The importance of anchorage in determining a strained protein loop conformation

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Abstract

We examine the role of the conformational restriction imposed by constrained ends of a protein loop on the determination of a strained loop conformation. The Lys 116‐Pro 117 peptide bond of staphylococcal nuclease A exists in equilibrium between the cis and trans isomers. The folded protein favors the strained cis isomer with an occupancy of 90%. This peptide bond is contained in a solvent‐exposed, flexible loop of residues 112‐117 whose ends are anchored by Val 111 and Asn 118. Asn 118 is constrained by 2 side‐chain hydrogen bonds. We investigate the importance of this constraint by replacing Asn 118 with aspartate, alanine, and glycine. We found that removing 1 or more of the hydrogen bonds observed in Asn 118 stabilizes the trans configuration over the cis configuration. By protonating the Asp 118 side chain of N118D through decreased pH, the hydrogen bonding character of Asp 118 approached that of Asn 118 in nuclease A, and the cis configuration was stabilized relative to the trans configuration. These data suggest that the rigid anchoring of the loop end is important in establishing the strained cis conformation. The segment of residues 112‐117 in nuclease A provides a promising model system for study of the basic principles that determine polypeptide conformations. Such studies could be useful in the rational design or redesign of protein molecules. Copyright © 1994 The Protein Society

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Hodel, A., Kautz, R. A., Adelman, D. M., & Fox, R. O. (1994). The importance of anchorage in determining a strained protein loop conformation. Protein Science, 3(4), 549–556. https://doi.org/10.1002/pro.5560030403

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