Characterization of human catalase by isoelectric focusing in presence of urea
- PMID: 2289463
- DOI: 10.1002/elps.1150110810
Characterization of human catalase by isoelectric focusing in presence of urea
Abstract
Human catalase from erythrocytes and liver were analyzed by polyacrylamide gel isoelectric focusing in presence and absence of urea using two different pH gradients, namely pH 6-8 and pH 6.7-7.7. In presence of urea, human catalase focused in the pH range 6.75-7.0, slightly anodal to that of hemoglobin A. In narrow pH gradients, human erythrocyte catalase was microheterogeneous. Neuraminidase from different sources and peptide-N-glycosidase F were applied to investigate the presence of sialic acid and/or carbohydrate chains in human catalase. A shift in the focusing pattern of both erythrocyte and liver catalase towards the anode was observed after treatment with one of the commercially available neuroaminidase preparations. This unusual result could be related to a contaminating protease since no effect was observed when the catalases were treated in presence of a serine protease inhibitor. In contrast, bovine liver and Macaca erythrocyte catalase did not display any detectable change in their focusing patterns after treatment with any of the neuraminidase preparations.
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