High-performance liquid chromatographic method for the simultaneous purification of cathepsins B, H and L from human liver

A high-performance liquid chromatographic procedure for the isolation of the three cysteine proteinases, namely cathepsins B, H and L, is described. The method is based on the following four steps. (1) A classical AcA 44 gel permeation separation with a 30–70% ammonium sulphate fraction from the hum...

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Published inJournal of chromatography. Biomedical applications Vol. 568; no. 1; pp. 55 - 68
Main Authors Dalet-Fumeron, Véronique, Guinec, Nathalie, Pagano, Maurice
Format Journal Article
LanguageEnglish
Published Amsterdam Elsevier B.V 17.07.1991
Elsevier
Subjects
Analytical, structural and metabolic biochemistry
Biological and medical sciences
Enzymes and enzyme inhibitors
Fundamental and applied biological sciences. Psychology
General aspects, investigation methods
Human
Separation method
Cathepsin L
Enzyme
Cathepsin H
Liver
Cathepsin B
HPLC chromatography
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Summary:A high-performance liquid chromatographic procedure for the isolation of the three cysteine proteinases, namely cathepsins B, H and L, is described. The method is based on the following four steps. (1) A classical AcA 44 gel permeation separation with a 30–70% ammonium sulphate fraction from the human liver homogenate is used to remove the non-enzymic high-molecular-mass components. (2) Preparative cation-exchange chromatography on a CM-SW TSK column can separate the three proteinases. (3) An anion-exchange step on a semi-preparative DEAE-SW TSK column for the cathepsin H fraction is used to remove a small amount of cathepsins B and L activities. (4) The three separated enzymes are purified on an analytical TSK gel 2000 SW column. The purity of each enzyme is assessed by sodium dodecyl sulphate polyacrylamide gel electrophoresis and electrofocusing on polyacrylamide gels. To check the activities of the purified proteinases, the kinetic constants [Michaelis constant ( K M) and catalytic constant ( K cat)] and the ratio K cat/ K M against the fluorigenic substrates Arg-NH-Mec, Z-Arg-Arg-NH-Mec and Z-Phe-Arg-NH-Mec after active-site titration using E-64, were determined. Z-Phe-Phe-CNH 2 was also used as a specific inhibitor of cathepsin L. This method requires only 6 g of human liver, and gives a high yield of the three lysosomal cysteine-proteinases: thus, about 150 μg of cathepsin B and 50 μg each of cathepsins L and H are obtained in a single run.
ISSN:0378-4347
DOI:10.1016/0378-4347(91)80340-I