R. Verbruggen scite author profile

A method was developed which involved electroimmunoassay and crossed immunoelectrophoresis of subtilopeptidase A (EC 3.4.21.14). Initial trials with unfractionated antiserum were not successful and interaction of the enzyme with non-immunoglobulin serum components were shown to be the cause of the failures. Quantitative immunoelectrophoresis was possible when purified immunoglobulins were used. A pH of6.5 (lower than the usual pH8.6) was necessary to obtain a proper baseline definition. Subtilopeptidase A was confirmed as a multiple isoenzyme system. Qualitative inter-batch variations were detected. Di-isopropyl phosphorofluoridate inhibition altered the electrophoretic pattern, but no loss of antigenic determinants was observed.

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Demonstration of α2-macroglobulin in cultured fibroblasts, using crossed immunoelectrophoresis

Leuven

Verbruggen

Cassiman

et al. 1977

Experimental Cell Research

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Analysis of murine C-type virus structural proteins by rocket and crossed immunoelectrophoresis

Georgiades

Billiau

Verbruggen

et al. 1977

Journal of Immunological Methods

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R. Verbruggen

Quantitative Immunoelectrophoretic Methods: A Literature Survey

On the heterogeneity and the autodigestion of subtilisin “Carlsberg” as studied by agarose electrophoresis and grabar-williams immunoelectrophoresis

Subtilopeptidase A isoenzyme system. Interaction with serum components and its importance for quantitative immunoelectrophoresis

Demonstration of α2-macroglobulin in cultured fibroblasts, using crossed immunoelectrophoresis

Analysis of murine C-type virus structural proteins by rocket and crossed immunoelectrophoresis

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