A single-strand specific endonuclease activity copurifies with overexpressed T5 D15 exonuclease

Abstract

The T5 D15 exonuclease purified from an overproducing strain of E. coil was shown to possess a low level of endonucleolytic activity specific for single-stranded DNA when assayed with 1 – 10 mM Mg²⁺ as co-factor. Endonuclease activity on double-stranded circular DNA could not be detected under these conditions. Nicked circular DNA was first gapped by the enzyme's exonucleolytic activity, creating a single-stranded region. This gapped substrate was then endonucleolytically cleaved and rapidly degraded. We show that a gapped and not a nicked substrate is required for this activity as previously suggested (Moyer, R. W. and Roth, C. T. 1977, J. Virol. 24, 177–193). The single-strand endonuclease activity could be selectively suppressed by using low concentrations of Mg²⁺ as co-factor (< 1 mM), thus allowing nicked double-stranded circular DNA to be gapped to a single-stranded circular species. We also report on sequence similarities between the T5 exonuclease and several prokaryotic DNA polymerases.