Structural Basis for the Interaction Between Yeast Chromatin Assembly Factor 1 and Proliferating Cell Nuclear Antigen: Binding of CAF-1 PIP motif by PCNA

Keely S. Orndorff, Evan J. Veltri, Nicole M. Hoitsma, Ivy L. Williams, Ian Hall, Grace E. Jaworski, Grace E. Majeres, Samaya Kallepalli, Abigayle F. Vito, Lucas R. Struble, Gloria E.O. Borgstahl, Lynne M. Dieckman

Research output: Contribution to journalArticlepeer-review

Abstract

Proliferating cell nuclear antigen (PCNA), the homotrimeric eukaryotic sliding clamp protein, recruits and coordinates the activities of a multitude of proteins that function on DNA at the replication fork. Chromatin assembly factor 1 (CAF-1), one such protein, is a histone chaperone that deposits histone proteins onto DNA immediately following replication. The interaction between CAF-1 and PCNA is essential for proper nucleosome assembly at silenced genomic regions. Most proteins that bind PCNA contain a PCNA-interacting peptide (PIP) motif, a conserved motif containing only eight amino acids. Precisely how PCNA is able to discriminate between binding partners at the replication fork using only these small motifs remains unclear. Yeast CAF-1 contains a PIP motif on its largest subunit, Cac1. We solved the crystal structure of the PIP motif of CAF-1 bound to PCNA using a new strategy to produce stoichiometric quantities of one PIP motif bound to each monomer of PCNA. The PIP motif of CAF-1 binds to the hydrophobic pocket on the front face of PCNA in a similar manner to most known PIP-PCNA interactions. However, several amino acids immediately flanking either side of the PIP motif bind the IDCL or C-terminus of PCNA, as observed for only a couple other known PIP-PCNA interactions. Furthermore, mutational analysis suggests positively charged amino acids in these flanking regions are responsible for the low micromolar affinity of CAF-1 for PCNA, whereas the presence of a negative charge upstream of the PIP prevents a more robust interaction with PCNA. These results provide additional evidence that positive charges within PIP-flanking regions of PCNA-interacting proteins are crucial for specificity and affinity of their recruitment to PCNA at the replication fork.

Original languageEnglish (US)
Article number168695
JournalJournal of Molecular Biology
Volume436
Issue number16
DOIs
StatePublished - Aug 15 2024

Keywords

  • Chromatin assembly factor 1
  • Gene silencing
  • Nucleosome assembly
  • PCNA-interacting peptide (PIP)
  • Proliferating cell nuclear antigen

ASJC Scopus subject areas

  • Biophysics
  • Structural Biology
  • Molecular Biology

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