Replacement of Phe274 With Conserved Residue Tyr274 for Reactive Center Loop Expulsion in Antithrombin

  • Duhan, Urmila

  • 1Center for Molecular Biology of Oral Diseases, College of Dentistry, Chicago, IL, USA

Corresponding Author:

Urmila Duhan, Center for Molecular Biology of Oral Diseases, Rm 530E, College of Dentistry (M/C 860), S. Paulina Street, Chicago, IL 60612, USA.

Email: [email protected]

Clinical & Applied Thrombosis/Hemostasis 17(3):p 273-278, June 2011. | DOI: 10.1177/1076029609360529

Abstract

Background:

The reactive center loop (RCL) of native antithrombin is partially inserted in the main serpin body. It must be fully exposed for optimal inhibitory function.

Objective:

To test the hypothesis that P14-s2B interaction affects loop insertion in antithrombin. By mutating Phe274 to Tyr274, the objective was to introduce P14-s2B interaction in antithrombin.

Methods:

Site-directed mutagenesis and affinity chromatography were used to obtain purified recombinant protein. Antithrombin's ability to form sodium dodecyl sulfate (SDS)-stable complex with thrombin, stoichiometry of thrombin inhibition, second-order rate constant for thrombin and factor Xa (fXa) inhibition (M-1 s-1), and heparin dissociation constant (KD; tryptophan fluorescence emission spectra) were determined.

Results and Conclusion:

A marginal, but inconclusive, difference between the wild type and the mutant was observed. The result highlights the variable effect of P14-s2B interaction in different serpins. Alternate hypothesis for achieving loop expulsion is proposed.

Copyright ©2011Sage Publications
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