). A two-amino-acidmutation introduced into this putative NLS [to give mutant NLS(NQ)]or deletion of the entire NLS (delta NLS) abrogated exclusivenuclear localization, yielding proteins which were distributedeither equally throughout the cell or predominantly in the cytoplasm.A mutant protein [NLS(NQ)/delta 22] containing both the mutatedNLS and a deletion of exon 22, previously shown to disrupt theinteraction of p110RB1 with several cellular transcription factorsand oncoproteins, accumulated only in the cytoplasm. When fusedto the C terminus of Escherichia coli beta-galactosidase, theRB1 NLS directed this protein to the nucleus, indicating thatthe motif is not only necessary but also sufficient for nucleartransport. Neither NLS(NQ) nor delta NLS was hyperphosphorylatedin vivo, but both retained their abilities to interact, in vitro,with simian virus 40 large T antigen, adenovirus E1a, and thecellular transcription factor E2F. When transfected at multiplecopy number, the NLS mutant alleles displayed reduced biologicalactivity, measured by inhibition of growth of the osteogenicsarcoma cell line Saos-2, which has no wild-type RB1. Naturallyoccurring mutations and deletions in exon 25 of RB1 which disruptthe NLS may lead to partial or complete inactivation of p110RB1and may be responsible for some retinoblastoma and other tumors.

Mol Cell Biol. 1993 August; 13(8): 4588-4599

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