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Literature DB >> 28530710

Engineering protein stability with atomic precision in a monomeric miniprotein.

Emily G Baker¹, Christopher Williams^1,2, Kieran L Hudson¹, Gail J Bartlett¹, Jack W Heal¹, Kathryn L Porter Goff¹, Richard B Sessions^2,3, Matthew P Crump^1,2, Derek N Woolfson^1,2,3.

Abstract

Miniproteins simplify the protein-folding problem, allowing the dissection of forces that stabilize protein structures. Here we describe PPα-Tyr, a designed peptide comprising an α-helix buttressed by a polyproline II helix. PPα-Tyr is water soluble and monomeric, and it unfolds cooperatively with a midpoint unfolding temperature (TM) of 39 °C. NMR structures of PPα-Tyr reveal proline residues docked between tyrosine side chains, as designed. The stability of PPα is sensitive to modifications in the aromatic residues: replacing tyrosine with phenylalanine, i.e., changing three solvent-exposed hydroxyl groups to protons, reduces the TM to 20 °C. We attribute this result to the loss of CH-π interactions between the aromatic and proline rings, which we probe by substituting the aromatic residues with nonproteinogenic side chains. In analyses of natural protein structures, we find a preference for proline-tyrosine interactions over other proline-containing pairs, and observe abundant CH-π interactions in biologically important complexes between proline-rich ligands and SH3 and similar domains.

Entities: Chemical

Mesh：

Substances：
Peptides

Year: 2017 PMID： 28530710 PMCID： PMC5860740 DOI： 10.1038/nchembio.2380

Source DB: PubMed Journal: Nat Chem Biol ISSN： 1552-4450 Impact factor: 15.040

55 in total

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10 in total