A chimeric Cre recombinase with regulated directionality

Warren, David J.; Laxmikanthan, Gurunathan; Landy, Arthur

doi:10.1073/pnas.0809949105

Cited by 26 publications

(30 citation statements)

References 40 publications

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“…Our strategy for genetically testing the Int bridges in a full recombination reaction depends on a previously constructed and characterized chimeric recombinase in which the amino-terminal domain of λ-integrase was fused with the Cre recombinase (17). Here we refer to this recombinase as Crn1.…”

Section: Confirmation Of the Hj Int Bridges In Complete Recombinationmentioning

confidence: 99%

Mapping the λ Integrase bridges in the nucleoprotein Holliday junction intermediates of viral integrative and excisive recombination

Tong

Warren

Seah

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

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The site-specific recombinase encoded by bacteriophage λ [λ Integrase (Int)] is responsible for integrating and excising the viral chromosome into and out of the chromosome of its Escherichia coli host. In contrast to the other well-studied and highly exploited tyrosine recombinase family members, such as Cre and Flp, Int carries out a reaction that is highly directional, tightly regulated, and depends on an ensemble of accessory DNA bending proteins acting on 240 bp of DNA encoding 16 protein binding sites. This additional complexity enables two pathways, integrative and excisive recombination, whose opposite, and effectively irreversible, directions are dictated by different physiological and environmental signals. Int recombinase is a heterobivalent DNA binding protein that binds via its small amino-terminal domain to high affinity arm-type DNA sites and via its large, compound carboxyl-terminal domain to core-type DNA sites, where DNA cleavage and ligation are executed. Each of the four Int protomers, within a multiprotein 400-kDa recombinogenic complex, is thought to bind and, with the aid of DNA bending proteins, bridge one arm-and one core-type DNA site. Despite a wealth of genetic, biochemical, and functional information generated by many laboratories over the last 50 y, it has not been possible to decipher the patterns of Int bridges, an essential step in understanding the architectures responsible for regulated directionality of recombination. We used site-directed chemical cross-linking of Int in trapped Holliday junction recombination intermediates and recombination reactions with chimeric recombinases, to identify the unique and monogamous patterns of Int bridges for integrative and excisive recombination.site-specific recombination | regulation of directionality | recombinogenic architectures | molecular machines

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Section: Confirmation Of the Hj Int Bridges In Complete Recombinationmentioning

confidence: 99%

Mapping the λ Integrase bridges in the nucleoprotein Holliday junction intermediates of viral integrative and excisive recombination

Tong

Warren

Seah

et al. 2014

Proc. Natl. Acad. Sci. U.S.A.

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“…The simplicity of this system, requiring only a single recombinase enzyme and short recombination sequences for robust activity in a variety of contexts (15), has been an important factor in both cases. Cre has also been used in experiments designed to understand the functions of other recombination systems (16)(17)(18).…”

Section: Introductionmentioning

confidence: 99%

Cre Recombinase

Duyne

2015

Microbiol Spectr

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The use of Cre recombinase to carry out conditional mutagenesis of transgenes and insert DNA cassettes into eukaryotic chromosomes is widespread. In addition to the numerous in vivo and in vitro applications that have been reported since Cre was first shown to function in yeast and mammalian cells nearly 30 years ago, the Cre-loxP system has also played an important role in understanding the mechanism of recombination by the tyrosine recombinase family of site-specific recombinases. The simplicity of this system, requiring only a single recombinase enzyme and short recombination sequences for robust activity in a variety of contexts, has been an important factor in both cases. This review discusses advances in the Cre recombinase field that have occurred over the past 12 years since the publication of Mobile DNA II. The focus is on those recent contributions that have provided new mechanistic insights into the reaction. Also discussed are modifications of Cre and/or the loxP sequence that have led to improvements in genome engineering applications.

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“…An article in a recent issue of PNAS (4) provides important new insights into both questions. By making a chimeric protein composed of Cre recombinase fused to a small DNAbinding domain of -integrase, Warren et al (4) have turned the normally unregulated Cre into a regulated integrase with the same requirements and directionality found in the -integrase system.…”

mentioning

confidence: 99%

“…Because the presence of an armbinding N-domain is the most obvious difference between the Cre and -integrase proteins, Warren et al (4) asked whether adding an N-domain to Cre would lead to a novel recombinase with the regulatory properties of -integrase. To test this idea, they generated modified attP and attB sites for integration (called lotP and lotB) and modified attL and attR sites for excision (called lotL and lotR) in which the core -integrase binding sites were replaced by weakened Cre binding sites.…”

mentioning

confidence: 99%

“…The first could occur by simple mutation of the recombinase and/or the binding sites. The second could occur as the outcome of homologous recombination events, but Warren et al (4) point out that an alternative, more efficient mechanism could also play an important role. Many recombinase genes are located adjacent to their att sites, setting the stage for fusion with new sequences via site-specific recombination with weak att sites located within the recombinase gene and elsewhere in the bacterial genome.…”

mentioning

confidence: 99%

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