Directed co-evolution of interacting protein–peptide pairs by compartmentalized two-hybrid replication (C2HR)

生物 定向进化 过程性 聚合酶 DNA聚合酶 DNA钳 DNA复制 融合蛋白 遗传学 分子生物学 DNA 聚合酶链反应 基因 重组DNA 逆转录酶 突变体
作者
Jia Wei Siau,Samuel G. Nonis,Sharon Chee,Li Quan Koh,Fernando Ferrer,Christopher J. Brown,Farid J. Ghadessy
出处
期刊:Nucleic Acids Research [Oxford University Press]
卷期号:48 (22): e128-e128 被引量:4
标识
DOI:10.1093/nar/gkaa933
摘要

Abstract Directed evolution methodologies benefit from read-outs quantitatively linking genotype to phenotype. We therefore devised a method that couples protein–peptide interactions to the dynamic read-out provided by an engineered DNA polymerase. Fusion of a processivity clamp protein to a thermostable nucleic acid polymerase enables polymerase activity and DNA amplification in otherwise prohibitive high-salt buffers. Here, we recapitulate this phenotype by indirectly coupling the Sso7d processivity clamp to Taq DNA polymerase via respective fusion to a high affinity and thermostable interacting protein–peptide pair. Escherichia coli cells co-expressing protein–peptide pairs can directly be used in polymerase chain reactions to determine relative interaction strengths by the measurement of amplicon yields. Conditional polymerase activity is further used to link genotype to phenotype of interacting protein–peptide pairs co-expressed in E. coli using the compartmentalized self-replication directed evolution platform. We validate this approach, termed compartmentalized two-hybrid replication, by selecting for high-affinity peptides that bind two model protein partners: SpyCatcher and the large fragment of NanoLuc luciferase. We further demonstrate directed co-evolution by randomizing both protein and peptide components of the SpyCatcher–SpyTag pair and co-selecting for functionally interacting variants.

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