Nucleic Acids Research, Vol 26, Issue 15 3611-3613, Copyright © 1998 by Oxford University Press
TL Criswell and S Bradshaw
Manipulation of genomic inserts cloned into the bacteriophage P1 vector is
hindered by the large size of the inserts. We have used co- transformation
mediated recombination between the yeast-bacteria shuttle vector, pClasper,
and various P1 clones to transfer the entire insert from the P1 into
pClasper. This results in the insert being stably maintained in yeast,
facilitating mutagenesis by homologous recombination. The recombinant
plasmid can subsequently be transferred to and stably maintained in
bacteria for efficient plasmid preparation. This method can also be applied
to inserts from P1 artificial chromosome or bacterial artificial chromosome
vectors.
ARTICLES
Transfer of P1 inserts into a yeast-bacteria shuttle vector by co- transformation mediated homologous recombination
Department of Biological Sciences, PO Box 210006, University of Cincinnati, Cincinnati, OH 45221-0006, USA.
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