Rapid Amplification of Plasmid and Phage DNA Using Phi29 DNA Polymerase and Multiply-Primed Rolling Circle Amplification

  1. Frank B. Dean1,3,
  2. John R. Nelson2,3,
  3. Theresa L. Giesler2, and
  4. Roger S. Lasken1,4
  1. 1Molecular Staging, Inc., New Haven, Connecticut 06511, USA; 2Amersham Pharmacia Biotech, Piscataway, New Jersey 08855-1327, USA

Abstract

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 φ29 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.

Footnotes

  • 3 These authors contributed equally to this work.

  • 4 Corresponding author.

  • E-MAIL rogerl{at}molecularstaging.com; FAX (203) 776-5276.

  • Article and publication are at www.genome.org/cgi/doi/10.1101/gr.180501.

    • Received November 18, 2000.
    • Accepted March 22, 2001.
| Table of Contents

This Article

  1. doi: 10.1101/gr.180501 Genome Res. 11: 1095-1099 Cold Spring Harbor Laboratory Press

Article Category

Share

Preprint Server



Current Issue

  1. February 2024, 34 (2)
  1. Current Issue
  1. Alert me to new issues of Genome Research