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Cell-free protein synthesis from a release factor 1 deficient Escherichia coli activates efficient and multiple site-specific non-standard amino acid incorporation.

ACS Synth Biol.. 2013-12; 
SH Hong, I Ntai,?AD Haimovich, NL Kelleher, Farren J. Isaacs , and Michael C. Jewett. Department of Chemical and Biological Engineering,Northwestern University,Evanston, IL 60208, USA.
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摘要

Site-specific incorporation of non-standard amino acids (NSAAs) into proteins enables the creation of biopolymers, proteins, and enzymes with new chemical properties, new structures, and new functions. To achieve this, amber (TAG codon) suppression has been widely applied. However, the suppression efficiency is limited due to the competition with translation termination by release factor 1 (RF1), which leads to truncated products. Recently, we constructed a genomically recoded Escherichia coli strain lacking RF1 where 13 occurrences of the amber stop codon have been reassigned to the synonymous TAA codon (rEc.E13.prfA). Here, we assessed and characterized cell-free protein synthesis (CFPS) in crude S30 cell lys... More

关键词

cell-free protein synthesis; PURE translation; non-standard amino acid; release factor 1; genomically recoded organisms