Ctf18-RFC and DNA Pol ϵ form a stable leading strand polymerase/clamp loader complex required for normal and perturbed DNA replication

Author:

Stokes Katy1,Winczura Alicja1,Song Boyuan23,De Piccoli Giacomo1,Grabarczyk Daniel B2ORCID

Affiliation:

1. University of Warwick, Warwick Medical School, Coventry, UK

2. Rudolf Virchow Center for Integrative and Translational Bioimaging, Institute for Structural Biology, University of Würzburg, Josef-Schneider-Str. 2, Würzburg 97080, Germany

3. Department of Biochemistry, Biocenter, University of Würzburg, Am Hubland, Würzburg 97074, Germany

Abstract

AbstractThe eukaryotic replisome must faithfully replicate DNA and cope with replication fork blocks and stalling, while simultaneously promoting sister chromatid cohesion. Ctf18-RFC is an alternative PCNA loader that links all these processes together by an unknown mechanism. Here, we use integrative structural biology combined with yeast genetics and biochemistry to highlight the specific functions that Ctf18-RFC plays within the leading strand machinery via an interaction with the catalytic domain of DNA Pol ϵ. We show that a large and unusually flexible interface enables this interaction to occur constitutively throughout the cell cycle and regardless of whether forks are replicating or stalled. We reveal that, by being anchored to the leading strand polymerase, Ctf18-RFC can rapidly signal fork stalling to activate the S phase checkpoint. Moreover, we demonstrate that, independently of checkpoint signaling or chromosome cohesion, Ctf18-RFC functions in parallel to Chl1 and Mrc1 to protect replication forks and cell viability.

Funder

Cancer Research UK

DFG

Publisher

Oxford University Press (OUP)

Subject

Genetics

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