Summary information and primary citation

PDB-id
8unf; SNAP-derived features in text and JSON formats; DNAproDB
Class
replication
Method
cryo-EM (3.15 Å)
Summary
cryo-EM structure of t4 bacteriophage clamp loader with sliding clamp and DNA
Reference
Marcus K, Huang Y, Subramanian S, Gee CL, Gorday K, Ghaffari-Kashani S, Luo XR, Zheng L, O'Donnell M, Subramaniam S, Kuriyan J (2024): "Autoinhibition of a clamp-loader ATPase revealed by deep mutagenesis and cryo-EM." Nat.Struct.Mol.Biol., 31, 424-435. doi: 10.1038/s41594-023-01177-3.
Abstract
Clamp loaders are AAA+ ATPases that facilitate high-speed DNA replication. In eukaryotic and bacteriophage clamp loaders, ATP hydrolysis requires interactions between aspartate residues in one protomer, present in conserved 'DEAD-box' motifs, and arginine residues in adjacent protomers. We show that functional defects resulting from a DEAD-box mutation in the T4 bacteriophage clamp loader can be compensated by widely distributed single mutations in the ATPase domain. Using cryo-EM, we discovered an unsuspected inactive conformation of the clamp loader, in which DNA binding is blocked and the catalytic sites are disassembled. Mutations that restore function map to regions of conformational change upon activation, suggesting that these mutations may increase DNA affinity by altering the energetic balance between inactive and active states. Our results show that there are extensive opportunities for evolution to improve catalytic efficiency when an inactive intermediate is involved.

Cartoon-block schematics in six views (download the tarball)

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