Characterization of bothrojaracin interaction with human prothrombin
Abstract
Bothrojaracin (BJC) is a 27-kD snake venom protein from Bothrops jararaca that has been characterized as a potent thrombin inhibitor. BJC binds to exosites I and II, with a dissociation constant of 0.7 nM, and influences but does not block the proteinase catalytic site. BJC also binds prothrombin through an interaction that has not been characterized. In the present work we characterize the interaction of BJC with prothrombin quantitatively for the first time, and identify the BJC binding site on human prothrombin. Gel filtration chromatography demonstrated calcium-independent, 1:1 complex formation between fluorescein-labeled BJC ([5F]BJC) and prothrombin, whereas no interactions were observed with activation fragments 1 or 2 of prothrombin. Isothermal titration calorimetry showed that binding of BJC to prothrombin is endothermic, with a dissociation constant of 76 ± 32 nM. The exosite I-specific ligand, hirudin (Hir (SO3), displaced competitively [5F]BJC from prothrombin. Titration of the fluorescent hirudin derivative, [5F]Hir(SO3), with human prothrombin showed a dissociation constant of 7.0 ± 0.2 μM, indicating a ∼100-fold lower binding affinity than that exhibited by BJC. Both ligands, however, displayed a similar, ∼100-fold increase in affinity for exosite I when prothrombin was activated to thrombin. BJC efficiently displaced [5F]Hir(SO3) from complexes formed with thrombin or prothrombin with dissociation constants of 0.7 ± 0.9 nM and 11 ± 80 nM, respectively, indicating that BJC and Hir(SO3) compete for the same exosite on these molecules. The results indicate that BJC is a potent and specific probe of the partially exposed anion-binding exosite (proexosite I) of human prothrombin.
The blood-clotting serine proteinase, thrombin, is formed by cleavage of two peptide bonds in prothrombin by blood coagulation factor Xa. Thrombin generation is accompanied by separation of the prothrombin activation fragment 1 and 2 domains and the protease domain (thrombin). The prothrombin fragment 1 domain functions in prothrombin activation by binding calcium and negatively charged phospholipid surfaces (Gitel et al. 1973; Dombrose et al. 1979). Binding of prothrombin to the cofactor protein, factor Va, which regulates the activation of prothrombin by factor Xa, is thought to involve fragment 2 and/or an exosite in the proteinase domain of prothrombin (Kotkow et al. 1995; Krishnaswamy and Walker 1997; Anderson et al. 2000b). During the conversion of prothrombin into thrombin, the catalytic site is activated and additional allosteric regulatory sites become expressed on the enzyme (Liu et al. 1991b; Wu et al. 1994). Anion-binding exosite I is a positively charged site on thrombin that interacts with fibrinogen (Naski et al. 1990), the platelet thrombin receptor (Liu et al. 1991a), thrombomodulin (Ye et al. 1992), heparin cofactor II (Hortin et al. 1989), factor V and Va (Dharmawardana et al. 1999), and with C-terminal hirudin peptides (Krstenansky and Mao 1987). Through these interactions, exosite I plays key roles in the specificity of thrombin towards macromolecular substrates, cofactors, and some inhibitors (Stubbs and Bode 1993; Guillin et al. 1995). Recently, exosite I has been shown to be partially exposed on prothrombin in a precursor state (proexosite I), and is fully expressed on thrombin, with a ∼100-fold increase in affinity for hirudin peptides (Anderson et al. 2000a). Another positively charged site on thrombin is anion-binding exosite II, which binds heparin (Sheehan and Sadler 1994) and fragment 2 (Walker and Esmon 1979). The crystal structure of the thrombin–fragment 2, domain–domain complex indicates that exosite II is not accessible on prothrombin (Arni et al. 1993).
Bothrojaracin (BJC) is a potent and highly specific thrombin inhibitor isolated from the venom of the jararaca snake common to Brazil (Bothrops jararaca) (Zingali et al. 1993). BJC is a 27-kD disulfide-linked heterodimer that belongs to the C-type (Ca-dependent) lectin-like related protein family (Arocas et al. 1997). The mechanism of thrombin inhibition is unusual in that BJC interacts with both exosites I and II on thrombin (Arocas et al. 1996), forming a 1:1 noncovalent complex and inhibiting thrombin activity toward fibrinogen, platelets, protein C, and factor V (Zingali et al. 1993; Arocas et al. 1998), while the activity towards tripeptide chromogenic substrates is modulated but not impaired (Monteiro et al. 1999). In addition, BJC has been found to form a noncovalent complex with prothrombin (Arocas et al. 1996), and this was associated with inhibition by BJC of prothrombin activation by Oxyuranus scutellatus venom (Monteiro and Zingali 2000). However, the mechanism by which BJC binds to prothrombin is not known, and the binding site on prothrombin has not been identified.
In the present work we quantitatively characterize the binding of BJC to prothrombin for the first time, and identify the binding site on prothrombin as proexosite I in the catalytic domain of prothrombin. Competitive binding studies employing fluorescence probes showed that specific binding of sulfated hirudin (Hir[SO3]) to proexosite I displaced BJC from the complex formed with prothrombin. BJC similarly disrupted the prothrombin complex with Hir(SO3), indicating that BJC and Hir(SO3) bind competitively to proexosite I on human prothrombin. The results for BJC represent the highest affinity interaction with proexosite I described thus far, and may therefore aid the development of novel anticoagulants based on exosite inhibitors.
Acknowledgments
We thank Dr. C. Nogueira (Serviço de Hemoterapia/HUCFF/UFRJ) for providing the human plasma samples used for prothrombin and α-thrombin purifications; Instituto Butantan (São Paulo, Brazil) for providing Bothrops jararaca venom. We thank Dr. J.L. Silva and D. Foguel for the use of the fluorescence equipment, and Dr. L. de Meis for calorimetric facilities; Drs. C. Barja-Fidalgo and Patricia J. Anderson for help with the analysis and careful revision of the manuscript; Ana Lúcia O. Carvalho and Denis L.S. Dutra for their technical assistance; the Laboratory of Microsequencing of Proteins and Peptides (LMPP) from the Medical Biochemistry Department (UFRJ); and Prof. L.M.T. Lima for helpful discussions. This work was supported by Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq), Financiadora de Estudos e Projetos do Brasil (FINEP), Fundação de Amparo à Pesquisa do Estado do Rio de Janeiro (FAPERJ), European Economic Community (EEC) contract Cl1*-CT94-0073 BR, and in part supported by National Institutes of Health Grant HL-38779 to P.E.B.
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Abbreviations
BJC, bothrojaracin
[5F]BJC, bothrojaracin labeled with fluorescein 5-isothiocyanate
Hir (SO3), Gly-Asp-Phe-Glu-Glu-Ile-Pro-Glu-Glu-Tyr(SO3)-Leu-Gln
[5F]Hir (SO3)
Hir (SO3) labeled at the amino terminus with 5-carboxy(fluorescein)
TBS, Tris-buffered saline (20 mM Tris-HCl, 150 mM NaCl, pH 7.5)
Notes
Article and publication are at http://www.proteinscience.org/cgi/doi/10.1101/