Your search keyword '"Crouse GF"' showing total 5 results

1. Mutagenesis assays in yeast.

Author

Crouse GF

Subjects

DNA Damage, DNA Repair, Gene Deletion, Point Mutation, DNA Mutational Analysis methods, Mutagenicity Tests methods, Plasmids genetics, Yeasts genetics

Abstract

Analyzing mutation spectra is a very powerful method to determine the effects of various types of DNA damage and to understand the workings of various DNA repair pathways. However, compiling sequence-specific mutation spectra is laborious; even with modern sequencing technology, it is rare to obtain spectra with more than several hundred data points. Two assay systems are described for yeast, one for insertion/deletion mutations and one for base substitution mutations, that allow determination of specific mutations without the necessity of DNA sequencing. The assay for insertion/deletion mutations uses a variety of different simple repeats placed in frame with URA3 such that insertions or deletions lead to a selectable Ura(-) phenotype; essentially all such mutations are in the simple repeat sequence. The assay for base substitution mutations uses a series of six strains with different mutations in one essential codon of the CYC1 gene. Because only true reversions lead to a selectable phenotype, the bases mutated in any reversion event are known. The advantage of these assays is that they can quantitatively determine over several orders of magnitude the types of mutations that occur under a given set of conditions, without DNA sequencing., (Copyright 2000 Academic Press.)

Published

2000

2. Gene engineering by selectable intraplasmid recombination: construction of novel dihydrofolate reductase minigenes.

Author

Crouse GF, New L, and Stivaletta LA

Subjects

Animals, Base Sequence, Cloning, Molecular methods, DNA, Recombinant metabolism, Escherichia coli genetics, Exons, Galactokinase genetics, Genetic Engineering methods, Introns, Mice, Molecular Sequence Data, Promoter Regions, Genetic, Restriction Mapping, Genes, Plasmids, Tetrahydrofolate Dehydrogenase genetics

Abstract

An intraplasmid recombination system in Escherichia coli has been designed to make possible the engineering of various genes using methods that greatly reduce dependence on appropriately placed restriction enzyme sites. This system has been used to manipulate intervening sequences in dihydrofolate reductase minigenes and to vary the number of 48-bp repeats in the promoter region. In this method, the two fragments to be recombined are cloned into a plasmid separated by a fragment of DNA containing an expressible galactokinase-encoding gene (galK). Selection for loss of the galK gene, but for retention of the plasmid in E. coli, results in a plasmid in which the two fragments have undergone homologous recombination. Several new plasmids are reported here which contain an expressible galK gene flanked by multiple restriction sites. These plasmids should be useful in recombination and as convenient sources of a gene for which both positive and negative selections are available in E. coli.

Published

1989

3. An integrated and simplified approach to cloning into plasmids and single-stranded phages.

Author

Crouse GF, Frischauf A, and Lehrach H

Subjects

DNA Restriction Enzymes, Genetic Engineering methods, Genetic Vectors, Cloning, Molecular, Coliphages genetics, DNA, Single-Stranded genetics, Escherichia coli genetics, Plasmids

Published

1983

4. Restriction map of the region surrounding the EcoRI site in the pCR1 plasmid and analysis of an inserted ovalbumin gene.

Author

Wickens MP, Buell GN, Crouse GF, Carbon J, and Schimke RT

Subjects

Base Sequence, Chromosome Mapping, Chromosomes, Bacterial, DNA, Bacterial genetics, Escherichia coli drug effects, Genes, Kanamycin pharmacology, Transferases genetics, Transformation, Bacterial, DNA Restriction Enzymes genetics, DNA, Recombinant, Escherichia coli genetics, Ovalbumin genetics, Plasmids

Abstract

We have determined a restriction map of a 1650 base pair region surrounding the EcoRI site of the bacterial plasmid, pCR1. We have used pCR1 as a vector in cloning synthetic ovalbumin double-stranded cDNA. Using the pCR1 restriction map, we have characterized the ovalbumin sequences inserted in one recombinant plasmid, pOvE12. POvE12 appears to contain all, or nearly all, of the sequences found in full length, double-stranded cDNA synthesized in vitro.

Published

1979

5. Plasmids supplying the Q-qut-controlled gam function permit growth of lambda red- gam- (Fec-) bacteriophages on recA- hosts.

Author

Crouse GF

Subjects

DNA Restriction Enzymes, Escherichia coli genetics, Genes, Bacterial, Genotype, Mutation, Promoter Regions, Genetic, Bacteriophage lambda genetics, Genes, Viral, Plasmids

Abstract

A plasmid, pgam, has been constructed which expresses the phage lambda gene, gam, under the control of the lambda late promoter, p'R, contained in a form of a p'R-qut-t'R1 module. Lambda red- gam-, which normally do not grow on recA- hosts, are able to grow on recA- hosts containing pgam, because their Q function can turn on the gam gene expression. This facilitates cloning with lambda red- gam- vectors in recA- hosts.

Published

1985