Amplification and Excision of Integrated Polyoma DNA Sequences Require a Functional Origin of Replication

Overview

Journal Cell

Publisher Cell Press

Specialty Cell Biology

Date 1984 Apr 1

PMID 6323029

Citations 24

Authors

S Pellegrini

L Dailey

C Basilico

Affiliations

Soon will be listed here.

Abstract

Cells transformed by Polyoma virus (Py) can undergo a high rate of excision or amplification of integrated viral DNA sequences, and these phenomena require the presence of homology (i.e., repeats) within the viral insertion as well as a functional viral large T antigen (T-Ag). To determine whether the main role of large T-Ag in excision and amplification was replicative or recombination-promoting, we studied transformed rat cell lines containing tandem insertions of a ts-a Py molecule (encoding a thermolabile large T-Ag) with a deletion of the origin of viral DNA replication. Culturing of these cells at the temperature permissive for large T-Ag function did not result in any detectable excision or amplification of integrated Py sequences. We then introduced into origin-defective lines a recombinant plasmid containing the viral origin of replication and the gene coding for resistance to the antibiotic G418. All G418-resistant clones analyzed readily amplified the integrated plasmid molecules when grown under conditions permissive for large T-Ag function, showing that these cells produced viral large T-Ag capable of promoting amplification in trans of DNA sequences containing the Py origin. These observations strongly suggest that Polyoma large T antigen promotes excision or amplification of viral DNA by initiating replication at the integrated origin, providing a favorable substrate for subsequent recombination.

Citing Articles

Does a new polyomavirus contribute to Merkel cell carcinoma?.

Garneski K, DeCaprio J, Nghiem P Genome Biol. 2008; 9(6):228.

PMID: 18598371 PMC: 2481414. DOI: 10.1186/gb-2008-9-6-228.

High-frequency recombination mediated by polyomavirus large T antigen defective in replication.

St-Onge L, Bouchard L, Bastin M J Virol. 1993; 67(4):1788-95.

PMID: 8445711 PMC: 240224. DOI: 10.1128/JVI.67.4.1788-1795.1993.

Amplification mediated by polyomavirus large T antigen defective in replication.

St-Onge L, Bastin M J Virol. 1993; 67(8):5025-9.

PMID: 8392627 PMC: 237891. DOI: 10.1128/JVI.67.8.5025-5029.1993.

Elements of the polyomavirus replication origin required for homologous recombination mediated by large T antigen.

Laurent S, Bastin M J Virol. 1995; 69(11):7304-8.

PMID: 7474159 PMC: 189659. DOI: 10.1128/JVI.69.11.7304-7308.1995.

Isolation of large T antigen-producing mouse cell lines capable of supporting replication of polyomavirus-plasmid recombinants.

Muller W, Naujokas M, Hassell J Mol Cell Biol. 1984; 4(11):2406-12.

PMID: 6096696 PMC: 369071. DOI: 10.1128/mcb.4.11.2406-2412.1984.