Methylation of single-stranded DNA in vitro introduces new restriction endonuclease cleavage sites (original) (raw)
- Letter
- Published: 01 March 1978
Nature volume 272, pages 375–377 (1978)Cite this article
Abstract
RESTRICTION endonucleases recognise specific sequences in DNA, and these endonucleases, especially those which generate cohesive ends, have been widely used to clone DNA1. However, many DNAs lack sequences which are recognised by endonucleases such as _Eco_RI, _Hin_dIII or _Bam_HI. A general method of overcoming this problem has been described recently2. This approach involves the synthesis of oligonucleotides sensitive to a specific endonuclease and the blunt end ligation of these molecules to the DNA to be cloned. In contrast, we sought a method which avoids the insertion of additional nucleotides into a DNA sequence, but depends on direct modification of DNA. If a DNA sequence differs in only one base pair from the recognition sequence of a restriction endonuclease, a particular change of this base pair will generate the proper sequence. Here we describe a way of generating restriction endonuclease cleavage sites by single base changes derived after in vitro methylation of single-stranded DNA.
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Author notes
- JOACHIM MESSING
Present address: Department of Bacteriology, University of California, Davis, California, 95616
Authors and Affiliations
- Institut für Genetik der Universität zu Köln, Weyertal 121, 5000, Köln, 41, FRG
BRUNO GRONENBORN - Max-Planck Institut für Biochemie, 8033, Martinsried, FRG
JOACHIM MESSING
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- BRUNO GRONENBORN
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GRONENBORN, B., MESSING, J. Methylation of single-stranded DNA in vitro introduces new restriction endonuclease cleavage sites.Nature 272, 375–377 (1978). https://doi.org/10.1038/272375a0
- Received: 30 December 1977
- Accepted: 20 January 1978
- Published: 01 March 1978
- Issue Date: 23 March 1978
- DOI: https://doi.org/10.1038/272375a0