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Primer protein of bacteriophage M2 exposes the RGD receptor site upon linking the first deoxynucleotide
Authors:Christina Lyra   Harri Savilahti  Dennis H. Bamford
Affiliation:(1) Department of Genetics, University of Helsinki, Arkadiankatu 7, SF-00100 Helsinki, Finland
Abstract:Summary Using electroporation with the phage PRD1 genome, we set up a high-frequency DNA transfer system for a linear dsDNA molecule with 5prime-covalently linked terminal proteins. The transfer was saturated when more than 100 ng of PRD1 genome was used. Electroporation efficiency was about four orders of magnitude higher than that obtained with transfection. Removal of the terminal protein abolished plaque formation, which could not be rescued by supplying the terminal protein or phage DNA polymerase or both in trans.
Keywords:Linear DNA  Electroporation  Transfection  DNA terminal protein  Bacteriophage PRD1
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