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Literature DB >> 21962254

Iterative in situ click chemistry assembles a branched capture agent and allosteric inhibitor for Akt1.

Steven W Millward¹, Ryan K Henning, Gabriel A Kwong, Suresh Pitram, Heather D Agnew, Kaycie M Deyle, Arundhati Nag, Jason Hein, Su Seong Lee, Jaehong Lim, Jessica A Pfeilsticker, K Barry Sharpless, James R Heath.

Abstract

We describe the use of iterative in situ click chemistry to design an Akt-specific branched peptide triligand that is a drop-in replacement for monoclonal antibodies in multiple biochemical assays. Each peptide module in the branched structure makes unique contributions to affinity and/or specificity resulting in a 200 nM affinity ligand that efficiently immunoprecipitates Akt from cancer cell lysates and labels Akt in fixed cells. Our use of a small molecule to preinhibit Akt prior to screening resulted in low micromolar inhibitory potency and an allosteric mode of inhibition, which is evidenced through a series of competitive enzyme kinetic assays. To demonstrate the efficiency and selectivity of the protein-templated in situ click reaction, we developed a novel QPCR-based methodology that enabled a quantitative assessment of its yield. These results point to the potential for iterative in situ click chemistry to generate potent, synthetically accessible antibody replacements with novel inhibitory properties.

Entities: Chemical Disease Gene Mutation Species

Mesh：

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Year: 2011 PMID： 21962254 PMCID： PMC3651860 DOI： 10.1021/ja2064389

Source DB: PubMed Journal: J Am Chem Soc ISSN： 0002-7863 Impact factor: 15.419

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