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Mutually Orthogonal DNA Replication Systems In Vivo.

ACS Synth Biol. 2018; 
ArzumanyanGarri A,GabrielKristin N,RavikumarArjun,JavanpourAlex A,LiuCha
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Gene Synthesis To clone the expression vector for wild type TP-DNAP2 (pGA55), TP-DNAP2 was codon optimized for expression in S. cerevisiae with GenScript’s OptimumGene™ tool, and the recoded ORF was synthesized as three gene fragments, which were assembled downstream of the REV1 promoter in a CEN6/ARS4 vector containing selection markers HIS3 and KanR. Get A Quote

摘要

The yeast cytoplasmically localized pGKL1/TP-DNAP1 plasmid/DNA polymerase pair forms an orthogonal DNA replication system whose mutation rate can be drastically increased without influencing genomic replication, thereby supporting in vivo continuous evolution. Here, we report that the pGKL2/TP-DNAP2 plasmid/DNA polymerase pair forms a second orthogonal replication system. We show that custom genes can be encoded and expressed from pGKL2, that error-prone TP-DNAP2s can be engineered, and that pGKL2 replication by TP-DNAP2 is both orthogonal to genomic replication in Saccharomyces cerevisiae and mutually orthogonal with pGKL1 replication by TP-DNAP1. This demonstration of two mutually orthogonal DNA repli... More

关键词

DNA replication,in vivo mutagenesis,linear plasmids,orthogonal replication,polymerase engineering,protein-primed replica