PLoS ONE (Jan 2014)

NMR characterization of the interaction of the endonuclease domain of MutL with divalent metal ions and ATP.

  • Ryota Mizushima,
  • Ju Yaen Kim,
  • Isao Suetake,
  • Hiroaki Tanaka,
  • Tomoyo Takai,
  • Narutoshi Kamiya,
  • Yu Takano,
  • Yuichi Mishima,
  • Shoji Tajima,
  • Yuji Goto,
  • Kenji Fukui,
  • Young-Ho Lee

DOI
https://doi.org/10.1371/journal.pone.0098554
Journal volume & issue
Vol. 9, no. 6
p. e98554

Abstract

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MutL is a multi-domain protein comprising an N-terminal ATPase domain (NTD) and C-terminal dimerization domain (CTD), connected with flexible linker regions, that plays a key role in DNA mismatch repair. To expand understanding of the regulation mechanism underlying MutL endonuclease activity, our NMR-based study investigated interactions between the CTD of MutL, derived from the hyperthermophilic bacterium Aquifex aeolicus (aqMutL-CTD), and putative binding molecules. Chemical shift perturbation analysis with the model structure of aqMutL-CTD and circular dichroism results revealed that tight Zn(2+) binding increased thermal stability without changing secondary structures to function at high temperatures. Peak intensity analysis exploiting the paramagnetic relaxation enhancement effect indicated the binding site for Mn(2+), which shared binding sites for Zn(2+). The coexistence of these two metal ions appears to be important for the function of MutL. Chemical shift perturbation analysis revealed a novel ATP binding site in aqMutL-CTD. A docking simulation incorporating the chemical shift perturbation data provided a putative scheme for the intermolecular interactions between aqMutL-CTD and ATP. We proposed a simple and understandable mechanical model for the regulation of MutL endonuclease activity in MMR based on the relative concentrations of ATP and CTD through ATP binding-regulated interdomain interactions between CTD and NTD.