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Literature DB >> 11387225

Tipping the balance between replicative and simple transposition.

Abstract

The bacterial insertion sequence IS903 has the unusual ability to transpose both replicatively and non-replicatively. The majority of products are simple insertions, while co-integrates, the product of replicative transposition, occur at a low frequency (<0.1% of simple insertions). In order to define the critical steps that determine the outcome of IS903 transposition, we have isolated mutants that specifically increase the rate of replicative transposition. Here we show that the nucleotide immediately flanking the transposon influences both overall transposition frequency and co-integrate formation. In particular, when the 3'-flanking nucleotide is A, co-integrates are increased 500-fold compared with a 3' C. In addition, we have isolated five transposase mutants that increase replicative transposition. These residues are close to the catalytic residues and are thus likely to be part of the active site. These are the first transposase mutations described that affect the product of transposition. Our results are consistent with the hypothesis that a delay in cleavage of the 5'-flanking DNA will increase the effective half-life of the 3'-nicked transposon intermediate and consequently enhance co-integrate formation.

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Year: 2001 PMID： 11387225 PMCID： PMC125483 DOI： 10.1093/emboj/20.11.2923

Source DB: PubMed Journal: EMBO J ISSN： 0261-4189 Impact factor: 11.598

38 in total

1. Anatomy of a preferred target site for the bacterial insertion sequence IS903.

Authors: W Y Hu; W Thompson; C E Lawrence; K M Derbyshire
Journal: J Mol Biol Date: 2001-02-23 Impact factor: 5.469

Review 2. Transpositional recombination: mechanistic insights from studies of mu and other elements.

Authors: K Mizuuchi
Journal: Annu Rev Biochem Date: 1992 Impact factor: 23.643

3. Residues critical for retroviral integrative recombination in a region that is highly conserved among retroviral/retrotransposon integrases and bacterial insertion sequence transposases.

Authors: J Kulkosky; K S Jones; R A Katz; J P Mack; A M Skalka
Journal: Mol Cell Biol Date: 1992-05 Impact factor: 4.272

4. Tn7 transposition in vitro proceeds through an excised transposon intermediate generated by staggered breaks in DNA.

Authors: R Bainton; P Gamas; N L Craig
Journal: Cell Date: 1991-05-31 Impact factor: 41.582

Review 5. Efficient site-directed mutagenesis using uracil-containing DNA.

Authors: T A Kunkel; K Bebenek; J McClary
Journal: Methods Enzymol Date: 1991 Impact factor: 1.600

6. A specific class of IS10 transposase mutants are blocked for target site interactions and promote formation of an excised transposon fragment.

Authors: D B Haniford; A R Chelouche; N Kleckner
Journal: Cell Date: 1989-10-20 Impact factor: 41.582

7. Genetic analysis of the interaction of the insertion sequence IS903 transposase with its terminal inverted repeats.

Authors: K M Derbyshire; L Hwang; N D Grindley
Journal: Proc Natl Acad Sci U S A Date: 1987-11 Impact factor: 11.205

8. Analysis of the structure and function of the kanamycin-resistance transposon Tn903.

Authors: N D Grindley; C M Joyce
Journal: Cold Spring Harb Symp Quant Biol Date: 1981

9. Binding of the IS903 transposase to its inverted repeat in vitro.

Authors: K M Derbyshire; N D Grindley
Journal: EMBO J Date: 1992-09 Impact factor: 11.598

10. Structural aspects of a higher order nucleoprotein complex: induction of an altered DNA structure at the Mu-host junction of the Mu type 1 transpososome.

Authors: B D Lavoie; B S Chan; R G Allison; G Chaconas
Journal: EMBO J Date: 1991-10 Impact factor: 11.598

7 in total

1. Transposable element ISHp608 of Helicobacter pylori: nonrandom geographic distribution, functional organization, and insertion specificity.

Authors: Dangeruta Kersulyte; Billie Velapatiño; Giedrius Dailide; Asish K Mukhopadhyay; Yoshiyuki Ito; Lizbeth Cahuayme; Alan J Parkinson; Robert H Gilman; Douglas E Berg
Journal: J Bacteriol Date: 2002-02 Impact factor: 3.490

Tipping the balance between replicative and simple transposition.

1. Anatomy of a preferred target site for the bacterial insertion sequence IS903.

Review 2. Transpositional recombination: mechanistic insights from studies of mu and other elements.

3. Residues critical for retroviral integrative recombination in a region that is highly conserved among retroviral/retrotransposon integrases and bacterial insertion sequence transposases.

4. Tn7 transposition in vitro proceeds through an excised transposon intermediate generated by staggered breaks in DNA.

Review 5. Efficient site-directed mutagenesis using uracil-containing DNA.

6. A specific class of IS10 transposase mutants are blocked for target site interactions and promote formation of an excised transposon fragment.

7. Genetic analysis of the interaction of the insertion sequence IS903 transposase with its terminal inverted repeats.

8. Analysis of the structure and function of the kanamycin-resistance transposon Tn903.

9. Binding of the IS903 transposase to its inverted repeat in vitro.

10. Structural aspects of a higher order nucleoprotein complex: induction of an altered DNA structure at the Mu-host junction of the Mu type 1 transpososome.

1. Transposable element ISHp608 of Helicobacter pylori: nonrandom geographic distribution, functional organization, and insertion specificity.

2. Requirement of IS911 replication before integration defines a new bacterial transposition pathway.

3. Estimating the fitness effect of an insertion sequence.

4. Homologues of bacterial TnpB_IS605 are widespread in diverse eukaryotic transposable elements.

5. Characteristics of MuA transposase-catalyzed processing of model transposon end DNA hairpin substrates.

6. Identification and Characterisation of pST1023 A Mosaic, Multidrug-Resistant and Mobilisable IncR Plasmid.

7. Alternative mechanisms for tn5 transposition.