| Literature DB >> 24161951 |
Shweta Singh1, Kate Rockenbach1, Rebekah M Dedrick1, Andrew P VanDemark1, Graham F Hatfull2.
Abstract
Phage-encoded serine integrases are large serine recombinases that mediate integrative and excisive site-specific recombination of temperate phage genomes. They are well suited for use in heterologous systems and for synthetic genetic circuits as the attP and attB attachment sites are small (<50 bp), there are no host factor or DNA supercoiling requirements, and they are strongly directional, doing only excisive recombination in the presence of a recombination directionality factor. Combining different recombinases that function independently and without cross-talk to construct complex synthetic circuits is desirable, and several different serine integrases are available. However, we show here that these functions are not reliably predictable, and we describe a pair of serine integrases encoded by mycobacteriophages Bxz2 and Peaches with unusual and unpredictable specificities. The integrases share only 59% amino acid sequence identity and the attP sites have fewer than 50% shared bases, but they use the same attB site and there is non-reciprocal cross-talk between the two systems. The DNA binding specificities do not result from differences in specific DNA contacts but from the constraints imposed by the configuration of the component half-sites within each of the attachment site DNAs.Entities:
Keywords: BSA; C-terminal domain; CC; CTD; N-terminal domain; NTD; RD; ZD; attachment site selection; bovine serum albumin; coiled coil; integrase; phage integration; recombinase domain; serine recombinase; site-specific recombination; zinc-nucleated domain
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Year: 2013 PMID: 24161951 PMCID: PMC3947336 DOI: 10.1016/j.jmb.2013.10.013
Source DB: PubMed Journal: J Mol Biol ISSN: 0022-2836 Impact factor: 5.469