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Two-dimensional gel analysis of rolling circle replication in the presence and absence of bacteriophage T4 primase
Author(s) -
Karyn Goudie Belanger,
Christine Mirzayan,
Helen E. Kreuzer,
Bruce Alberts,
Kenneth N. Kreuzer
Publication year - 1996
Publication title -
nucleic acids research
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 9.008
H-Index - 537
eISSN - 1362-4954
pISSN - 0305-1048
DOI - 10.1093/nar/24.11.2166
Subject(s) - biology , primase , dnag , dna replication , rolling circle replication , dna , replisome , microbiology and biotechnology , duplex (building) , prokaryotic dna replication , bacteriophage , origin of replication , genetics , circular bacterial chromosome , polymerase chain reaction , gene , reverse transcriptase , escherichia coli
The rolling circle DNA replication structures generated by the in vitro phage T4 replication system were analyzed using two-dimensional agarose gels. Replication structures were generated in the presence or absence of T4 primase (gp61), permitting the analysis of replication forks with either duplex or single-stranded tails. A characteristic arc shape was visualized when forks with single-stranded tails were cleaved by a restriction enzyme with the help of an oligonucleotide that anneals to restriction sites in the single-stranded tail. After calibrating the gel system with this well-studied rolling circle replication reaction, we then analyzed the in vivo replication directed by a T4 replication origin cloned within a plasmid. DNA samples were generated from infections with either wild-type or primase-deletion mutant phage. The only replicative arc that could be detected in the wild-type sample corresponded to duplex Y forms, consistent with very efficient lagging strand synthesis. Surprisingly, we obtained evidence for both duplex and single-stranded DNA tails in the samples from the primase-deficient infection. We conclude that a relatively inefficient mechanism primes lagging strand DNA synthesis in vivo when gp61 is absent.

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