Restriction enzyme-mediated DNA family shuffling
Description
DNA shuffling is an established recombinatorial method that was originally developed to increase the speed of directed evolution experiments beyond what could be accomplished using error-prone PCR alone. To achieve this, mutated copies of a protein-coding sequence are fragmented with DNase I and the fragments are then reassembled in a PCR without primers. The fragments anneal where there is sufficient sequence identity, resulting in full-length variants of the original gene that have inherited mutations from multiple templates. Subsequent studies demonstrated that directed evolution could be further accelerated by shuffling similar native protein-coding sequences from the same gene family, rather than mutated variants of a single gene. Generally at least 65-75 % global identity between parental sequences is required in DNA family shuffling, with recombination mostly occurring at sites with at least five consecutive nucleotides of local identity. Since DNA shuffling was originally developed, many variations on the method have been published. In particular, the use of restriction enzymes in the fragmentation step allows for greater customization of fragment lengths than DNase I digestion and avoids the risk that parental sequences may be over-digested into unusable very small fragments. Restriction enzyme-mediated fragmentation also reduces the occurrence of undigested parental sequences that would otherwise reduce the number of unique variants in the resulting library. In the current chapter, we provide a brief overview of the alternative methods currently available for DNA shuffling as well as a protocol presented here that improves on several previous implementations of restriction enzyme-mediated DNA family shuffling, in particular with regard to purification of DNA fragments for reassembly.
Impact and interest:
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| ID Code: | 233130 | ||||
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| Item Type: | Chapter in Book, Report or Conference volume (Chapter) | ||||
| Series Name: | Methods in Molecular Biology | ||||
| ORCID iD: |
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| Measurements or Duration: | 13 pages | ||||
| Keywords: | DNA shuffling, Mutant libraries, Protein engineering, Restriction enzyme | ||||
| DOI: | 10.1007/978-1-4939-1053-3_12 | ||||
| ISBN: | 978-1-4939-1052-6 | ||||
| Pure ID: | 112018556 | ||||
| Copyright Owner: | 2014 Springer Science+Business Media New York | ||||
| Copyright Statement: | This work is covered by copyright. Unless the document is being made available under a Creative Commons Licence, you must assume that re-use is limited to personal use and that permission from the copyright owner must be obtained for all other uses. If the document is available under a Creative Commons License (or other specified license) then refer to the Licence for details of permitted re-use. It is a condition of access that users recognise and abide by the legal requirements associated with these rights. If you believe that this work infringes copyright please provide details by email to qut.copyright@qut.edu.au | ||||
| Deposited On: | 30 Jun 2022 05:03 | ||||
| Last Modified: | 02 Mar 2024 03:12 |
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