Peptide <i>o</i>‐Aminoanilides as Crypto‐Thioesters for Protein Chemical Synthesis

Wang, Jiaxing; Fang, Ge‐Min; He, Yao; Qu, Da-Liang; Yu, Min; Hong, Zhangyong; Liu, Lei

doi:10.1002/anie.201408078

Cited by 145 publications

(112 citation statements)

References 47 publications

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“…However, the conversion was incomplete, probably due to the sterically hindered C‐terminal Thr(tBu)‐370. Thus, we decided to cleave the peptide from the resin in the Dbz form 3a , which is more stable than the Nbz form 3 but may be orthogonally converted into a benzotriazole moiety with NaNO 2 and then displaced by the thiol additive in the ligation buffer to afford the peptide thioester in situ . The TFA‐cleaved product 3a showed satisfactory homogeneity (~60%) (Scheme ).…”

Section: Resultsmentioning

confidence: 99%

“…Unfortunately, in our case, the use of DMF did not solve the problem, and no Nbz peptide was formed (probably, because of the presence of the β‐branched threonine). Thus, we activated the Dbz peptide 3a by converting it into an N‐acyl‐benzotriazole peptide by using NaNO 2 at pH~3, as previously shown by Liu and coworkers . For the Acm cleavage from the C‐terminal free acid of 8 , we used the Pd‐catalyzed reaction reported by Brik and coworkers .…”

Section: Discussionmentioning

confidence: 99%

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An explorative study towards the chemical synthesis of the immunoglobulin G1 Fc CH3 domain

Grassi

Roschger

Stanojlović

et al. 2018

Journal of Peptide Science

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Monoclonal antibodies, fusion proteins including the immunoglobulin fragment c (Ig Fc) CH2‐CH3 domains, and engineered antibodies are prominent representatives of an important class of drugs and drug candidates, which are referred to as biotherapeutics or biopharmaceuticals. These recombinant proteins are highly heterogeneous due to their glycosylation pattern. In addition, enzyme‐independent reactions, like deamidation, dehydration, and oxidation of sensitive side chains, may contribute to their heterogeneity in a minor amount. To investigate the biological impact of a spontaneous chemical modification, especially if found to be recurrent in a biotherapeutic, it would be necessary to reproduce it in a homogeneous manner. Herein, we undertook an explorative study towards the chemical synthesis of the IgG1 Fc CH3 domain, which has been shown to undergo spontaneous changes like succinimide formation and methionine oxidation. We used Fmoc‐solid‐phase peptide synthesis (SPPS) and native chemical ligation (NCL) to test the accessibility of large fragments of the IgG1 Fc CH3 domain. In general, the incorporation of pseudoproline dipeptides improved the quality of the crude peptide precursors; however, sequences larger than 44 residues could not be achieved by standard stepwise elongation with Fmoc‐SPPS. In contrast, the application of NCL with cysteine residues, which were either native or introduced ad hoc, allowed the assembly of the C‐terminal IgG1 Fc CH3 sequence 371 to 450. The syntheses reported here show advantages and limitations of the chemical approaches chosen for the preparation of the synthetic IgG1 Fc CH3 domain and will guide future plans towards the synthesis of both the native and selectively modified full‐length domain.

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Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

An explorative study towards the chemical synthesis of the immunoglobulin G1 Fc CH3 domain

Grassi

Roschger

Stanojlović

et al. 2018

Journal of Peptide Science

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“…The o ‐aminoanilides were activated to thioesters by using NaNO 2 on the fully deprotected peptides. Subsequent NCL and desulfurization afforded the unmodified H2B .…”

Section: Total Chemical Synthesis Of Modified Histonesmentioning

confidence: 99%

Chemical and semisynthesis of modified histones

Maity

Jbara

Brik

2016

Journal of Peptide Science

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Post-translational modifications (PTMs) of histones play critical roles in the epigenetic regulation of eukaryotic genome by directly altering the biophysical properties of chromatin or by recruiting effector proteins. The large number of PTMs and the inherent complexity in their population and signaling processes make it highly challenging to understand epigenetics-related processes. To address these challenges, accesses to homogeneously modified histones are obligatory. Over the last decade, synthetic protein chemists have been devising novel synthetic tools and applying state-of-the-art chemoselective ligation strategies to prepare precious materials useful in answering fundamental questions in this area. In this short review, we cover some of the recent breakthroughs in these directions in particular the synthesis and semi-synthesis of modified histones and their use to unravel the mysteries of epigenetics. Copyright © 2016 European Peptide Society and John Wiley & Sons, Ltd.

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“…On the other hand, a total chemical synthesis approach, whereby the entire modified protein is synthesized via the assembly of synthetic peptides generated by solid phase peptide synthesis (SPPS), makes it possible to incorporate unlimited variations in the protein sequence, including the installation of PTMs at any desired position(s). [15] …”

mentioning

confidence: 99%

“…Notably, despite the presence of methoxylamine, in the second ligation only a minor amount of the side product generated from the attack of methoxylamine on fragment 3 was observed. [15a, 15b, 21] This is probably due to the rapid ligation reaction between fragments 3 and 4 . Subsequently, one-pot desulfurization [22] was carried out in presence of the initiator 2,2′-Azobis[2-(2-imidazolin-2-yl)propane]dihydrochloride (VA-044), TCEP and t -BuSH for 3h to produce the full length histone H2AY57p in ~25% isolated yield (Figure 1).…”

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confidence: 99%

Chemical Synthesis of Phosphorylated Histone H2A at Tyr57 Reveals Insight into the Inhibition Mode of the SAGA Deubiquitinating Module

et al. 2016

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Monoubiquitination of histone H2B plays a central role in transcription activation and is required for downstream histone methylation events. Deubiquitination of H2B by the Spt-Ada-Gcn5 acetyltransferase (SAGA) coactivator complex is regulated by a recently discovered histone mark, phosphorylated H2AY57 (H2AY57p), which inhibits deubiquitination of H2B by the SAGA complex as well as restricting demethylation of H3 and increasing its acetylation. Evidence for the effect of H2AY57p however, was indirect and was investigated in vivo by monitoring the effects of chemical inhibition of Tyr kinase CK2 or by mutating the phosphorylation site. We applied total chemical synthesis of proteins to prepare H2AY57p efficiently and study the molecular details of this regulation. This analogue, together with the semisynthetically prepared ubiquitinated H2B enabled us to provide direct evidence on the cross talk between those two marks and the inhibition of SAGA activity by H2AY57p.

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Peptide o‐Aminoanilides as Crypto‐Thioesters for Protein Chemical Synthesis

Cited by 145 publications

References 47 publications

An explorative study towards the chemical synthesis of the immunoglobulin G1 Fc CH3 domain

An explorative study towards the chemical synthesis of the immunoglobulin G1 Fc CH3 domain

Chemical and semisynthesis of modified histones

Chemical Synthesis of Phosphorylated Histone H2A at Tyr57 Reveals Insight into the Inhibition Mode of the SAGA Deubiquitinating Module

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