Insertional mutagenesis by a modified in vitro Ty1 transposition system

Levi A. Garraway; Luiz R.O. Tosi; Yixin Wang; Jeffrey B. Moore; Deborah E. Dobson; Stephen M. Beverley

doi:10.1016/s0378-1119(97)00288-6

Insertional mutagenesis by a modified in vitro Ty1 transposition system

Levi A. Garraway, Luiz R.O. Tosi, Yixin Wang, Jeffrey B. Moore, Deborah E. Dobson, Stephen M. Beverley

Research output: Contribution to journal › Article › peer-review

23 Scopus citations

Abstract

Transposable elements are useful tools for insertional mutagenesis and have many potential applications in the characterization of complex genomes. Here we describe a system which facilitates the construction of large transposon insertion libraries useful for genome sequencing and functional genomic analysis. We developed two transposons, TyK and TyK'GFP + , which can be introduced into target DNAs by Ty1-mediated transposition in vitro, and several modifications which decrease the frequency of false transposition events and direct the recovery of transpositions into passenger rather than vector DNA. Insertions of TyK'GFP+ additionally may yield fusions to the Aequorea green fluorescent protein (GFP), useful in studies of gene expression and protein targeting. Transposition in vitro was obtained into target DNAs of up to 50 kb in size, restriction mapping showed insertion to be relatively random, and the sequence of 55 insertion sites showed neither strong site nor base compositional preference. Our data suggest that TyK-based artificial transposons will be suitable for a variety of genetic applications in many organisms.

Original language	English
Pages (from-to)	27-35
Number of pages	9
Journal	Gene
Volume	198
Issue number	2 JAN
DOIs	https://doi.org/10.1016/s0378-1119(97)00288-6
State	Published - 1997

Keywords

DNA sequencing
Gene fusions
Green fluorescent protein
Transposon

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10.1016/s0378-1119(97)00288-6

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@article{890b81290cb643949cd7ea9beb6c033a,

title = "Insertional mutagenesis by a modified in vitro Ty1 transposition system",

abstract = "Transposable elements are useful tools for insertional mutagenesis and have many potential applications in the characterization of complex genomes. Here we describe a system which facilitates the construction of large transposon insertion libraries useful for genome sequencing and functional genomic analysis. We developed two transposons, TyK and TyK'GFP + , which can be introduced into target DNAs by Ty1-mediated transposition in vitro, and several modifications which decrease the frequency of false transposition events and direct the recovery of transpositions into passenger rather than vector DNA. Insertions of TyK'GFP+ additionally may yield fusions to the Aequorea green fluorescent protein (GFP), useful in studies of gene expression and protein targeting. Transposition in vitro was obtained into target DNAs of up to 50 kb in size, restriction mapping showed insertion to be relatively random, and the sequence of 55 insertion sites showed neither strong site nor base compositional preference. Our data suggest that TyK-based artificial transposons will be suitable for a variety of genetic applications in many organisms.",

keywords = "DNA sequencing, Gene fusions, Green fluorescent protein, Transposon",

author = "Garraway, {Levi A.} and Tosi, {Luiz R.O.} and Yixin Wang and Moore, {Jeffrey B.} and Dobson, {Deborah E.} and Beverley, {Stephen M.}",

note = "Funding Information: We thank G. Fink for yeast strain JB224, E.I. Vivas and M. Dziejman for plasmids used in construction of pTyK, S. Chiang for DH5 α λ pir , S. Cilmi for pSC1 and Lynne Garrity for ID-2; C. Andre, J. Boeke, J. Brookman and members of K. Struhl's laboratory for advice and discussions; and F. Gueiros-Filho for comments on this manuscript. This work was supported by NRSA Fellowships HG00092 (L.A.G.) and AI09382 (Y.W.), a NSERC Canada Fellowship (J.B.M.) and NIH grants to D.E.D. and S.M.B. L.R.O.T. is a PEW Latin American Fellow. ",

year = "1997",

doi = "10.1016/s0378-1119(97)00288-6",

language = "English",

volume = "198",

pages = "27--35",

journal = "Gene",

issn = "0378-1119",

number = "2 JAN",

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TY - JOUR

T1 - Insertional mutagenesis by a modified in vitro Ty1 transposition system

AU - Garraway, Levi A.

AU - Tosi, Luiz R.O.

AU - Wang, Yixin

AU - Moore, Jeffrey B.

AU - Dobson, Deborah E.

AU - Beverley, Stephen M.

N1 - Funding Information: We thank G. Fink for yeast strain JB224, E.I. Vivas and M. Dziejman for plasmids used in construction of pTyK, S. Chiang for DH5 α λ pir , S. Cilmi for pSC1 and Lynne Garrity for ID-2; C. Andre, J. Boeke, J. Brookman and members of K. Struhl's laboratory for advice and discussions; and F. Gueiros-Filho for comments on this manuscript. This work was supported by NRSA Fellowships HG00092 (L.A.G.) and AI09382 (Y.W.), a NSERC Canada Fellowship (J.B.M.) and NIH grants to D.E.D. and S.M.B. L.R.O.T. is a PEW Latin American Fellow.

PY - 1997

Y1 - 1997

N2 - Transposable elements are useful tools for insertional mutagenesis and have many potential applications in the characterization of complex genomes. Here we describe a system which facilitates the construction of large transposon insertion libraries useful for genome sequencing and functional genomic analysis. We developed two transposons, TyK and TyK'GFP + , which can be introduced into target DNAs by Ty1-mediated transposition in vitro, and several modifications which decrease the frequency of false transposition events and direct the recovery of transpositions into passenger rather than vector DNA. Insertions of TyK'GFP+ additionally may yield fusions to the Aequorea green fluorescent protein (GFP), useful in studies of gene expression and protein targeting. Transposition in vitro was obtained into target DNAs of up to 50 kb in size, restriction mapping showed insertion to be relatively random, and the sequence of 55 insertion sites showed neither strong site nor base compositional preference. Our data suggest that TyK-based artificial transposons will be suitable for a variety of genetic applications in many organisms.

AB - Transposable elements are useful tools for insertional mutagenesis and have many potential applications in the characterization of complex genomes. Here we describe a system which facilitates the construction of large transposon insertion libraries useful for genome sequencing and functional genomic analysis. We developed two transposons, TyK and TyK'GFP + , which can be introduced into target DNAs by Ty1-mediated transposition in vitro, and several modifications which decrease the frequency of false transposition events and direct the recovery of transpositions into passenger rather than vector DNA. Insertions of TyK'GFP+ additionally may yield fusions to the Aequorea green fluorescent protein (GFP), useful in studies of gene expression and protein targeting. Transposition in vitro was obtained into target DNAs of up to 50 kb in size, restriction mapping showed insertion to be relatively random, and the sequence of 55 insertion sites showed neither strong site nor base compositional preference. Our data suggest that TyK-based artificial transposons will be suitable for a variety of genetic applications in many organisms.

KW - DNA sequencing

KW - Gene fusions

KW - Green fluorescent protein

KW - Transposon

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U2 - 10.1016/s0378-1119(97)00288-6

DO - 10.1016/s0378-1119(97)00288-6

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SN - 0378-1119

VL - 198

SP - 27

EP - 35

JO - Gene

JF - Gene

IS - 2 JAN

ER -

Insertional mutagenesis by a modified in vitro Ty1 transposition system

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Keywords

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