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Genome research, Vol. 11, No. 6. (01 June 2001), pp. 1095-1099, doi:10.1101/gr.180501 Key: citeulike:707170
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We describe a simple method of using rolling circle amplification to amplify vector DNA such as M13 or plasmid DNA from single colonies or plaques. Using random primers and phi29 DNA polymerase, circular DNA templates can be amplified 10,000-fold in a few hours. This procedure removes the need for lengthy growth periods and traditional DNA isolation methods. Reaction products can be used directly for DNA sequencing after phosphatase treatment to inactivate unincorporated nucleotides. Amplified products can also be used for in vitro cloning, library construction, and other molecular biology applications.
This methods described in this article are very useful for amplification of pure plasmids in vitro. Applications include preparation of transfection grade plasmids, free of endotoxins.
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