Bacteriophage lambda cloning vehicles for studies of genetic recombination |
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Authors: | D Carroll R S Ajioka C Georgopoulos |
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Institution: | Department of Cellular, Viral and Molecular Biology, University of Utah Medical Center, Salt Lake City, UT 84132 U.S.A. |
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Abstract: | A pair of bacteriophage lambda cloning vehicles has been constructed for use in studies of genetic recombination. These phages, lambda rva and lambda rvb, have the following properties: (1) Each vector has a single HindIII site in the immunity region, at which segments of DNA can be inserted. (2) These HindIII sites are flanked by selectable markers with the following phenotypes: Spi+/- (Fec+/-) to the left, and imm lambda or imm434 to the right. (3) There is essentially no sequence homology between the two phages in this region, so recombination of the markers at reasonable frequency depends on the presence of homologous inserts at the HindIII sites. As a consequence, recovered recombinants must have resulted from a crossover event within the insert DNA. Restriction enzyme maps of the vectors have been determined. Variants of the original vectors have been isolated which permit separate examination of the viral (Red) and bacterial (Rec) generalized recombination mechanisms, and which provide a standard interval to which frequencies of recombination in cloned DNAs can be compared. |
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Keywords: | Recombinant DNA restriction enzyme maps Rec system Red system bp base pairs %λ unit 490 bp |
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