Article

  • The EMBO Journal (2004) 23, 4342 - 4352
  • doi:10.1038/sj.emboj.7600438

Published online: 7 October 2004

Defining the position of the switches between replicative and bypass DNA polymerases

Shingo Fujii and Robert P Fuchs

  1. UPR 9003 du CNRS, Cancerogenese et Mutagenese Moleculaire et Structurale, ESBS, Blvd S Brant Strasbourg, Illkirch, France

Correspondence to:

Robert P Fuchs, UPR 9003 Cancerogenese & Mutagenese, Moleculaire et Structurale CNRS, ESBS Pole API, Boulevard Sebastien Brant, 67400 Illkirch-Graffenstaden, France. Tel.: +33 390 244 688; Fax: +33 390 244 686; E-mail: fuchs@esbs.u-strasbg.fr

Received 30 June 2004; Accepted 15 September 2004


Cells contain specialized DNA polymerases that are able to copy past lesions with an associated risk of generating mutations, the major cause of cancer. Here, we reconstitute translesion synthesis (TLS) using the replicative (Pol III) and major bypass (Pol V) DNA polymerases from Escherichia coli in the presence of accessory factors. When the replicative polymerase disconnects from the template in the vicinity of a lesion, Pol V binds the blocked replication intermediate and forms a stable complex by means of a dual interaction with the tip of the RecA filament and the beta-clamp, the processivity factor donated by the blocked Pol III holoenzyme. Both interactions are required to confer to Pol V the processivity that will allow it synthesize, in a single binding event, a TLS patch long enough to support further extension by Pol III. In the absence of these accessory factors, the patch synthesized by Pol V is too short, being degraded by the Pol III-associated exonuclease activity that senses the distortion induced by the lesion, thus leading to an aborted bypass process.

  • Keywords:

    • Pol III holoenzyme,
    • Pol V,
    • polymerase switch,
    • processivity factor beta-clamp,
    • RecA filament
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