A single oligonucleotide can be used to rapidly isolate DNA sequences flanking a transposon Tn5 insertion by the polymerase chain reaction

doi:10.1093/nar/18.22.6673

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Nucleic Acids Research, 1990, Vol. 18, No. 22 6673-6676
© 1990

MOLECULAR BIOLOGY

A single oligonucleotide can be used to rapidly isolate DNA sequences flanking a transposon Tn5 insertion by the polymerase chain reaction

Jessica J. Rich¹ and David K. Willis¹^,2^,*

¹Department of Plant Pathology, University of Wisconsin Madison, Wl 53706, USA ²ARS/USDA Plant Disease Resistance Research Unit, University of Wisconsin Madison, Wl 53706, USA

^* To whom correspondence should be addressed

Received May 9, 1990. Revised October 9, 1990. Accepted October 9, 1990.

We have developed a strategy to rapidly construct DNA hybridizationprobes for the isolation of genes disrupted by transposon Tn5insertions. A single oligonucleotide complementary to and extendingoutward from the ends of the inverted repeat of Tn5 was usedto prime DNA synthesis in the polymerase chain reaction. Theamplified product consisted of DNA sequences adjacent to bothends of the transposon insertion. The general feasibility ofthe approach was tested by amplifying pBR322 sequences froma derivative of pBR322 containing a Tn5 insertion. To amplifygenomic DNA sequences flanking a Tn5 insertion in the chromosomeof a Pseudomonas syrlngae strain, circular substrates were generatedby ligating EcoRI-digested genomic DNA. Tn5 was contained intactwithin one such circular molecule, as the transposon does notcontain sites for cleavage by EcoRI. The amplified product ( $~$ 2.5kb) was used as a DNA hybridization probe to isolate the homologousfragment from a cosmid library of wild-type Pseudomonas syrlngaegenomic DNA. This approach may be applied to the efficient isolationof sequences flanking any Tn5 insertion.

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