<i>In vitro</i>
            site-specific integration of bacteriophage DNA catalyzed by a recombinase of the resolvase/invertase family

Thorpe, Helena; Smith, Margaret Caroline MacHin

doi:10.1073/pnas.95.10.5505

Cited by 405 publications

(372 citation statements)

References 37 publications

Supporting

Mentioning

353

Contrasting

Order By: Relevance

“…ϕC31 is a bacteriophage that encodes an integrase that mediates sequence directed recombination between a 34 nucleotide long bacterial attachment site (attB) and a 39 base-pair long phage attachment site (attP). ϕC31 integrase has a high efficiency of recombination, requires no accessory factors 5,6 and has been effectively used to integrate genes into plant cells 7 , mammalian cells 1,[8][9][10][11][12][13] , and Drosophila 14 . The ϕC31 integrase does not require an attP site to have perfect sequence fidelity for it to be recognized and cleaved 9 .…”

Section: Introductionmentioning

confidence: 99%

Transgenic Xenopus laevis embryos can be generated using φC31 integrase

2005

View full text Add to dashboard Cite

Phage ϕC31 encodes an integrase that can mediate the insertion of extrachromosomal DNA into genomic DNA 1 . Here we show ϕC31 integrase can be used to generate transgenic Xenopus laevis embryos. mRNA encoding integrase was co-injected with a reporter plasmid containing a CMV promoter driven GFP into one cell embryos. The reporter plasmid was integrated into the genome. GFP expression, though robust, was in a limited number of tissues and varied among the embryos analyzed. We attributed this restriction to transcriptional silencing by chromosome position effects. Modification of the reporter plasmid by bracketing the CMV-GFP region with tandem copies of the chicken β-globin 5′ HS4 insulator 2 relieved position effects. Embryos transgenic with insulated CMV-GFP expressed GFP uniformly. Tissue specific expression was achieved when the CMV promoter was replaced with a 551 base-pair minimal gamma crystallin lens promoter from Xenopus. Embryos transgenic with this plasmid had GFP expression limited to the lens of the eye. We observed that about a third of embryos assayed one week after fertilization were transgenic. These experiments demonstrate that the integration of insulated gene sequences using ϕC31 integrase can be used to efficiently create transgenic embryos in Xenopus laevis and may increase the practical use of ϕC31 integrase in other systems as well.The ability to generate transgenic animals has revolutionized studies on gene function. Transgenic frogs of the genus Xenopus have been made using methods based on a restriction-enzyme mediated sperm integration approach described by Kroll and Amaya 3 . This method has been remarkably successful, but can be technically demanding. In addition, many embryos contain multiple copies of the transgene inserted at random insertion sites 3, 4 .We have tried an alternative approach, creating transgenic Xenopus embryos by using ϕC31 integrase mediated recombination. ϕC31 is a bacteriophage that encodes an integrase that mediates sequence directed recombination between a 34 nucleotide long bacterial attachment site (attB) and a 39 base-pair long phage attachment site (attP). ϕC31 integrase has a high efficiency of recombination, requires no accessory factors 5,6 and has been effectively used to integrate genes into plant cells 7 , mammalian cells 1,[8][9][10][11][12][13] , and Drosophila 14 . The ϕC31 integrase does not require an attP site to have perfect sequence fidelity for it to be recognized and cleaved 9 . These imperfect attP sites, or psuedo-attP sites, may have a similarity as low as 24% to an attP site and still allow recombination 9 . It has been estimated that a mammalian genome may contain 100-1000 psuedo attP sites 9 . Since the Xenopus laevis genome is approximately the same size as a mammalian genome (3×10 9 base pairs), we hypothesized that there would also be psuedo-attP sites in its genome that could be used to create transgenic Xenopus embryos. In the experiments that follow all the figure 1e. The half life of the GFP protein has been estimate...

show abstract

Section: Introductionmentioning

confidence: 99%

Transgenic Xenopus laevis embryos can be generated using φC31 integrase

2005

View full text Add to dashboard Cite

show abstract

“…In other organisms, methods utilizing site-specific recombination, instead of homologous recombination, have allowed much higher integration efficiencies (e.g., Lyznik et al 2003, Schweizer 2003, and references therein). One particularly useful site-specific recombinase system utilizes the Streptomyces bacteriophage φC31 integrase (Thorpe and Smith 1998).…”

Section: Introductionmentioning

confidence: 99%

New methods for tightly regulated gene expression and highly efficient chromosomal integration of cloned genes for Methanosarcina species

Guss

Rother

Zhang

et al. 2008

Archaea

117

179

View full text Add to dashboard Cite

Summary A highly efficient method for chromosomal integration of cloned DNA into Methanosarcina spp. was developed utilizing the site-specific recombination system from the Streptomyces phage φC31. Host strains expressing the φC31 integrase gene and carrying an appropriate recombination site can be transformed with non-replicating plasmids carrying the complementary recombination site at efficiencies similar to those obtained with self-replicating vectors. We have also constructed a series of hybrid promoters that combine the highly expressed M. barkeri PmcrB promoter with binding sites for the tetracycline-responsive, bacterial TetR protein. These promoters are tightly regulated by the presence or absence of tetracycline in strains that express the tetR gene. The hybrid promoters can be used in genetic experiments to test gene essentiality by placing a gene of interest under their control. Thus, growth of strains with tetR-regulated essential genes becomes tetracycline-dependent. A series of plasmid vectors that utilize the site-specific recombination system for construction of reporter gene fusions and for tetracycline regulated expression of cloned genes are reported. These vectors were used to test the efficiency of translation at a variety of start codons. Fusions using an ATG start site were the most active, whereas those using GTG and TTG were approximately one half or one fourth as active, respectively. The CTG fusion was 95% less active than the ATG fusion.

show abstract

“…Using hydrodynamic injection, delivery of a SB-containing plasmid along with a plasmid containing F.IX transgene resulted in robust long-term hF.IX expression in mice (178). Similarly, hydrodynamic gene transfer using the ΦC31 integrase (derived from a bacteriophage) induced persistent F.IX expression in hemophilic mice (179)(180)(181). However, as previously mentioned, this procedure is currently not applicable to larger animal models.…”

Section: Integrases and Non-viral Approachesmentioning

confidence: 91%

Gene therapy for hemophilia

2001

Indian J Pediatr

View full text Add to dashboard Cite

Hemophilia is an X-linked inherited bleeding disorder consisting of two classifications, hemophilia A and hemophilia B, depending on the underlying mutation. Although the disease is currently treatable with intravenous delivery of replacement recombinant clotting factor, this approach represents a significant cost both monetarily and in terms of quality of life. Gene therapy is an attractive alternative approach to the treatment of hemophilia that would ideally provide lifelong correction of clotting activity with a single injection. In this review, we will discuss the multitude of approaches that have been explored for the treatment of both hemophilia A and B, including both in vivo and ex vivo approaches with viral and nonviral delivery vectors.

show abstract

In vitro site-specific integration of bacteriophage DNA catalyzed by a recombinase of the resolvase/invertase family

Cited by 405 publications

References 37 publications

Transgenic Xenopus laevis embryos can be generated using φC31 integrase

Transgenic Xenopus laevis embryos can be generated using φC31 integrase

New methods for tightly regulated gene expression and highly efficient chromosomal integration of cloned genes for Methanosarcina species

Gene therapy for hemophilia

Contact Info

Product

Resources

About