CAF-1 deposits newly synthesized histones during DNA replication using distinct mechanisms on the leading and lagging strands

Author:

Rouillon Clément,Eckhardt Bruna V.,Kollenstart Leonie,Gruss Fabian,Verkennis Alexander E.E.,Rondeel Inge,Krijger Peter H.L.,Ricci Giulia,Biran Alva,van Laar Theo,Delvaux de Fenffe Charlotte M.,Luppens Georgiana,Albanese Pascal,Scheltema Richard A.,de Laat Wouter,Dekker Nynke H.,Groth Anja,Mattiroli FrancescaORCID

Abstract

ABSTRACTDuring every cell cycle, both the genome and the associated chromatin must be accurately replicated. Chromatin Assembly Factor-1 (CAF-1) is a key regulator of chromatin replication, but how CAF-1 cooperates with the DNA replication machinery is unknown. Here, we reveal that this crosstalk differs between the leading and lagging strand at replication forks. Using biochemical reconstitution, we show that DNA and histones promote CAF-1 recruitment to its binding partner PCNA and reveal that two CAF-1 complexes are required for efficient nucleosome assembly under these conditions. Remarkably, in the context of the replisome, CAF-1 competes with the leading strand DNA polymerase epsilon (Polε) for PCNA binding, but not with the lagging strand DNA polymerase Delta (Polδ). Yet, in cells, CAF-1 deposits newly synthesized histones equally on both daughter strands. Thus, on the leading strand, chromatin assembly by CAF-1 cannot occur simultaneously to DNA synthesis, while on the lagging strand both processes are coupled. We propose that these differences may facilitate distinct parental histone recycling mechanisms and accommodate the inherent asymmetry of DNA replication.

Publisher

Cold Spring Harbor Laboratory

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