Total Synthesis of desB30 Insulin Analogues by Biomimetic Folding of Single‐Chain Precursors

Tofteng, A. Pernille; Jensen, Knud J.; Schäffer, Lauge; Høeg-Jensen, Thomas

doi:10.1002/cbic.200800430

Cited by 55 publications

(60 citation statements)

References 38 publications

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“…This single chain insulin analog that was based entirely on the insulin sequence proved more difficult to prepare and was only obtained with the aid of an N-terminal polyglutamic acid leader sequence (peptide 20) that was removed proteolytically. 29 This demonstrates the biophysical virtue of IGF-1 based analogs. The additional amino acids at the N-terminal end of peptide 20 did not change activation at the insulin and IGF-1 receptors.…”

Section: ■ Results and Discussionmentioning

confidence: 86%

Discovery of High Potency, Single-Chain Insulin Analogs with a Shortened B-Chain and Nonpeptide Linker

et al. 2013

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A series of novel, single chain insulin analogs containing polyethylene glycol based connecting segments were synthesized by native chemical ligation and tested for biological activity. While the full length single chain insulin analogs exhibited low potency, deletion of amino acids B26-B30 unexpectedly generated markedly higher activity. This observation is unprecedented in all previous studies of single chain insulin analogs and is consistent with the presumption that in the native hormone this sequence must translocate to achieve high potency insulin receptor interaction. Optimization of the sequence yielded an insulin analog with potency and selectivity comparable to that of native insulin. These results establish a basis for discovery of novel higher potency, single chain insulin analogs of shortened length.

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Section: ■ Results and Discussionmentioning

confidence: 86%

Discovery of High Potency, Single-Chain Insulin Analogs with a Shortened B-Chain and Nonpeptide Linker

et al. 2013

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“…These proteases robustly and specifically recognize and cleave C-terminal to the basic amino acid lysine, even following with proline or glutamic acid, making them useful enzymes for various applications, including proteomic sample preparation and human insulin production [2,5,6]. Current proteomic grade protease IV products of high purity and activity supplied by vendors such as Wako, and others, are extracted from the native bacteria L. enzymogenes using an inefficient process [2,7].…”

Section: Introductionmentioning

confidence: 99%

Recombinant expression, refolding, purification and characterization of Pseudomonas aeruginosa protease IV in Escherichia coli

Zhao

Man²,

et al. 2016

Protein Expression and Purification

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“…They share the native linear order of proinsulin where the N-terminus of the A-chain is indirectly connected to the C-terminus of the B-chain. Conversion to the two-chain form initially employed enzymatic conversion and was restricted by the requirement for a unique proteolytic site [11][12][13][14][15] . The more recent reports employing chemically labile linkers represent a leap forward by eliminating the need for a proteolytic site, and the enzyme itself.…”

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confidence: 99%

Synthesis of disulfide-rich heterodimeric peptides through an auxiliary N, N-crosslink

et al. 2018

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Insulins, relaxins, and other insulin-like peptides present a longstanding synthetic challenge due to their unique cysteine-rich heterodimeric structure. While their three disulfide signature is conserved within the insulin superfamily, sequences of the constituent chains exhibit considerable diversity. As a result, methods which rely on sequence-specific strategies fail to provide universal access to these important molecules. Biomimetic methods utilizing native and chemical linkers to tether the A-chain N-terminus to the B-chain Cterminus, entail complicated installation, and require a unique proteolytic site, or a two-step chemical release. Here we present a strategy employing a linkage of the A-and B-chains Ntermini offering unrestricted access to these targets. The approach utilizes a symmetrical linker which is released in a single chemical step. The simplicity, efficiency, and scope of the method are demonstrated in the synthesis of insulin, relaxin, a 4-disulfide insulin analog, two penicillamine-substituted insulins, and a prandial insulin lispro.

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Total Synthesis of desB30 Insulin Analogues by Biomimetic Folding of Single‐Chain Precursors

Cited by 55 publications

References 38 publications

Discovery of High Potency, Single-Chain Insulin Analogs with a Shortened B-Chain and Nonpeptide Linker

Discovery of High Potency, Single-Chain Insulin Analogs with a Shortened B-Chain and Nonpeptide Linker

Recombinant expression, refolding, purification and characterization of Pseudomonas aeruginosa protease IV in Escherichia coli

Synthesis of disulfide-rich heterodimeric peptides through an auxiliary N, N-crosslink

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