Abstract

A. Yarleque, S. Campos, E. Escobar, F. Lazo, N. Sanchez, S. Hyslop, N. A. Marsh, P. J. Butterworth and R. G. Price. Isolation and characterization of a fibrinogen-clotting enzyme from venom of the snake Lachesis muta muta(Peruvian bushmaster). Toxicon 27, 1189–1197, 1989.—A fibrinogen-clotting enzyme from the venom of the Peruvian bushmaster snake was purified to homogeneity by gel filtration on Sephadex G-100 followed by DEAE-cellulose ion-exchange chromatography using a linear ionic strength gradient with NaCl. The specific activity of the enzyme was 866 NIH U/mg, representing a 55-fold purification, with a recovery of 45%. The amino acid composition was Asx 30, Thr 14, Ser 15, Glx 33, Pro 23, Gly 22, Ala 15, Val 22, Cys 18, Met 3, Ile 18, Leu 23, Tyr 2, Phe 13, His 8, Lys 11, Arg 11. The total carbohydrate content was 13.4%, comprised of 3.4% hexose, 8.7% hexosamine and 1.3% sialic acid. The enzyme was active against the synthetic amide substrate α- N-benzoyl- dl-arginine- p-nitroanilide (BAPNA) and against the ester substrates α- N-benzoyl- l-arginine ethyl ester (BAEE) and tosyl- l-arginine methyl ester (TAME). Kinetic parameters for TAME esterolysis were: V max , 135 μmoles/min/mg and K m , 2.5 × 10 −4M. The pH optimum was 8.0. V max for BAPNA amidolysis was 0.363 μmoles/min/mg and K m , 7.5 × 10 −5M. Enzyme activity was reduced by diethylpyrocarbonate and by photo-oxidation, suggesting that the enzyme is a serine protease with a histidine residue involved in the active site. The enzyme released fibrinopeptide A rapidly from purified human fibrinogen and fibrinopeptide B more slowly. Factor XIII was not activated and the clotting activity was not inhibited by heparin. A dose of 50 μg/kg brought about defibrinogenation in anaesthetized rats but rabbits were unaffected. A dose of 80 μg/kg defibrinogenated conscious rats after 5 hr. There were no hypotensive or haemorrhagic effects.

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