DNA polymerase β: effects of gapped DNA substrates on dNTP specificity, fidelity, processivity and conformational changes

Abstract

Pre-steady-state kinetic analysis was used to compare the catalytic properties of DNA polymerase β (Pol β) for single-base gap-filling and regular duplex DNA synthesis. The rate of polymerization (k_pol) and the apparent equilibrium dissociation constant of dNTP (K_d) were determined with single-nucleotide gapped DNA substrates for all four possible correct base pairs and twelve possible incorrect base pairs, and the results were compared with those obtained previously with non-gapped primer/template duplex DNA substrates. For correct dNTP incorporation, the use of single-nucleotide gapped DNA led to significant decreases in the K_d of dNTP. Although k_pol was little affected, the catalytic efficiency k_pol/K_d increased significantly owing to the decreases in K_d. In contrast, for incorrect dNTP incorporation, the use of single-nucleotide gapped DNA substrates did not affect the K_d of dNTP appreciably but caused the k_pol (and thus k_pol/K_d) for incorrect dNTP incorporation to increase. As a consequence the fidelity of Pol β was not significantly affected by the use of single-nucleotide gapped DNA substrates. In addition we show that under processive polymerization conditions the processivity of Pol β increases in the gap-filling synthesis owing to a decreased rate of DNA dissociation. Finally, with a single-nucleotide gapped DNA substrate the rate-limiting conformational change step before chemistry was also observed. However, the preceding fast conformational change observed with duplex DNA substrates was not clearly detected. A possible cause is that in the complex with the gapped DNA, the 8 kDa N-terminal domain of Pol β already exists in a closed conformation. This interpretation was supported by tryptic digestion experiments.