Structural features of the priming signal recognized by primase: mutational analysis of the phage G4 origin of complementary DNA strand synthesis

Abstract

45 mutations (insertion, deletion and base substitution) of the G4 Gori_c were tested for their functional activity in M13 and R199 in vivo. The critical mutants were also assayed for their ability to synthesize pRNA in vitro using SSB and primase. The results demonstrate that the secondary structure and spacing of stem-loops I and III are essential for Gori_c activity and that the 5′-CTG-3′ sequence flanking stem-loop I is essential for initiation of pRNA synthesis.