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Letter
Nature 448, 828-831 (16 August 2007) | doi:10.1038/nature06032; Received 21 February 2007; Accepted 19 June 2007; Corrected 18 October 2007
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Multiple Postdoctoral Positions
- University of Iowa
- Coralville, Iowa, USA
Assistant Professor and Associate Professor
- Massachusetts General Hospital/ Harvard Medical School
- Charlestown, MA
Selection and evolution of enzymes from a partially randomized non-catalytic scaffold
Burckhard Seelig1 & Jack W. Szostak1
- Howard Hughes Medical Institute, Department of Molecular Biology, and Center for Computational and Integrative Biology (CCIB), 7215 Simches Research Center, Massachusetts General Hospital, 185 Cambridge Street, Boston, Massachusetts 02114, USA
Correspondence to: Correspondence and requests for materials should be addressed to J.W.S. (Email: szostak@molbio.mgh.harvard.edu).
Abstract
Enzymes are exceptional catalysts that facilitate a wide variety of reactions under mild conditions, achieving high rate-enhancements with excellent chemo-, regio- and stereoselectivities. There is considerable interest in developing new enzymes for the synthesis of chemicals and pharmaceuticals1, 2, 3 and as tools for molecular biology. Methods have been developed for modifying and improving existing enzymes through screening, selection and directed evolution4, 5. However, the design and evolution of truly novel enzymes has relied on extensive knowledge of the mechanism of the reaction6, 7, 8, 9, 10. Here we show that genuinely new enzymatic activities can be created de novo without the need for prior mechanistic information by selection from a naive protein library of very high diversity, with product formation as the sole selection criterion. We used messenger RNA display, in which proteins are covalently linked to their encoding mRNA11, to select for functional proteins from an in vitro translated protein library of >1012 independent sequences without the constraints imposed by any in vivo step. This technique has been used to evolve new peptides and proteins that can bind a specific ligand12, 13, 14, 15, 16, 17, 18, from both random-sequence libraries12, 14, 15, 16 and libraries based on a known protein fold17, 18. We now describe the isolation of novel RNA ligases from a library that is based on a zinc finger scaffold18, 19, followed by in vitro directed evolution to further optimize these enzymes. The resulting ligases exhibit multiple turnover with rate enhancements of more than two-million-fold.
- Howard Hughes Medical Institute, Department of Molecular Biology, and Center for Computational and Integrative Biology (CCIB), 7215 Simches Research Center, Massachusetts General Hospital, 185 Cambridge Street, Boston, Massachusetts 02114, USA
Correspondence to: Correspondence and requests for materials should be addressed to J.W.S. (Email: szostak@molbio.mgh.harvard.edu).
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