Display Selection of Exotic Macrocyclic Peptides Expressed under a Radically Reprogrammed 23 Amino Acid Genetic Code

Passioura, Toby; Liu, Wenyu; Dunkelmann, Daniel; Higuchi, Takashi; Suga, Hiroaki

doi:10.1021/jacs.8b03367

Cited by 57 publications

(56 citation statements)

References 23 publications

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“…30 We withdrew the natural initiator amino acid Met and its cognate aaRS during the construction of a custom reconstituted in vitro translation system, 31 and supplemented this with initiator tRNA loaded with ClAc-D-Phe, 22 using an artificial ribozyme flexizyme. 32 We then further reprogrammed the genetic code to remove the charged amino acids Glu, Asp, and Arg, and add the following non-canonical amino acids: 22,29,33 three N-methylated: MeGly, MeAla and MePhe; two D-stereochemistry: D-Phe and D-Ala, and the linear hydrophobic side-chain Aoc (Fig. 1A).…”

Section: Construction Of a Highly Non-proteinogenic Cyclic Peptide LImentioning

confidence: 99%

“…A potential route to such molecules is to screen cyclic peptide libraries which include from the beginning non-canonical amino acids known to confer desirable physical properties. 22,29 However, it is not yet known if cyclic peptides from such a library can succeed at a challenging molecular recognition task like specific Ub chain binding. Here, we constructed and screened a highly nonproteinogenic peptide library to discover de novo cyclic peptides capable of modulating specific Lys48-linked ubiquitin chains.…”

Section: Introductionmentioning

confidence: 99%

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In vivo modulation of ubiquitin chains by N-methylated non-proteinogenic cyclic peptides

et al. 2021

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Section: Construction Of a Highly Non-proteinogenic Cyclic Peptide LImentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

In vivo modulation of ubiquitin chains by N-methylated non-proteinogenic cyclic peptides

et al. 2021

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“…Owing to the broad tolerance of flexizyme for tRNAs and amino acids, including NAAs, various NAA-tRNAs can be prepared. The combination of a reconstituted E. coli translation system and NAA-tRNAs prepared by flexizyme is referred to as the flexible in vitro translation (FIT) system, which enables the synthesis of various peptides containing NAAs by means of genetic code reprogramming (Yamagishi et al, 2011;Katoh et al, 2017;Passioura et al, 2018a;Katoh and Suga, 2019).…”

Section: Genetic Code Manipulation Technologies For Incorporation Of mentioning

confidence: 99%

Methodologies for Backbone Macrocyclic Peptide Synthesis Compatible With Screening Technologies

et al. 2020

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Backbone macrocyclic structures are often found in diverse bioactive peptides and contribute to greater conformational rigidity, peptidase resistance, and potential membrane permeability compared to their linear counterparts. Therefore, such peptide scaffolds are an attractive platform for drug-discovery endeavors. Recent advances in synthetic methods for backbone macrocyclic peptides have enabled the discovery of novel peptide drug candidates against diverse targets. Here, we overview recent technical advancements in the synthetic methods including 1) enzymatic synthesis, 2) chemical synthesis, 3) split-intein circular ligation of peptides and proteins (SICLOPPS), and 4) in vitro translation system combined with genetic code reprogramming. We also discuss screening methodologies compatible with those synthetic methodologies, such as one-beads one-compound (OBOC) screening compatible with the synthetic method 2, cell-based assay compatible with 3, limiting-dilution PCR and mRNA display compatible with 4.

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“…A lysine derivative with biotin group ( 88 ) was used as an affinity handle. The ncAAs with varying hydrophobicity and properties ( 89-91 ) (Passioura et al, 2018 ) were used to build libraries with expanded diversity for peptide selection (Kawakami et al, 2013b ). A warhead ncAA, ε-N-trifluoroacetyl-Lysine ( 92 ), in peptide sequence was used to achieve selective inhibition of the de-acylation activity of Human Deacetylase SIRT2 (Morimoto et al, 2012 ).…”

Section: Genetic Encoding Of Ncaasmentioning

confidence: 99%

Cell-Free Approach for Non-canonical Amino Acids Incorporation Into Polypeptides

Cui

Johnston

Alexandrov

2020

Front. Bioeng. Biotechnol.

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Composition Crude extract (>500 proteins) + necessary factors 36 purified proteins+ tRNAs + ribosomes + necessary factors Energy source Versatile energy sources including variants that take advantage of cellular metabolism Creatine phosphate/creatine kinase ATP regeneration system Flexibility Partial control of translational machinery Full control of translational machinery Linear template Unstable, requires special strains, or lysate treatment Stable Peptide synthesis Unstable, requires special strains, or lysate treatment Stable Applications Small scale protein expression Peptide expression for mRNA display Large scale protein biomanufacturing Isotopically labeled peptides (MS standard) Biological process prototyping Translation factor characterization Compatibility with selection systems Ribosome display mRNA display Microbead display (in vitro compartmentation) cDNA display Amber suppression Frequently used Seldom used Initiation reassignment Seldom used Limited amino acid structures Commonly used A wide range of ncAAs (Figure 5) Elongator codon reassignment Less used Commonly used (residue-specific manner) A wide range of ncAAs (Figure 6)

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Display Selection of Exotic Macrocyclic Peptides Expressed under a Radically Reprogrammed 23 Amino Acid Genetic Code

Cited by 57 publications

References 23 publications

In vivo modulation of ubiquitin chains by N-methylated non-proteinogenic cyclic peptides

In vivo modulation of ubiquitin chains by N-methylated non-proteinogenic cyclic peptides

Methodologies for Backbone Macrocyclic Peptide Synthesis Compatible With Screening Technologies

Cell-Free Approach for Non-canonical Amino Acids Incorporation Into Polypeptides

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