Probing the molecular basis of factor Xa specificity by mutagenesis of the serpin, antithrombin

The molecular basis of the substrate and inhibitor specificity of factor Xa, the serine proteinase of the prothrombinase complex, was investigated by constructing two mutants of human antithrombin (HAT) in which the reactive site loop of the serpin from the P4–P4′ site was replaced with the correspo...

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Published in:Biochimica et biophysica acta 2001-10, Vol.1528 (2), p.167-176
Main Authors: Rezaie, Alireza R, Yang, Likui
Format: Article
Language:English
Subjects:
Antithrombin
Antithrombins - biosynthesis
Antithrombins - genetics
Antithrombins - metabolism
Enzyme Precursors - metabolism
Factor V - metabolism
Factor Va - pharmacology
Factor Xa
Factor Xa - metabolism
Factor Xa Inhibitors
Genetic Vectors
Heparin - pharmacology
Humans
Kinetics
Mutation
Peptide Fragments - pharmacology
Prothrombin
Prothrombin - biosynthesis
Prothrombin - chemistry
Prothrombin - metabolism
Prothrombinase
Recombinant Proteins - isolation & purification
Sequence Alignment
Serpin
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Summary:The molecular basis of the substrate and inhibitor specificity of factor Xa, the serine proteinase of the prothrombinase complex, was investigated by constructing two mutants of human antithrombin (HAT) in which the reactive site loop of the serpin from the P4–P4′ site was replaced with the corresponding residues of the two factor Xa cleavage sites in prothrombin (HAT/Proth-1 and HAT/Proth-2). These mutants together with prethrombin-2, the smallest zymogen form of thrombin containing only the second factor Xa cleavage site, were expressed in mammalian cells, purified to homogeneity and characterized in kinetic reactions with factor Xa in both the absence and presence of cofactors; factor Va, high affinity heparin and pentasaccharide fragment of heparin. HAT/Proth-1 inactivated factor Xa ∼3–4-fold better than HAT/Proth-2 in either the absence or presence of heparin cofactors. In the absence of a cofactor, factor Xa reacted with the HAT/Proth-2 and prethrombin-2 with similar second-order rate constants (∼2–3×10 2 M −1 s −1). Pentasaccharide catalyzed the inactivation rate of factor Xa by the HAT mutants 300–500-fold. A similar 10 4–10 5-fold enhancement in the reactivity of factor Xa with prethrombin-2 and the HAT mutants was observed in the presence of the cofactors Va and heparin, respectively. Factor Va did not influence the reactivity of factor Xa with either one of the HAT mutants. These results suggest that (1) in the absence of a cofactor, the P4–P4′ residues of HAT and prethrombin-2 primarily determine the specificity reactions with factor Xa, (2) factor Va binding to factor Xa is not associated with allosteric changes in the catalytic pocket of enzyme that would involve interactions with the P4–P4′ binding sites, and (3) similar to allosteric activation of HAT by heparin, a role for factor Va in the prothrombinase complex may involve rearrangement of the residues surrounding the scissile bond of the substrate to facilitate its optimal docking into the catalytic pocket of factor Xa.
ISSN:0304-4165
0006-3002
1872-8006
DOI:10.1016/S0304-4165(01)00189-1