Development of New Thioester Equivalents for Protein Chemical Synthesis

Zheng, Ji‐Min; Tang, Shan; Huang, Yichao; Liu, Lei

doi:10.1021/ar400012w

Cited by 155 publications

(85 citation statements)

References 68 publications

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“…One important step toward the design of mild transamidation and amide metathesis reactions that operate with peptide substrates in water was inspired by recent advances in the design of N,S-acyl shift systems ( Figure 3) [13][14][15][16][17][18][19][20]21 ]. Indeed, some N-(2-sulfanylethyl) amides are able to rearrange into transient thioesters by spontaneous acyl migration from nitrogen to sulfur.…”

Section: Introductionmentioning

confidence: 99%

From protein total synthesis to peptide transamidation and metathesis: playing with the reversibility of N,S-acyl or N,Se-acyl migration reactions

Melnyk

Agouridas

2014

Current Opinion in Chemical Biology

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Section: Introductionmentioning

confidence: 99%

From protein total synthesis to peptide transamidation and metathesis: playing with the reversibility of N,S-acyl or N,Se-acyl migration reactions

Melnyk

Agouridas

2014

Current Opinion in Chemical Biology

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“…These methods were problematic for several reasons, including the favorable Curtius rearrangement which acyl azides readily undergo. In an attempt to overcome these limitations, Liu and co-workers have investigated extensively peptide hydrazines and their conversion to acyl azides [134]. They found that the conversion of hydrazide 96 to acyl azide 97 could be completed nearly C. Subsequent addition of thiols, such as MPAA, to the reaction mixture, followed by an increase in pH to 7.0, reliably generated the required thioester 98 in a convenient one-pot procedure.…”

Section: New Methods For Activated Peptide Synthesismentioning

confidence: 99%

New Methods for Chemical Protein Synthesis

Guan

Chaffey

Zeng

2014

Topics in Current Chemistry

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Chemical protein synthesis is a useful tool to generate pure proteins which are otherwise difficult to obtain in sufficient amounts for structure and property analysis. Additionally, because of the precise and flexible nature of chemical synthesis, it allows for controllable variation of protein sequences, which is valuable for understanding the relationships between protein structure and function. Despite the usefulness of chemical protein synthesis, it has not been widely adopted as a tool for protein characterization, mainly because of the lack of general and efficient methods for the preparation and coupling of peptide fragments and for the folding of polypeptide chains. To address these issues, many new methods have recently been developed in the areas of solid-phase peptide synthesis, peptide fragment assembly, and protein folding. Here we review these recent technological advances and highlight the gaps needing to be addressed in future research.

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“…The two peptide fragments may be obtained by solid-phase peptide synthesis using well-established fluorenylmethoxycarbonyl (Fmoc-) or tertbutyloxycarbonyl (Boc-) amine protecting group strategies. Several chemical linkers and derivatization strategies are available for the synthesis of peptide α-thioesters by both chemistries [49,50]. Since most histone marks are found in the N-terminal tails, the C-terminal fragment may be larger and obtained by heterologous expression in Escherichia coli (Figure 8.2).…”

Section: Strategies Of Native Chemical and Expressed Protein Ligationmentioning

confidence: 99%