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Cloning of cDNAs for cellular proteins that bind to the retinoblastoma gene product

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Abstract

THE E7 transforming protein of human papilloma virus-16 binds to the retinoblastoma gene product (pRb)1, 2 through a nine-amino-acid segment of E7 (21–29)3–5. This segment of E7 is homologous to the pRb-binding domains of the simian virus 40 large T and adenovirus El A transforming proteins6–9. Each of these viral transá-forming proteins bind to the same region of pRb10, 11. To isolate cellular proteins that interact with this viral protein-binding domain on pRb12, 13, we used recombinant pRb to screen a human complementary DNA expression library. Two cDNAs were isolated that encode retinoblastoma binding proteins (RBP-1 and RBP-2). We report here that these RBP genes exist in separate loci and produce discrete messenger RNAs. The predicted amino-acid sequence of these genes showed no homology to known proteins, but both RBPs contain the pRb binding motif conserved between E7, large T and E1A14. In vitro expression of the RBP cDNAs yielded proteins that specifically bound to pRb. Recombinant E7 protein, the E7 21–29 peptide and the homologous RBP-1 peptide inhibited RBP-pRb binding. Mutations introduced into the putaá-tive pRb-binding segment in RBP-1 impaired its binding activity. These studies indicate that the cellular RBP-1, RBP-2 and viral E7 proteins interact with pRb through similar domains.

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Defeo-Jones, D., Huang, P., Jones, R. et al. Cloning of cDNAs for cellular proteins that bind to the retinoblastoma gene product. Nature 352, 251–254 (1991). https://doi.org/10.1038/352251a0

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