Fig. 6.
Kinetic titration of fused and unfused hirudin as an inhibitor of thrombin-mediated amidolysis. The initial velocity of the reaction of thrombin with chromogenic substrate S2238 was determined in the presence of increasing concentrations of either unfused (HV1, top graph) or fused hirudin (HLA, bottom graph). Results shown are from one paired experiment that is representative of a total of three.

Kinetic titration of fused and unfused hirudin as an inhibitor of thrombin-mediated amidolysis. The initial velocity of the reaction of thrombin with chromogenic substrate S2238 was determined in the presence of increasing concentrations of either unfused (HV1, top graph) or fused hirudin (HLA, bottom graph). Results shown are from one paired experiment that is representative of a total of three.

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