The Interaction Between Xanthine Oxidase and Its Antibody*

SummaryRabbits inoculated with purified Clostridiam histolyticum collagenase (Clostridiopeptidase A (E.C. 3.44.19) formed precipitating and enzyme activity inhibiting antibodies.The inhibiting effect of immune 7-globulin and of the immune Fab fragment depends on the antibody to enzyme ratio, on the time of preincubation between these two components, and on the presence of Ca 2 + during preincubation.Ca 2 + appears to be necessary to the formation of the collagenase-anticollagenase antibody complex and implicitly to the inhibition of collagenase activity by the antibody.Neither the high molecular substrate collagen, nor the small molecular substrate CBC-hexapeptide protect the collagenase activity against the inhibiting effect of the anticollagenase antibody.The present paper deals with some immunological properties of Clostridium histolyticum collagenase (Clostridiopeptidase A (EC. 3.44.19), few indications of which were found in literature (I, 2).A purification procedure and some chemical properties of this enzyme were reported in two previous papers (3, 4). Materials and MethodsCollagen was supplied by NBCo Laboratories; carbobenzoxy-glycyl-L-prolyl-glycyl-glycyl-L-prolyl- Dr. W. Junk b.v. Publishers -The Hague, The NetherlandsL-alanine 1 and the tripeptide glycyl-L-prolyl-L-alanyl were supplied by Mann Research Laboratories; Bio Gel P-300 and P-60 by Bio-Rad Laboratories; Sephadex G-200 by Pharmacia Uppsala; and bovine serum albumin (twice crystallized) by NBCo Laboratories. All other chemicals were analytical-grade products. MethodsProtein was determined by the method of LOWRY, as modified by MILLER (5), with bovine serum albumin used in plotting the standard curve. Collagenase assayEnzyme activity was determined by using the highmolecular undegraded collagen as a substrate, as well as the small molecular CBZ-hexapeptide substrate. With collagen as a substrate the method of Leach (6) was appliëd, and with CBZ-hexapeptide as a substrate the method of GRASS~AN and NORDWlG 7. Both methods were adapted to our experimental conditions (3,4). When collagen was used as a substrate a calcium-containing buffer, i.e. 0.I M Na-Veronal-10 -3 M Ca-acetate, pH 7.2, was added to the system to start collagenase activity. After an incubation of 1 hr at 37 ° the mixture was inactivated with ethanol. The precipitate forrned was discarded by centrifugation. Hydroxyproline (HyP) was determined with the 1 Abbreviation used: Carbobenzoxy-glycyl-L-prolyl-glycylglycyl-L-prolyl-L-alanine = CBZ-hexapeptide.

show abstract

The Interaction Between Xanthine Oxidase and Its Antibody*

Cited by 12 publications

References 7 publications

Radiometric Methods of Enzyme Assay

Radiometric Methods of Enzyme Assay

Enzymprotein als Antigen Immunologische Studien an Lactatdehydrogenasen

Immunoenzymology of clostridium histolyticum collagenase

Contact Info

Product

Resources

About