Structural Basis for the Substrate Specificity of Tobacco Etch Virus Protease

Jason Phan; Alexander Zdanov; Artem G. Evdokimov; Joseph E. Tropea; H K Peters; Rachel B. Kapust; Mi Li; Alexander Wlodawer; David S. Waugh

doi:10.1074/jbc.m207224200

Structural Basis for the Substrate Specificity of Tobacco Etch Virus Protease

Jason Phan(National Institutes of Health), Alexander Zdanov(National Institutes of Health), Artem G. Evdokimov(National Institutes of Health), Joseph E. Tropea(National Institutes of Health), H K Peters(National Institutes of Health), Rachel B. Kapust(National Institutes of Health), Mi Li(National Institutes of Health), Alexander Wlodawer(National Institutes of Health), David S. Waugh(National Institutes of Health)

Journal of Biological Chemistry

December 1, 2002

10.1074/jbc.m207224200

Cited by 259Open Access

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Abstract

Because of its stringent sequence specificity, the 3C-type protease from tobacco etch virus (TEV) is frequently used to remove affinity tags from recombinant proteins. It is unclear, however, exactly how TEV protease recognizes its substrates with such high selectivity. The crystal structures of two TEV protease mutants, inactive C151A and autolysis-resistant S219D, have now been solved at 2.2- and 1.8-A resolution as complexes with a substrate and product peptide, respectively. The enzyme does not appear to have been perturbed by the mutations in either structure, and the modes of binding of the product and substrate are virtually identical. Analysis of the protein-ligand interactions helps to delineate the structural determinants of substrate specificity and provides guidance for reengineering the enzyme to further improve its utility for biotechnological applications.

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