Serpin polymerization is prevented by a hydrogen bond network that is centered on His-334 and stabilized by glycerol

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Abstract

Polymerization of serpins commonly results from mutations in the shutter region underlying the bifurcation of strands 3 and 5 of the A-sheet, with entry beyond this point being barred by a H-bond network centered on His-334. Exposure of this histidine in antithrombin, which has a partially opened sheet, allows polymerization and peptide insertion to occur at pH 6 or less when His-334 will be predictably protonated with disruption of the H-bond network. Similarly, thermal stability of antithrombin is pH-dependent with a single unfolding transition at pH 6, but there is no such transition when His-334 is buried by a fully closed A-sheet in heparin-complexed antithrombin or in α1-antitrypsin. Replacement of His-334 in α1-antitrypsin by a serine or alanine at pH 7.4 results in the same polymerization and loop-peptide acceptance observed with antithrombin at low pH. The critical role of His-334 and the re-formation of its H-bond network by the conserved P8 threonine, on the full insertion of strand 4, are relevant for the design of therapeutic blocking agents. This is highlighted here by the crystallographic demonstration that glycerol, which at high concentrations blocks polymerization, can replace the P8 threonine and re-form the disrupted H-bond network with His-334.

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Zhou, A., Stein, P. E., Huntington, J. A., & Carrell, R. W. (2003). Serpin polymerization is prevented by a hydrogen bond network that is centered on His-334 and stabilized by glycerol. Journal of Biological Chemistry, 278(17), 15116–15122. https://doi.org/10.1074/jbc.M211663200

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