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Preparation of Highly Purified Prothrombin Complex
Bovine prothrombin, an α 2 -glycoprotein clotting factor of plasma, has been isolated in high degree of purity in crystalline form as the barium glycoprotein product of interaction. Chemical determinations made on the product showed the following composition, in percentage of the dry weight: protei...
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| Published in: | The Journal of biological chemistry 1968-08, Vol.243 (15), p.4151-4167 |
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| Main Authors: | , , |
| Format: | Article |
| Language: | English |
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| Online Access: | Get full text |
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| Summary: | Bovine prothrombin, an α 2 -glycoprotein clotting factor of plasma, has been isolated in high degree of purity in crystalline form as the barium glycoprotein
product of interaction. Chemical determinations made on the product showed the following composition, in percentage of the
dry weight: protein, 21.5%; barium, 32%; and citrate, 8.9%. That the crystals represent a true prothrombin-metal complex has
been established by control studies, x-ray diffraction pattern, chemical composition, and recrystallization. The product showed
constant solubility characteristics.
Extensive physical and chemical studies of the barium-free protein are presented. Further purification was achieved by gel
filtration on Sephadex G-100. The peak fractions evidenced prothrombin activity of 3000 "Iowa" units (Seegers, W. H., Prothrombin,
Harvard University Press, Cambridge, Massachusetts, 1962, p. 420) per mg (corresponding to a 600-fold purification), as well
as appreciable Factors VII, IX, and X coagulant activities. This product is designated "prothrombin complex," in accordance
with the nomenclature used by other investigators. The preparation was homogeneous by sedimentation velocity pattern, sedimentation
equilibrium analysis, and gel filtration. Despite these indications of homogeneity, physical heterogeneity was shown by immuno-
and disc electrophoresis. The multiple coagulant activities and protein subcomponents were found to be homogeneous with respect
to molecular weight (70,477 ± 2,789), determined by sedimentation equilibrium in a dissociating solvent consisting of 6 m guanidine hydrochloride and 0.5% mercaptoethanol, and also with respect to Stokes radius. Physical constants, determined
in various systems, include diffusion constant, sedimentation coefficient, frictional ratio, isoelectric point, isoionic point,
electrophoretic mobility, and extinction coefficient. Physical data failed to show evidence of dissociation into subunits
or fragmentation by dilution to below 0.1% protein or by prolonged exposure to a dissociating solvent. The latter observation
suggests that the reduction in sedimentation constant noted in high ionic strength solvents in this study, and by other observers,
is probably attributable to changes in shape and hydration of the kinetic unit. The product was also shown to undergo rapid,
reversible association in solvents of low ionic strength (T/2 = 0.15).
DEAE-Sephadex chromatography resulted in partial activation of the prothrombin complex, an |
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| ISSN: | 0021-9258 1083-351X |
| DOI: | 10.1016/S0021-9258(18)93292-8 |