Functional analysis reports. Precise gene disruption in <i>Saccharomyces cerevisiae</i> by double fusion polymerase chain reaction

David C. Amberg(Stanford University), David Botstein(Stanford University), Ellen M. Beasley(Stanford University)
Yeast
October 1, 1995
10.1002/yea.320111307
Cited by 125

Abstract

We adapted a fusion polymerase chain reaction (PCR) strategy to synthesize gene disruption alleles of any sequenced yeast gene of interest. The first step of the construction is to amplify sequences flanking the reading frame we want to disrupt and to amplify the selectable marker sequence. Then we fuse the upstream fragment to the marker sequence by fusion PCR, isolate this product and fuse it to the downstream sequence in a second fusion PCR reaction. The final PCR product can then be transformed directly into yeast. This method is rapid, relatively inexpensive, offers the freedom to choose from among a variety of selectable markers and allows one to construct precise disruptions of any sequenced open reading frame in Saccharomyces cerevisiae.

Related Papers

Molecular Cloning: A Laboratory Manual
Joseph Sambrook, Elisabeth Fritsch, Tom Maniatis|Unknown|1989|130k
Molecular cloning: A laboratory manual
Prescott L. Deininger|Analytical Biochemistry|1990|86.2k
Site-directed mutagenesis by overlap extension using the polymerase chain reaction
Steffan N. Ho, Henry D. Hunt, Robert M. Horton et al.|Gene|1989|7.5k
[12] One-step gene disruption in yeast
Rodney Rothstein|Methods in enzymology on CD-ROM/Methods in enzymology|1983|3.3k
New heterologous modules for classical or PCR‐based gene disruptions in <i>Saccharomyces cerevisiae</i>
Achim Wach, Arndt Brachat, Rainer Pöhlmann et al.|Yeast|1994|2.6k