4.6 Review

To get what we aim for-progress in diversity generation methods

Journal

FEBS JOURNAL
Volume 280, Issue 13, Pages 2961-2978

Publisher

WILEY
DOI: 10.1111/febs.12325

Keywords

directed evolution; diversity generation; epPCR; focused mutagenesis; gene shuffling; high-throughput screening; protein engineering; random mutagenesis; recombination; saturation mutagenesis

Funding

  1. European Union Seventh Framework Programme (FP7-KBBE) [212281]

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Protein re-engineering by directed evolution has become a standard approach for tailoring enzymes in many fields of science and industry. Advances in screening formats and screening systems are fueling progress and enabling novel directed evolution strategies, despite the fact that the quality of mutant libraries can still be improved significantly. Diversity generation strategies in directed enzyme evolution comprise three options: (a) focused mutagenesis (selected residues are randomized); (b) random mutagenesis (mutations are randomly introduced over the whole gene); and (c) gene recombination (stretches of genes are mixed to chimeras in a random or rational manner). Either format has both advantages and limitations depending on the targeted enzyme and property. The quality of diverse mutant libraries plays a key role in finding improved mutants. In this review, we summarize methodological advancements and novel concepts (since 2009) in diversity generation for all three formats. Advancements are discussed with respect to the state of the art in diversity generation and high-throughput screening capabilities, as well as robustness and simplicity in use. Furthermore, limitations and remaining challenges are emphasized to get what we aim for' through optimal diversity' generation.

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