The anticoagulant thrombin mutant W215A/E217A has a collapsed primary specificity pocket

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Abstract

The thrombin mutant W215A/E217A features a drastically impaired catalytic activity toward chromogenic and natural substrates but efficiently activates the anticoagulant protein C in the presence of thrombomodulin. As the remarkable anticoagulant properties of this mutant continue to be unraveled in preclinical studies, we solved the x-ray crystal structures of its free form and its complex with the active site inhibitor H-D-Phe-Pro-Arg-CH2Cl (PPACK). The PPACK-bound structure of W215A/E217A is identical to the structure of the PPACK-bound slow form of thrombin. On the other hand, the structure of the free form reveals a collapse of the 215-217 strand that crushes the primary specificity pocket. The collapse results from abrogation of the stacking interaction between Phe-227 and Trp-215 and the polar interactions of Glu-217 with Thr-172 and Lys-224. Other notable changes are a rotation of the carboxylate group of Asp-189, breakage of the H-bond between the catalytic residues Ser-195 and His-57, breakage of the ion pair between Asp-222 and Arg-187, and significant disorder in the 186- and 220-loops that define the Na+ site. These findings explain the impaired catalytic activity of W215A/E217A and demonstrate that the analysis of the molecular basis of substrate recognition by thrombin and other proteases requires crystallization of both the free and bound forms of the enzyme.

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Pineda, A. O., Chen, Z. W., Caccia, S., Cantwell, A. M., Savvides, S. N., Waksman, G., … Di Cera, E. (2004). The anticoagulant thrombin mutant W215A/E217A has a collapsed primary specificity pocket. Journal of Biological Chemistry, 279(38), 39824–39828. https://doi.org/10.1074/jbc.M407272200

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