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  • Intracellular directed evolution of proteins from combinatorial libraries based on conditional phage replication.

Intracellular directed evolution of proteins from combinatorial libraries based on conditional phage replication.

Nature protocols (2017-08-11)
Andreas K Brödel, Alfonso Jaramillo, Mark Isalan
摘要

Directed evolution is a powerful tool to improve the characteristics of biomolecules. Here we present a protocol for the intracellular evolution of proteins with distinct differences and advantages in comparison with established techniques. These include the ability to select for a particular function from a library of protein variants inside cells, minimizing undesired coevolution and propagation of nonfunctional library members, as well as allowing positive and negative selection logics using basally active promoters. A typical evolution experiment comprises the following stages: (i) preparation of a combinatorial M13 phagemid (PM) library expressing variants of the gene of interest (GOI) and preparation of the Escherichia coli host cells; (ii) multiple rounds of an intracellular selection process toward a desired activity; and (iii) the characterization of the evolved target proteins. The system has been developed for the selection of new orthogonal transcription factors (TFs) but is capable of evolving any gene-or gene circuit function-that can be linked to conditional M13 phage replication. Here we demonstrate our approach using as an example the directed evolution of the bacteriophage λ cI TF against two synthetic bidirectional promoters. The evolved TF variants enable simultaneous activation and repression against their engineered promoters and do not cross-react with the wild-type promoter, thus ensuring orthogonality. This protocol requires no special equipment, allowing synthetic biologists and general users to evolve improved biomolecules within ∼7 weeks.

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硫酸镁, anhydrous, ReagentPlus®, ≥99.5%
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氨苄西林 钠盐, powder or crystals, BioReagent, suitable for cell culture
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KOD热启动DNA聚合酶, High fidelity DNA polymerase designed for accurate PCR amplification of long strand and GC- rich DNA templates for cloning and cDNA amplification applications.
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水, for molecular biology, sterile filtered
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卡那霉素 硫酸酯 来源于卡那霉素链霉菌, Animal Component-free
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羧苄青霉素 二钠盐, 89.0-100.5% anhydrous basis