Improved methods for creating migratable Holliday junction substrates

Nucleic Acids Res. 2013 Mar 1;41(5):e60. doi: 10.1093/nar/gks1343. Epub 2012 Dec 28.

Abstract

Previously, we published a method for creating a novel DNA substrate, the double Holliday junction substrate. This substrate contains two Holliday junctions that are mobile, topologically constrained and separated by a distance comparable with conversion tract lengths. Although useful for studying late stage homologous recombination in vitro, construction of the substrate requires significant effort. In particular, there are three bottlenecks: (i) production of large quantities of single-stranded DNA; (ii) the loss of a significant portion of the DNA following the recombination step; and (iii) the loss of DNA owing to inefficient gel extraction. To address these limitations, we have made the following changes to the protocol: (i) use of a helper plasmid, rather than exogenous helper phage, to produce single-stranded DNA; (ii) use of the unidirectional C31 integrase system in place of the bidirectional Cre recombinase reaction; and (iii) gel extraction by DNA diffusion. Here, we describe the changes made to the materials and methods and characterize the substrates that can be produced, including migratable single Holliday junctions, hemicatenanes and a quadruple Holliday junction substrate.

Publication types

  • Research Support, N.I.H., Extramural
  • Research Support, Non-U.S. Gov't

MeSH terms

  • Attachment Sites, Microbiological
  • Bacteriophage M13 / genetics
  • Cloning, Molecular
  • DNA, Cruciform / biosynthesis*
  • DNA, Cruciform / genetics
  • DNA, Cruciform / ultrastructure
  • Escherichia coli
  • Integrases / genetics
  • Integrases / metabolism
  • Plasmids / genetics
  • Viral Proteins / genetics
  • Viral Proteins / metabolism

Substances

  • DNA, Cruciform
  • Viral Proteins
  • Integrases