2015
DOI: 10.1002/bit.25587
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Genetically expanded cell‐free protein synthesis using endogenous pyrrolysyl orthogonal translation system

Abstract: Cell-free protein synthesis offers a facile and rapid method for synthesizing, monitoring, analyzing, and purifying proteins from a DNA template. At the same time, genetic code expansion methods are gaining attention due to their ability to site-specifically incorporate unnatural amino acids (UAAs) into proteins via ribosomal translation. These systems are based on the exogenous addition of an orthogonal translation system (OTS), comprising an orthogonal tRNA, and orthogonal aminoacyl tRNA synthetase (aaRS), t… Show more

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Cited by 49 publications
(59 citation statements)
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References 50 publications
(66 reference statements)
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“…Chemla et al. reported a similar yield (∼200 μg mL −1 ) in their synthesis of a GFP mutant with propargyllysine at a single position by reprogramming the amber codon in a CFPS system deficient in RF1 . And a similar yield was reported by Hong et al.…”
Section: Figuresupporting
confidence: 59%
“…Chemla et al. reported a similar yield (∼200 μg mL −1 ) in their synthesis of a GFP mutant with propargyllysine at a single position by reprogramming the amber codon in a CFPS system deficient in RF1 . And a similar yield was reported by Hong et al.…”
Section: Figuresupporting
confidence: 59%
“…G-GECO is dim in the absence of Ca 2+ and bright when bound to Ca 2+ with a Ca 2+ -dependent fluorescence increase of ~23–26 fold (Fig. 4A) 7 . We cloned G-GECO under the P70a promoter and verified that it can sense Ca 2+ in a plate reader assay (Fig.…”
mentioning
confidence: 97%
“…Modern TXTL platforms are used for medicine and biomolecular manufacturing, such as the production of vaccine and therapeutics 5, 6 . By performing non-natural chemistries 3, 7, 8 , the TXTL technology has been improved to expand the molecular repertoire of biological systems. Because the time for design-build-test cycle is dramatically reduced, TXTL has become a powerful platform to rapidly prototype genetic programs in vitro , from testing single regulatory elements to recapitulating metabolic pathways 9 .…”
mentioning
confidence: 99%
“…A slight modification of the same system enabled site-specific incorporation of different pyrrolysine analogs into a model protein via stop codon suppression 33 . The employed cell-free system [31][32][33] is based on an all E. coli transcription-translation system.…”
Section: Introductionmentioning
confidence: 99%
“…A slight modification of the same system enabled site-specific incorporation of different pyrrolysine analogs into a model protein via stop codon suppression 33 . The employed cell-free system [31][32][33] is based on an all E. coli transcription-translation system. Nevertheless, it enables protein expression as efficiently as in current bacteriophage systems (0.5 -1 mg/ml of recombinant protein) 32 , while retaining much of the original transcription-translation modularity.…”
Section: Introductionmentioning
confidence: 99%