Use of interplasmid recombination to generate stable selectable markers for yeast transformation: application to studies of actin gene control

A plasmid recombination system has been developed that relies upon interplasmid exchanges for yeast cell viability. Two types of plasmids, one carrying the LEU2 allele inserted within yeast actin gene sequences and the other carrying 2-microns plasmid DNA and an intact actin gene, were constructed....

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Bibliographic Details
Published inGenome Vol. 33; no. 5; pp. 696 - 706
Main Authors Hubberstey, A.V, Wildeman, A.G
Format Journal Article
LanguageEnglish
Published Canada 01.10.1990
Subjects
actin
Actins - genetics
Base Sequence
Blotting, Northern
Blotting, Southern
Escherichia coli - genetics
Gene Expression
Genetic Markers
genetic regulation
genetic transformation
homologous recombination
Molecular Sequence Data
Mutation
nucleotide sequences
Plasmids
Promoter Regions, Genetic
Recombination, Genetic
Restriction Mapping
Saccharomyces cerevisiae
Saccharomyces cerevisiae - genetics
Transformation, Genetic
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Summary:A plasmid recombination system has been developed that relies upon interplasmid exchanges for yeast cell viability. Two types of plasmids, one carrying the LEU2 allele inserted within yeast actin gene sequences and the other carrying 2-microns plasmid DNA and an intact actin gene, were constructed. Neither plasmid alone yielded transformants in the haploid Leu- strain AH22, but when cotransformed, a number of colonies were obtained. Southern blot analysis revealed that transformants arose because of recombination events within the homologous actin sequences that transferred the LEU2 gene to the actin gene on the 2-microns plasmid. The recombinant plasmids could be recovered, and sequence analysis of one recombination site revealed that the exchange event was faithful at the nucleotide level. The resulting recombinant plasmids carried a defective actin gene and presumably arose because of a double-crossover event. Deletion mutations that prevented actin gene expression on one donor plasmid enabled the recovery at a high frequency of transformants resulting primarily from single-crossover events between the two plasmids. This was presumably because such events no longer generated an intact actin gene on a multicopy plasmid. Infrequently a transformant from a plasmid with an intact gene was recovered, but in these cases the plasmid was not present in multiple copies. These cells exhibited a slower growth rate, and Northern blot analysis revealed an elevated level of actin mRNA.
ISSN:0831-2796
1480-3321
DOI:10.1139/g90-105